Chlamydia pneumoniae polynucleotides and uses thereof

Information

  • Patent Grant
  • 6559294
  • Patent Number
    6,559,294
  • Date Filed
    Monday, November 23, 1998
    26 years ago
  • Date Issued
    Tuesday, May 6, 2003
    22 years ago
Abstract
The subject of the invention is the genomic sequence and the nucleotide sequences encoding polypeptides of Chlamydia pneumoniae, such as cellular envelope polypeptides, which are secreted or specific, or which are involved in metabolism, in the replication process or in virulence, polypeptides encoded by such sequences, as well as vectors including the said sequences and cells or animals transformed with these vectors. The invention also relates to transcriptional gene products of the Chlamydia pneumoniae genome, such as, for example, antisense and ribozyme molecules, which can be used to control growth of the microorganism. The invention also relates to methods of detecting these nucleic acids or polypeptides and kits for diagnosing Chlamydia pneumoniae infection. The invention also relates to a method of selecting compounds capable of modulating bacterial infection and a method for the biosynthesis or biodegradation of molecules of interest using the said nucleotide sequences or the said polypeptides. The invention finally comprises, pharmaceutical, in particular vaccine, compositions for the prevention and/or treatment of bacterial, in particular Chlamydia pneumoniae, infections.
Description




The Sequence Listing for this application is on duplicate compact discs labeled “Copy 1” and “Copy 2.” Copy 1 and 2 each contain only one file named “seqlist-28July2001.txt” which was created on Jul. 30, 2001, and is 5,284 KB. The entire contents of each of the computer discs are incorporated herein by reference in their entireties.




The subject of the invention is the genomic sequence and the nucleotide sequences encoding polypeptides of


Chlamydia pneumoniae,


such as cellular envelope polypeptides, which are secreted or specific, or which are involved in metabolism, in the replication process or in virulence, polypeptides encoded by such sequences, as well as vectors including the said sequences and cells or animals transformed with these vectors. The invention also relates to transcriptional gene products of the


Chlamydia pneumoniae


genome, such as, for example, antisense and ribozyme molecules, which can be used to control growth of the microorganism. The invention also relates to methods of detecting these nucleic acids or polypeptides and kits for diagnosing


Chlamydia pneumoniae


infection. The invention also relates to a method of selecting compounds capable of modulating bacterial infection and a method for the biosynthesis or biodegradation of molecules of interest using the said nucleotide sequences or the said polypeptides. The invention finally comprises, pharmaceutical, in particular vaccine, compositions for the prevention and/or treatment of bacterial, in particular


Chlamydia pneumoniae,


infections.




Comparative analysis of the sequence of the gene encoding the ribosomal 16S RNA has been widely used for the phylogenetic study of prokaryotes. This approach has made it possible to classify the Chlamydiae among the eubacteria, among which they represent a well-isolated group, with, nevertheless, a very weak link with the planctomyces. The Chlamydiae thus exhibit some unique characteristics within the eubacteria, in particular their development cycle and the structure of their membranes. They have a unique two-phase cell cycle: the elementary body, a small extracellular form, attaches to the host and is phagocytosed; in the phagosome, it is converted to the replicative intracellular form, the reticulate body. The Chlamydiae are obligate intracellular bacteria which multiply in eukaryotic cells at the expense of their energy reserves and nucleotide pools; they are responsible for a wide variety of diseases in mammals and birds. The Chlamydiae are the only members of the order Chlamydiales, of the family Chlamydiaceae and of the genus Chlamydia. Within the genus Chlamydia, four species are currently described:


Chlamydia trachomatis, Chlamydia psittaci, Chlamydia pneumoniae


and


Chlamydia pecorum.


These bacteria are grouped together and share biological and biochemical properties. Among them, only the first three infect humans,


Chlamydia pecorum


being a pathogen of ruminants.




The species


Chlamydia psittaci


infects many animals, in particular birds, and is transmissible to humans. It is responsible for atypical pneumonia, for hepatic and renal dysfunction, for endocarditis and for conjunctivitis.




The species


Chlamydia trachomatis


is the best characterized. Besides a murine strain, it is divided into two groups which are distinguishable by the nature of the diseases for which they are responsible: trachoma, genital attack and venereal lymphogranulomatosis. There are fifteen human serotypes of


Chlamydia trachomatis


(A, K) and LGV (L1, L2, L3). Strains A to C are mainly found in eye infections, whereas strains D to K and LGV are essentially responsible for genital entry infections. It should be mentioned that the LGV strains are responsible for systemic diseases. Historically, it was in 1906 that Halberstaeder and on Provaseck discovered, in trachoma patients, the presence of inclusions in the cytoplasm of the cells derived from conjunctival scrapings. In 1940, Rake and Jones described these same inclusions in certain cells obtained by puncturing the ganglia from a patient suffering from venereal granulomatosis. Characterization of the


Chlamydia trachomatis


microorganism was only successfully carried out in 1957, after a series of isolations in cell cultures.




It was in 1983 that


Chlamydia pneumoniae


was recognized as a human pathogen (Grayston J T et al., 1986); since then, special attention has been paid to this bacterium and it is estimated (Gaydos C A et al., 1994) that 10% of pneumonias, and 5% of bronchitides and sinusites are attributable to


Chlamydia pneumoniae


(Aldous M B et al., 1992). More recently, the association of this bacterium with the pathogenesis of asthmatic disease and of cardiovascular impairments is increasingly of interest.




Serological studies have made it possible to observe that


Chlamydia pneumoniae


infection is common in children between 5 and 16 years of age. Before this age, it is rare to find antibodies; the increase in the number of individuals carrying antibodies is then correlated with age up to 20 years. Accordingly, 50% of adults are carriers of antibodies, it being possible for this prevalence to be as high as 75%. These figures are all the more striking since a first infection induces antibody levels of which the persistence over time is limited to 3 or at most 5 years, which suggests frequent reinfection during the entire lifespan. The annual seroconversion rate is about 8% between 8 and 12 years and about 6% between 12 and 16 years (Haidl et al., 1994). Before the age of 15 years, the seroprevalence of the disease is identical between both sexes. After this age, men are more frequently infected than women; this is true in all regions worldwide where such studies have been carried out.




These infections are geographically highly widespread, as shown by numerous studies carried out throughout the world (Kanamoto Y et al., 1991; Tong C Y et al., 1993). Developed countries of the north such as Canada, Denmark and Norway have the lowest infection rates; conversely, the highest prevalence rates are found in the less developed countries of tropical regions where the infection may occur before the age of 5 years.




Humans are the only known reservoir for


Chlamydia pneumoniae


and it is probable that the infection is caused by direct transmission, respiratory secretions probably being responsible for this low-yield transmission (Aldous et al., 1992). The chain of transmission may also appear to be indirect (Kleemola M et al., 1988), suggesting that the infection is caused by an effective transmission, but also that asymptomatic carriers exist, which could explain the high prevalence of the disease. Other studies (Mordhorst C H et al., 1992) show that the efficiency of the transmission varies according to the individuals and list cases of infection affecting all or the majority of members of one family or of a group of families. The period of incubation is several weeks, significantly longer in this regard than that of many other respiratory pathogenic agents. Although under conditions of high relative humidity the infectivity of


Chlamydia pneumoniae


in the open air decreases rapidly, suggesting a direct mode of transmission under these conditions, it is probable that the transmission occurs in some cases indirectly since the microorganism can survive for up to 30 hours in a hostile environment (Falsey et al., 1993).




Clinical manifestations due to


Chlamydia pneumoniae


are essentially respiratory diseases. Pneumonia and bronchitis are the most frequent because they are clinically patent: since etiological diagnosis is evoked in this case, the infectious agent is identified. The asymptomatic diseases are probably numerous (Grayston J T et al., 1992; Grayston J T et al., 1986; Thom D H et al., 1990). The disease then progresses via bronchitis or pneumonia; fever is absent at the time of examination but is sometimes reported by the patient. The degree of seriousness of the disease is variable and in hospitalized patients, it is common to observe pleural effusion; a generalized infection may also be observed and, in severe cases, anatomicopathological examination shows


Chlamydia pneumoniae


diseases.




Other syndromes such as sinusitis (Hashiguchi K et al., 1992), purulent otitis media (Ogawa H et al., 1992), or pharyngitis (Huovinen P et al., 1989) have been described, as well as infections with respiratory impairments similar to asthma (Hahn D L et al., 1991).


Chlamydia pneumoniae


has also been associated with sarcoidosis, with erythema nodosum (Sundelof et al., 1993) and one case of Guillain-Barrésyndrome has even been described (Haidl et al., 1992). The involvement of


Chlamydia pneumoniae


in Reiter's syndrome has also been evaluated (Braun J et al., 1994).




The association of


Chlamydia pneumoniae


with coronary diseases and with myocardial infarction was first suspected from the observation of the high antibody level in 71% of patients having a heart disease (Shor A et al., 1992; Kuo C C et al., 1993; Puolakkainen M et al., 1993; Thomas G N et al., 1997). Studies carried out in several countries have shown similar results in patients with atheromatous impairments (Shor A et al., 1992; Kuo C C et al., 1993; Puolakkainen M et al., 1993; Grayston J T et al., 1996; Casas-Ciria J et al., 1996; Thomas G N et al., 1997; Jackson L A et al., 1997) and in patients with carotid impairments. Anatomicopathological and microbiological studies have detected


Chlamydia pneumoniae


in the vessels. The electron microscope has made it possible to visualize the bacterium (Ladany S et al., 1989), which has in fact been demonstrated by other techniques such as PCR (Campbell L A et al., 1992; Kuo C C et al., 1993; Kuo C C et al., 1988). It also appears that the bacterium is more frequently found in old atheromatous lesions. Other studies carried out on young subjects from 15 to 35 years have given the opportunity to study the coronary arteries of people without atherosclerosis, this observation not being possible in older subjects (the onset of the atheromatous disease is early). In these young subjects, the PCR studies did not find


Chlamydia pneumoniae


in subjects free of atheromatous disease, but revealed the presence of


Chlamydia pneumoniae


in two of the eleven subjects who showed early lesions and in six of the seven subjects who developed atheroma plaques. These studies therefore show that the atheroma plaque is very strongly correlated with the presence of


Chlamydia pneumoniae,


but the role played by the bacterium in vascular pathology is not yet defined.




The data relating to controlled clinical studies analysing the effect of treatments in


Chlamydia pneumoniae


infections are limited in number. Unlike penicillin, ampicillin or the sulphamides, erythromycin, tetracycline or doxycycline show an antibiotic activity in vitro against


Chlamydia pneumoniae.


However, a treatment at high doses should be continued for several weeks in order to avoid a recurrence of the infection. Accordingly, the use of two new macrolides, clarithromycin and azithromycin, whose diffusion, bioavailability and half-life allow shorter and better tolerated cures, is nowadays preferred. In the absence of definitive proof based on the results of clinical studies, an effective, without recurrences, and well-tolerated treatment of


Chlamydia pneumoniae


infections therefore remains desirable.




An even more important need up until now relates to a specific and sensitive diagnosis, which can be carried out conveniently and rapidly, allowing early screening for the infection. Methods based on


Chlamydia pneumoniae


culture are slow and require a considerable know-how because of the difficulty involved in the collection, preservation and storage of the strain under appropriate conditions. Methods based on antigen detection (EIA, DFA) or on nucleic acid amplification (PCR) provide tests which are more suitable for laboratory practice. A reliable, sensitive and convenient test, which allows distinction between serogroups and a fortiori between


Chlamydia pneumoniae


species is therefore highly desirable.




This is all the more important since the symptoms of


Chlamydia pneumoniae


infection appear slowly, since all the pathologies associated with these infections have not yet been identified, and since, as has been mentioned above, an association is suspected between these infections and serious chronic infections, asthma or atherosclerosis.




No vaccine is yet available against


Chlamydia pneumoniae:


this is due to the labile nature of the antigens specific to the strain, which has so far prevented their specific identification.




Although the number of studies and of animal models developed is high, the antigens used have not induced sufficient protective immunity to lead to the development of human vaccines. In the case of


Chlamydia pneumoniae,


the role of the immune defense in the physiology and pathology of the disease should probably be understood in order to develop satisfactory vaccines.




More detailed information relating to the biology of these strains, their interactions with their hosts, the associated phenomena of infectivity and those of escaping the immune defenses of the host in particular, and finally their involvement in the development of the these associated pathologies, will allow a better understanding of these mechanisms. In the light of the preceding text which shows in particular the limitations of the means of controlling


Chlamydia pneumoniae


infection, it is therefore at present essential, on the one hand, to develop molecular tools, in particular from a better genetic knowledge of


Chlamydia pneumoniae,


but also to develop new preventive and therapeutic treatments, new diagnostic methods and new vaccine strategies which are specific, effective and tolerated. This is precisely the object of the present invention.




The subject of the present invention is the nucleotide sequence having the sequence SEQ ID No. 1 of the


Chlamydia pneumoniae


genome. However, the invention is not limited to SEQ ID No. 1, but encompasses genomes and nucleotides encoding polypeptides of strain variants, polymorphisms, allelic variants, and mutants.




Thus, the subject of the present invention encompasses nucleotide sequences characterized in that they are chosen from:




a) the nucleotide sequence of SEQ ID No. 1, a nucleotide sequence exhibiting at least 99.9% identity with the sequence SEQ ID No. 1, the nucleotide sequence of the genomic DNA contained within ATCC Deposit No. VR2634, the nucleotide sequence of a clone insert within ATCC Deposit No. 207000: 207001 and 207002;




b) a nucleotide sequence homologous to the sequence SEQ ID No. 1;




c) a polynucleotide sequence that hybridizes to the nucleotide sequence of a) under conditions of high or intermediate stringency as described below:




(i) By way of example and not limitation, procedures using conditions of high stringency are as follows: Prehybridization of filters containing DNA is carried out for 8 h to overnight at 65° C. in buffer composed of 6×SSC, 50 mM Tris-HCl (pH 7.5), 1 mM EDTA, 0.02% PVP, 0.02% Ficoll, 0.02% BSA, and 500 μg/ml denatured salmon sperm DNA. Filters are hybridized for 48 h at 65° C., the preferred hybridization temperature, in prehybridization mixture containing 100 μg/ml denatured salmon sperm DNA and 5-20×10


6


cpm of


32


P-labeled probe. Alternatively, the hybridization step can be performed at 65° C. in the presence of SSC buffer, 1×SSC corresponding to 0.15M NaCl and 0.05 M Na citrate. Subsequently, filter washes can be done at 37° C. for 1 h in a solution containing 2×SSC, 0.01% PVP, 0.01% Ficoll, and 0.01% BSA, followed by a wash in 0.1×SSC at 50° C. for 45 min. Alternatively, filter washes can be performed in a solution containing 2×SSC and 0.1% SDS, or 0.5×SSC and 0.1% SDS, or 0.1×SSC and 0.1% SDS at 68° C. for 15 minute intervals. Following the wash steps, the hybridized probes are detectable by autoradiography. Other conditions of high stringency which may be used are well known in the art and as cited in Sambrook et al., 1989, Molecular Cloning, A Laboratory Manual, Second Edition, Cold Spring Harbor Press, N.Y., pp. 9.47-9.57; and Ausubel et al., 1989, Current Protocols in Molecular Biology, Green Publishing Associates and Wiley Interscience, N.Y. are incorporated herein in their entirety.




(ii) By way of example and not limitation, procedures using conditions of intermediate stringency are as follows: Filters containing DNA are prehybridized, and then hybridized at a temperature of 60° C. in the presence of a 5×SSC buffer and labeled probe. Subsequently, filters washes are performed in a solution containing 2×SSC at 50° C. and the hybridized probes are detectable by autoradiography. Other conditions of intermediate stringency which may be used are well known in the art and as cited in Sambrook et al., 1989, Molecular Cloning, A Laboratory Manual, Second Edition, Cold Spring Harbor Press, N.Y., pp. 9.47-9.57; and Ausubel et al., 1989, Current Protocols in Molecular Biology, Green Publishing Associates and Wiley Interscience, N.Y. are incorporated herein in their entirety.




d) a nucleotide sequence complementary to the sequence SEQ ID No. 1 or complementary to a nucleotide sequence as defined in a), b) or c) and a nucleotide sequence of their corresponding RNA;




e) a nucleotide sequence of a representative fragment of the sequence SEQ ID No. 1, or of a representative fragment of the nucleotide sequence as defined in a), b), c) or d);




f) a nucleotide sequence comprising a sequence as defined in a), b), c), d) or e);




g) a nucleotide sequence capable of being obtained from a nucleotide sequence as defined in a), b), c), d), e) or f); and




h) a modified nucleotide sequence of a nucleotide sequence as defined in a), b), c), d), e), f) or g).




Nucleotide sequence, polynucleotide or nucleic acid are understood to mean, according to the present invention, either a double-stranded DNA, a single-stranded DNA or products of transcription of the said DNAs.




It should be understood that the present invention does not relate to the genomic nucleotide sequences of


Chlamydia pneumoniae


taken in their natural environment, that is to say in the natural state. They are sequences which may have been isolated, purified or partially purified, by separation methods such as, for example, ion-exchange chromatography, molecular size exclusion chromatography or affinity chromatography, or alternatively fractionation techniques based on solubility in various solvents, or by genetic engineering methods such as amplification, cloning or subcloning, it being possible for the sequences of the invention to be carried by vectors.




The nucleotide sequence SEQ ID No. 1 was obtained by sequencing the


Chlamydia pneumoniae


genome by the method of directed sequencing after fluorescent automated sequencing of the inserts of clones and assembling of these sequences of nucleotide fragments (inserts) by means of softwares (cf. Examples). In spite of the high precision of the sequence SEQ ID No. 1, it is possible that it does not perfectly, 100% represent the nucleotide sequence of the


Chlamydia pneumoniae


genome and that a few rare sequencing errors or uncertainties still remain in the sequence SEQ ID No. 1. In the present invention, the presence of an uncertainty for an amino acid is designated by “Xaa” and that for a nucleotide is designated by “N” in the sequence listing below. These few rare errors or uncertainties could be easily detected and corrected by persons skilled in the art using the entire chromosome and/or its representative fragments according to the invention and standard amplification, cloning and sequencing methods, it being possible for the sequences obtained to be easily compared, in particular by means of a computer software and using computer-readable media for recording the sequences according to the invention as described, for example, below. After correcting these possible rare errors or uncertainties, the corrected nucleotide sequence obtained would still exhibit at least 99.9% identity with the sequence SEQ ID No. 1. Such rare sequencing uncertainties are not present within the DNA contained within ATCC Deposit No. VR2634, 207000, 207001 or 207002, and whatever rare sequence uncertainties that exist within SEQ ID No. 1 can routinely be corrected utilizing the DNA of the ATCC deposits.




Homologous nucleotide sequence for the purposes of the present invention is understood to mean a nucleotide sequence having a percentage identity with the bases of the nucleotide sequence SEQ ID No. 1 of at least 80%, preferably 90% and 95%, this percentage being purely statistical and it being possible for the differences between the two nucleotide sequences to be distributed randomly and over their entire length. The said homologous sequences exhibiting a percentage identity with the bases of the nucleotide sequence SEQ ID No. 1 of at least 80%, preferably 90% and 95%, may comprise, for example, the sequences corresponding to the genomic sequence or to the sequences of its representative fragments of a bacterium belonging to the Chlamydia family, including the species


Chlamydia trachomatis, Chlamydia psittaci


and


Chlamydia pecorum


mentioned above, as well as the sequences corresponding to the genomic sequence or to the sequences of its representative fragments of a bacterium belonging to the variants of the species


Chlamydia pneumoniae.


In the present invention, the terms family and genus are mutually interchangeable, the terms variant, serotype, strain and subspecies are also mutually interchangeable. These homologous sequences may thus correspond to variations linked to mutations within the same species or between species and may correspond in particular to truncations, substitutions, deletions and/or additions of at least one nucleotide. The said homologous sequences may also correspond to variations linked to the degeneracy of the genetic code or to a bias in the genetic code which is specific to the family, to the species or to the variant and which are likely to be present in Chlamydia.




Protein and/or nucleic acid sequence homologies may be evaluated using any of the variety of sequence comparison algorithms and programs known in the art. Such algorithms and programs include, but are by no means limited to, TBLASTN, BLASTP, FASTA, TFASTA, and CLUSTALW (Pearson and Lipman, 1988,


Proc. Natl. Acad. Sci. USA


85(8):2444-2448; Altschul et al., 1990,


J. Mol. Biol.


215(3):403-410; Thompson et al., 1994,


Nucleic Acids Res.


22(2):4673-4680; Higgins et al., 1996,


Methods Enzymol.


266:383-402; Altschul et al., 1990,


J. Mol. Biol.


215(3):403-410; Altschul et al., 1993,


Nature Genetics


3:266-272).




In a particularly preferred embodiment, protein and nucleic acid sequence homologies are evaluated using the Basic Local Alignment Search Tool (“BLAST”) which is well known in the art (see, e.g., Karlin and Altschul, 1990,


Proc. Natl. Acad. Sci. USA


87:2267-2268; Altschul et al., 1990,


J. Mol. Biol.


215:403-410; Altschul et al., 1993,


Nature Genetics


3:266-272; Altschul et al., 1997,


Nuc. Acids Res.


25:3389-3402). In particular, five specific BLAST programs are used to perform the following task:




(1) BLASTP and BLAST3 compare an amino acid query sequence against a protein sequence database;




(2) BLASTN compares a nucleotide query sequence against a nucleotide sequence database;




(3) BLASTX compares the six-frame conceptual translation products of a query nucleotide sequence (both strands) against a protein sequence database;




(4) TBLASTN compares a query protein sequence against a nucleotide sequence database translated in all six reading frames (both strands); and




(5) TBLASTX compares the six-frame translations of a nucleotide query sequence against the six-frame translations of a nucleotide sequence database.




The BLAST programs identify homologous sequences by identifying similar segments, which are referred to herein as “high-scoring segment pairs,” between a query amino or nucleic acid sequence and a test sequence which is preferably obtained from a protein or nucleic acid sequence database. High-scoring segment pairs are preferably identified (i.e., aligned) by means of a scoring matrix, many of which are known in the art. Preferably, the scoring matrix used is the BLOSUM62 matrix (Gonnet et al., 1992,


Science


256:1443-1445; Henikoff and Henikoff, 1993,


Proteins


17:49-61). Less preferably, the PAM or PAM250 matrices may also be used (see, e.g., Schwartz and Dayhoff, eds., 1978,


Matrices for Detecting Distance Relationships: Atlas of Protein Sequence and Structure,


Washington: National Biomedical Research Foundation).




The BLAST programs evaluate the statistical significance of all high-scoring segment pairs identified, and preferably selects those segments which satisfy a user-specified threshold of significance, such as a user-specified percent homology. Preferably, the statistical significance of a high-scoring segment pair is evaluated using the statistical significance formula of Karlin (see, e.g., Karlin and Altschul, 1990,


Proc. Natl. Acad. Sci. USA


87:2267-2268).




Nucleotide sequence complementary to a sequence of the invention is understood to mean any DNA whose nucleotides are complementary to those of the sequence of the invention, and whose orientation is reversed (antiparallel sequence).




The present invention further comprises fragments of the sequences of a) through h), above. Representative fragments of the sequences according to the invention will be understood to mean any nucleotide fragment having at least 8 successive nucleotides, preferably at least 12 successive nucleotides, and still more preferably at least 15 or at least 20 successive nucleotides of the sequence from which it is derived. It is understood that such fragments refer only to portions of SEQ ID No. 1 that are not currently listed in a publicly available database.




Among these representative fragments, those capable of hybridizing under stringent conditions with a nucleotide sequence according to the invention are preferred. Hybridization under stringent conditions means that the temperature and ionic strength conditions are chosen such that they allow hybridization to be maintained between two complementary DNA fragments.




By way of illustration, high stringency conditions for the hybridization step for the purposes of defining the nucleotide fragments described above, are advantageously the following.




The hybridization is carried out at a preferred temperature of 65° C. in the presence of SSC buffer, 1×SSC corresponding to 0.15 M NaCl and 0.05 M Na citrate. The washing steps may be, for example, the following: 2×SSC, 0.1% SDS at room temperature followed by three washes with 1×SSC, 0.1% SDS; 0.5×SSC, 0.1% SDS; 0.1×SSC, 0.1% SDS at 68° C. for 15 minutes.




Intermediate stringency conditions, using, for example, a temperature of 60° C. in the presence of a 5×SSC buffer, or of low stringency, for example a temperature of 50° C. in the presence of a 5×SSC buffer, respectively require a lower overall complementarity for the hybridization between the two sequences.




The stringent hybridization conditions described above for a polynucleotide of about 300 bases in size will be adapted by persons skilled in the art for larger- or smaller-sized oligonucleotides, according to the teaching of Sambrook et al., 1989.




Among the representative fragments according to the invention, those which can be used as primer or probe in methods which make it possible to obtain homologous sequences or their representative fragments according to the invention, or to reconstitute a genomic fragment found to be incomplete in the sequence SEQ ID No. 1 or carrying an error or an uncertainty, are also preferred, these methods, such as the polymerase chain reaction (PCR), cloning and sequencing of nucleic acid being well known to persons skilled in the art. These homologous nucleotide sequences corresponding to mutations or to inter- or intra-species variations, as well as the complete genomic sequence or one of its representative fragments capable of being reconstituted, of course form part of the invention.




Among the said representative fragments, those which can be used as primer or probe in methods allowing diagnosis of the presence of


Chlamydia pneumoniae


or one of its associated microorganisms as defined below are also preferred.




The representative fragments capable of modulating, regulating, inhibiting or inducing the expression of a gene of


Chlamydia pneumoniae


or one of its associated microorganisms, and/or capable of modulating the replication cycle of


Chlamydia pneumoniae


or one of its associated microorganisms in the host cell and/or organism, are also preferred. Replication cycle is intended to designate invasion, multiplication, intracellular localization, in particular retention in the vacuole and inhibition of the process of fusion to the lysosome, and propagation of


Chlamydia pneumoniae


or one of its associated microorganisms from host cells to host cells.




Among the said representative fragments, those corresponding to nucleotide sequences corresponding to open reading frames, called ORF sequences (ORF for open reading frame), and encoding polypeptides, such as for example, but without being limited thereto, the ORF sequences which will be later described, are finally preferred.




The representative fragments according to the invention may be obtained, for example, by specific amplification, such as PCR, or after digestion, with appropriate restriction enzymes, of nucleotide sequences according to the invention; these methods are in particular described in the manual by Sambrook et al., 1989. The said representative fragments may also be obtained by chemical synthesis when they are not too large in size and according to methods well known to persons skilled in the art. For example, such fragments can be obtained by isolating fragments of the genomic DNA of ATCC Deposit No. VR2634 or a clone insert present at this ATCC Deposit No. 207000: 207001 and 207002.




The representative fragments according to the invention may be used, for example, as primer, to reconstitute some of the said representative fragments, in particular those in which a portion of the sequence is likely to be missing or imperfect, by methods well known to persons skilled in the art such as amplification, cloning or sequencing techniques.




Modified nucleotide sequence will be understood to mean any nucleotide sequence obtained by mutagenesis according to techniques well known to persons skilled in the art, and exhibiting modifications in relation to the normal sequences, for example mutations in the regulatory and/or promoter sequences for the expression of a polypeptide, in particular leading to a modification of the level of expression of the said polypeptide or to a modulation of the replicative cycle.




Modified nucleotide sequence will also be understood to mean any nucleotide sequence encoding a modified polypeptide as defined below.




The subject of the present invention also includes


Chlamydia pneumoniae


nucleotide sequences characterized in that they are chosen from a nucleotide sequence of an open reading frame (ORF), that is, the ORF2 to ORF1297 sequences.




The ORF2 to ORF1297 nucleotide sequences are defined in Tables 1 and 2, infra, by their position on the sequence SEQ ID No. 1. For example, the ORF2 sequence is defined by the nucleotide sequence between the nucleotides at position 42 and 794 on the sequence SEQ ID No. 1, ends included. ORF2 to ORF1297 have been identified via homology analyses as well as via analyses of potential ORF start sites, as discussed in the examples below. It is to be understood that each identified ORF of the invention comprises a nucleotide sequence that spans the contiguous nucleotide sequence from the codon immediately 3′ to the stop codon of the preceding ORF and through the 5′ codon to the next stop codon of SEQ ID No.:1 in-frame to the ORF nucleotide sequence. Table 2, infra, lists the beginning, end and potential start site of each of ORFs 1-1297. In one embodiment, the ORF comprises the contiguous nucleotide sequence spanning from the potential ORF start site downstream (that is, 3′) to the ORF stop codon (or the ORF codon immediately adjacent to and upstream of the ORF stop codon). ORF2 to ORF1297 encode the polypeptides of SEQ ID No. 2 to SEQ ID No. 1291 and of SEQ ID No. 6844 to SEQ ID No. 6849, respectively.




Upon introduction of minor frameshifts, certain individual ORFs can comprise larger “combined” ORFs. A list of such putative “combined” ORFs is shown in Table 3, below. For example, a combined ORF can comprise ORF 25, ORF 26 and ORF 27, including intervening in-frame, nucleotide sequences. The order of ORFs (5′ to 3′), within each “combined” ORF is as listed. It is to be understood that when ORF2 to ORF1297 are referred to herein, such reference is also meant to include “combined” ORFs. Polypeptide sequences encoded by such “combined” ORFs are also part of the present invention.














TABLE 3













ORF 25, ORF 26, ORF 27;







ORF 28, ORF 29, ORF 30;







ORF 31, ORF 32;







ORF 33, ORF 35;







ORF 466, ORF 467;







ORF 468, ORF 469;







ORF 477, ORF 476, ORF 474;







ORF 480, ORF 482;







ORF 483, ORF 485, ORF 486, ORF 500;







ORF 503, ORF 504, ORF 505;







ORF 506, ORF 507;







ORF 1211, ORF 647;







ORF 1286, ORF 1039;







ORF 691, ORF 690;







ORF 105, ORF 106;







ORF 170, ORF 171; ORF 394, ORF 393;







ORF 453, ORF 452, ORF 451;







ORF 526, ORF 525;







ORF 757, ORF 756, ORF 755;







ORF 856, ORF 855;







CRF 958, ORF 957;







ORF 915, ORF 914, ORF 913;







ORF 543, ORF 544;







ORF 1266, ORF 380;







ORF 745, ORF 744;







ORF 777, ORF 776;







ORF 343, ORF 1297, and representative fragments.















Table 1 also depicts the results of homology searches that compared the sequences of the polypeptides encoded by each of the ORFs to sequences present in public published databases. It is understood that those polypeptides listed in Table 1 as exhibiting greater than about 95% identity to a polypeptide present in a publicly disclosed database are not considered part of the present invention; likewise in this embodiment, those nucleotide sequences encoding such polypeptides are not considered part of the invention. In another embodiment, it is understood that those polypeptides listed in Table 1 as exhibiting greater than about 99% identity to a polypeptide present in a publicly disclosed database are not considered part of the invention; likewise, in this embodiment, those nucleotide sequences encoding such polypeptides are not considered part of the invention.




The invention also relates to the nucleotide sequences characterized in that they comprise a nucleotide sequence chosen from:




a) an ORF2 to ORF1297, a “combined” ORF nucleotide sequence, the nucleotide sequence of the genomic DNA contained within ATCC Deposit No. VR2634 or the nucleotide sequence of a clone insert in ATCC Deposit No. 207000: 207001 and 207002 according to the invention;




b) a homologous nucleotide sequence exhibiting at least 80% identity across an entire ORF2 to ORF1297 nucleotide sequence according to the invention or as defined in a);




c) a polynucleotide sequence that hybridizes to ORF2 to ORF1297 under conditions of high or intermediate stringency as described below:




(i) By way of example and not limitation, procedures using conditions of high stringency are as follows: Prehybridization of filters containing DNA is carried out for 8 h to overnight at 65° C. in buffer composed of 6×SSC, 50 mM Tris-HCl (pH 7.5), 1 mM EDTA, 0.02% PVP, 0.02% Ficoll, 0.02% BSA, and 500 μg/ml denatured salmon sperm DNA. Filters are hybridized for 48 h at 65° C., the preferred hybridization temperature, in prehybridization mixture containing 100 μg/ml denatured salmon sperm DNA and 5-20×10


6


cpm of


32


P-labeled probe. Alternatively, the hybridization step can be performed at 65° C. in the presence of SSC buffer, 1×SSC corresponding to 0.15M NaCl and 0.05 M Na citrate. Subsequently, filter washes can be done at 37° C. for 1 h in a solution containing 2×SSC, 0.01% PVP, 0.01% Ficoll, and 0.01% BSA, followed by a wash in 0.1×SSC at 50° C. for 45 min. Alternatively, filter washes can be performed in a solution containing 2×SSC and 0.1% SDS, or 0.5×SSC and 0.1% SDS, or 0.1×SSC and 0.1% SDS at 68° C. for 15 minute intervals. Following the wash steps, the hybridized probes are detectable by autoradiography. Other conditions of high stringency which may be used are well known in the art and as cited in Sambrook et al., 1989, Molecular Cloning, A Laboratory Manual, Second Edition, Cold Spring Harbor Press, N.Y., pp. 9.47-9.57; and Ausubel et al., 1989, Current Protocols in Molecular Biology, Green Publishing Associates and Wiley Interscience, N.Y. are incorporated herein in their entirety. Preferably, such sequences encode a homolog of a polypeptide encoded by one of ORF2 to ORF1297. In one embodiment, such sequences encode a


Chlamydia pneumoniae


polypeptide.




(ii) By way of example and not limitation, procedures using conditions of intermediate stringency are as follows: Filters containing DNA are prehybridized, and then hybridized at a temperature of 60° C. in the presence of a 5×SSC buffer and labeled probe. Subsequently, filters washes are performed in a solution containing 2×SSC at 50° C. and the hybridized probes are detectable by autoradiography. Other conditions of intermediate stringency which may be used are well known in the art and as cited in Sambrook et al., 1989, Molecular Cloning, A Laboratory Manual, Second Edition, Cold Spring Harbor Press, N.Y., pp. 9.47-9.57; and Ausubel et al., 1989, Current Protocols in Molecular Biology, Green Publishing Associates and Wiley Interscience, N.Y. are incorporated herein in their entirety. Preferably, such sequences encode a homolog of a polypeptide encoded by one of ORF2 to ORF1297. In one embodiment, such sequences encode a


Chlamydia pneumoniae


polypeptide.




d) complementary or RNA nucleotide sequence corresponding to an ORF2 to ORF1297 sequence according to the invention or as defined in a), b) or c);




e) a nucleotide sequence of a representative fragment of an ORF2 to ORF1297 sequence according to the invention or of a sequence as defined in a), b), c) or d);




f) a nucleotide sequence capable of being obtained from an ORF2 to ORF1297 sequence according to the invention or as defined in a), b), c), d) or e); and




g) a modified nucleotide sequence of an ORF2 to ORF1297 sequence according to the invention or as defined in a), b), c), d), e) or f);




As regards the homology with the ORF2 to ORF1297 nucleotide sequences, the homologous sequences exhibiting a percentage identity with the bases of one of the ORF2 to ORF1297 nucleotide sequences of at least 80%, preferably 90% and 95%, are preferred. Such homologous sequences are identified routinely via, for example, the algorithms described above and in the examples below. The said homologous sequences correspond to the homologous sequences as defined above and may comprise, for example, the sequences corresponding to the ORF sequences of a bacterium belonging to the Chlamydia family, including the species


Chlamydia trachomatis, Chlamydia psittaci


and


Chlamydia pecorum


mentioned above, as well as the sequences corresponding to the ORF sequences of a bacterium belonging to the variants of the species


Chlamydia pneumoniae.


These homologous sequences may likewise correspond to variations linked to mutations within the same species or between species and may correspond in particular to truncations, substitutions, deletions and/or additions of at least one nucleotide. The said homologous sequences may also correspond to variations linked to the degeneracy of the genetic code or to a bias in the genetic code which is specific to the family, to the species or to the variant and which are likely to be present in Chlamydia.




The invention comprises polypeptides encoded by a nucleotide sequence according to the invention, preferably by a representative fragment of the sequence SEQ ID No. 1 and corresponding to an ORF sequence, in particular the


Chlamydia pneumoniae


polypeptides, characterized in that they are chosen from the sequences SEQ ID No. 2 to SEQ ID No. 1291 or SEQ ID No. 6844 to SEQ ID No. 6849 and representative fragments thereof. However, the invention is not limited to polypeptides encoded by ORFs in SEQ ID No. 1 and its corresponding ORF sequences, but encompasses polypeptides of strain variants, polymorphisms, allelic variants, and mutants.




Thus, the invention also comprises the polypeptides characterized in that they comprise a polypeptide chosen from:




a) a polypeptide encoded by a polynucleotide sequence in SEQ ID No. 1 (e.g., any polypeptide encoded by a polynucleotide sequence corresponding to ORF2 to ORF1297 and/or representative fragments thereof) according to the invention;




b) a polypeptide homologous to a polypeptide according to the invention, or as defined in a);




c) a polypeptide encoded by a polynucleotide sequence that hybridizes to SEQ ID No. 1 or ORF2 to ORF1297 under high or intermediate stringency as described below:




(i) By way of example and not limitation, procedures using conditions of high stringency are as follows: Prehybridization of filters containing DNA is carried out for 8 h to overnight at 65° C. in buffer composed of 6×SSC, 50 mM Tris-HCl (pH 7.5), 1 mM EDTA, 0.02% PVP, 0.02% Ficoll, 0.02% BSA, and 500 μg/ml denatured salmon sperm DNA. Filters are hybridized for 48 h at 65° C., the preferred hybridization temperature, in prehybridization mixture containing 100 μg/ml denatured salmon sperm DNA and 5-20×10


6


cpm of


32


P-labeled probe. Alternatively, the hybridization step can be performed at 65° C. in the presence of SSC buffer, 1×SSC corresponding to 0.15M NaCl and 0.05 M Na citrate. Subsequently, filter washes can be done at 37° C. for 1 h in a solution containing 2×SSC, 0.01% PVP, 0.01% Ficoll, and 0.01% BSA, followed by a wash in 0.1×SSC at 50° C. for 45 min. Alternatively, filter washes can be performed in a solution containing 2×SSC and 0.1% SDS, or 0.5×SSC and 0.1% SDS, or 0.1×SSC and 0.1% SDS at 68° C. for 15 minute intervals. Following the wash steps, the hybridized probes are detectable by autoradiography. Other conditions of high stringency which may be used are well known in the art and as cited in Sambrook et al., 1989, Molecular Cloning, A Laboratory Manual, Second Edition, Cold Spring Harbor Press, N.Y., pp. 9.47-9.57; and Ausubel et al., 1989, Current Protocols in Molecular Biology, Green Publishing Associates and Wiley Interscience, N.Y. are incorporated herein in their entirety. Preferably such polypeptide represents a homolog of a polypeptide encoded by ORF2 to ORF1297. Preferably, such sequences encode a homolog of a polypeptide encoded by one of ORF2 to ORF1297. In one embodiment, such sequences encode a


Chlamydia pneumoniae


polypeptide.




(ii) By way of example and not limitation, procedures using conditions of intermediate stringency are as follows: Filters containing DNA are prehybridized, and then hybridized at a temperature of 60° C. in the presence of a 5×SSC buffer and labeled probe. Subsequently, filters washes are performed in a solution containing 2×SSC at 50° C. and the hybridized probes are detectable by autoradiography. Other conditions of intermediate stringency which may be used are well known in the art and as cited in Sambrook et al., 1989, Molecular Cloning, A Laboratory Manual, Second Edition, Cold Spring Harbor Press, N.Y., pp. 9.47-9.57; and Ausubel et al., 1989, Current Protocols in Molecular Biology, Green Publishing Associates and Wiley Interscience, N.Y. are incorporated herein in their entirety. Preferably, such sequences encode a homolog of a polypeptide encoded by one of ORF2 to ORF1297. In one embodiment, such sequences encode a


Chlamydia pneumoniae


polypeptide.




d) a fragment of at least 5 amino acids of a polypeptide according to the invention, or as defined in a), b) or c);




e) a biologically active fragment of a polypeptide according to the invention, or as defined in a), b), c) or d); and




f) a modified polypeptide of a polypeptide according to the invention, as defined in a), b), c), d) or e).




In the present description, the terms polypeptide, peptide and protein are interchangeable.




It should be understood that the invention does not relate to the polypeptides in natural form, that is to say hat they are not taken in their natural environment but that they may have been isolated or obtained by purification from natural sources, or alternatively obtained by genetic recombination, or else by chemical synthesis and that they may, in this case, comprise nonnatural amino acids, as will be described below.




Homologous polypeptide will be understood to designate the polypeptides exhibiting, in relation to the natural polypeptide, certain modifications such as in particular a deletion, addition or substitution of at least one amino acid, a truncation, an extension, a chimeric fusion, and/or a mutation, or polypeptides exhibiting post-translational modifications. Among the homologous polypeptides, those whose amino acid sequence exhibits at least 80%, preferably 90%, homology or identity with the amino acid sequences of the polypeptides according to the invention are preferred. In the case of a substitution, one or more consecutive or nonconsecutive amino acids are replaced by “equivalent” amino acids. The expression “equivalent” amino acid is intended here to designate any amino acid capable of being substituted for one of the amino acids in the basic structure without, however, essentially modifying the biological activities of the corresponding peptides and as will be defined later.




Protein and/or nucleic acid sequence homologies may be evaluated using any of the variety of sequence comparison algorithms and programs known in the art. Such algorithms and programs include, but are by no means limited to, TBLASTN, BLASTP, FASTA, TFASTA, and CLUSTALW (Pearson and Lipman, 1988,


Proc. Natl. Acad. Sci. USA


85(8):2444-2448; Altschul et al., 1990,


J. Mol. Biol.


215(3):403-410; Thompson et al., 1994,


Nucleic Acids Res.


22(2):4673-4680; Higgins et al., 1996,


Methods Enzymol.


266:383-402; Altschul et al., 1990,


J. Mol. Biol.


215(3):403-410; Altschul et al., 1993,


Nature Genetics


3:266-272).




In a particularly preferred embodiment, protein and nucleic acid sequence homologies are evaluated using the Basic Local Alignment Search Tool (“BLAST”) which is well know in the art (see, e.g., Karlin and Altschul, 1990,


Proc. Natl. Acad. Sci. USA


87:2267-2268; Altschul et al., 1990,


J. Mol. Biol.


215:403-410; Altschul et al., 1993,


Nature Genetics


3:266-272; Altschul et al., 1997,


Nuc. Acids Res.


25:3389-3402). In particular, five specific BLAST programs are used to perform the following task:




(1) BLASTP and BLAST3 compare an amino acid query sequence against a protein sequence database;




(2) BLASTN compares a nucleotide query sequence against a nucleotide sequence database;




(3) BLASTX compares the six-frame conceptual translation products of a query nucleotide sequence (both strands) against a protein sequence database;




(4) TBLASTN compares a query protein sequence against a nucleotide sequence database translated in all six reading frames (both strands); and




(5) TBLASTX compares the six-frame translations of a nucleotide query sequence against the six-frame translations of a nucleotide sequence database.




The BLAST programs identify homologous sequences by identifying similar segments, which are referred to herein as “high-scoring segment pairs,” between a query amino or nucleic acid sequence and a test sequence which is preferably obtained from a protein or nucleic acid sequence database. High-scoring segment pairs are preferably identified (i.e., aligned) by means of a scoring matrix, many of which are known in the art. Preferably, the scoring matrix used is the BLOSUM62 matrix (Gonnet et al., 1992,


Science


256:1443-1445; Henikoff and Henikoff, 1993,


Proteins


17:49-61). Less preferably, the PAM or PAM250 matrices may also be used (see, e.g., Schwartz and Dayhoff, eds., 1978,


Matrices for Detecting Distance Relationships: Atlas of Protein Sequence and Structure,


Washington: National Biomedical Research Foundation).




The BLAST programs evaluate the statistical significance of all high-scoring segment pairs identified, and preferably selects those segments which satisfy a user-specified threshold of significance, such as a user-specified percent homology. Preferably, the statistical significance of a high-scoring segment pair is evaluated using the statistical significance formula of Karlin (see, e.g., Karlin and Altschul, 1990,


Proc. Natl. Acad. Sci. USA


87:2267-2268).




Equivalent amino acids may be determined either based on their structural homology with the amino acids for which they are substituted, or on results of comparative tests of biological activity between the various polypeptides which may be carried out.




By way of example, there may be mentioned the possibilities of substitutions which may be carried out without resulting in a substantial modification of the biological activity of the corresponding modified polypeptides; the replacements, for example, of leucine with valine or isoleucine, of aspartic acid with glutamic acid, of glutamine with asparagine, of arginine with lysine, and the like, the reverse substitutions naturally being feasible under the same conditions.




The homologous polypeptides also correspond to the polypeptides encoded by the homologous nucleotide sequences as defined above and thus comprise in the present definition the mutated polypeptides or polypeptides corresponding to inter- or intra-species variations which may exist in Chlamydia, and which correspond in particular to truncations, substitutions, deletions and/or additions of at least one amino acid residue.




Biologically active fragment of a polypeptide according to the invention will be understood to designate in particular a polypeptide fragment, as defined below, exhibiting at least one of the characteristics of the polypeptides according to the invention, in particular in that it is:




capable of eliciting an immune response directed against


Chlamydia pneumoniae;


and/or




capable of being recognized by an antibody specific for a polypeptide according to the invention; and/or




capable of binding to a polypeptide or to a nucleotide sequence of


Chlamydia pneumoniae;


and/or




capable of modulating, regulating, inducing or inhibiting the expression of a gene of


Chlamydia pneumoniae


or one of its associated microorganisms, and/or capable of modulating the replication cycle of


Chlamydia pneumoniae


or one of its associated microorganisms in the host cell and/or organism; and/or




capable of generally exerting an even partial physiological activity, such as for example a structural activity (cellular envelope, ribosome), an enzymatic (metabolic) activity, a transport activity, an activity in the secretion or in the virulence.




A polypeptide fragment according to the invention is understood to designate a polypeptide comprising a minimum of 5 amino acids, preferably 10 amino acids or preferably 15 amino acids. It is to be understood that such fragments refer only to portions of polypeptides encoded by ORF2 to ORF1297 that are not currently listed in a publicly available database.




The polypeptide fragments according to the invention may correspond to isolated or purified fragments which are naturally present in


Chlamydia pneumoniae


or which are secreted by


Chlamydia pneumoniae,


or may correspond to fragments capable of being obtained by cleaving the said polypeptide with a proteolytic enzyme, such as trypsin or chymotrypsin or collagenase, or with a chemical reagent, such as cyanogen bromide (CNBr) or alternatively by placing the said polypeptide in a highly acidic environment, for example at pH 2.5. Such polypeptide fragments may be equally well prepared by chemical synthesis, using hosts transformed with an expression vector according to the invention containing a nucleic acid allowing the expression of the said fragments, placed under the control of appropriate elements for regulation and/or expression.




“Modified polypeptide” of a polypeptide according to the invention is understood to designate a polypeptide obtained by genetic recombination or by chemical synthesis as will be described below, exhibiting at least one modification in relation to the normal sequence. These modifications may in particular affect amino acids responsible for a specificity or for the efficiency of the activity, or responsible for the structural conformation, for the charge or for the hydrophobicity, and for the capacity for multimerization and for membrane insertion of the polypeptide according to the invention. It is thus possible to create polypeptides with an equivalent, an increased or a reduced activity, and with an equivalent, a narrower or a broader specificity. Among the modified polypeptides, there may be mentioned the polypeptides in which up to 5 amino acids may be modified, truncated at the N- or C-terminal end, or alternatively deleted, or else added.




As is indicated, the modifications of the polypeptide may have in particular the objective:




of making it capable of modulating, regulating, inhibiting or inducing the expression of a gene of Chlamydia, in particular of


Chlamydia pneumoniae


and its variants, or one of its associated microorganisms, and/or capable of modulating the replication cycle of Chlamydia, in particular of


Chlamydia pneumoniae


and its variants, or one of its associated microorganisms, in the host cell and/or organism,




of allowing its use in methods of biosynthesis or of biodegradation, or its incorporation into vaccine compositions,




of modifying its bioavailability as a compound for therapeutic use.




The said modified polypeptides may also be used on any cell or microorganism for which the said modified polypeptides will be capable of modulating, regulating, inhibiting or inducing gene expression, or of modulating the growth or the replication cycle of the said cell or of the said microorganism. The methods allowing demonstration of the said modulations on eukaryotic or prokaryotic cells are well known to persons skilled in the art. The said cells or microorganisms will be chosen, in particular, from tumour cells or infectious microorganisms and the said modified polypeptides may be used for the prevention or treatment of pathologies linked to the presence of the said cells or of the said microorganisms. It is also clearly understood that the nucleotide sequences encoding the said modified polypeptides may be used for the said modulations, for example by the intermediacy of vectors according to the invention and which are described below, so as to prevent or to treat the said pathologies.




The above modified polypeptides may be obtained using combinatory chemistry, in which it is possible to systematically vary portions of the polypeptide before testing them on models, cell cultures or microorganisms for example, so as to select the compounds which are the most active or which exhibit the desired properties.




Chemical synthesis also has the advantage of being able to use:




nonnatural amino acids, or




nonpeptide bonds.




Accordingly, in order to extend the life of the polypeptides according to the invention, it may be advantageous to use nonnatural amino acids, for example in the D form, or alternatively amino acid analogues, in particular sulphur-containing forms for example.




Finally, the structure of the polypeptides according to the invention, its homologous or modified forms, as well as the corresponding fragments may be integrated into chemical structures of the polypeptide type and the like. Accordingly, it may be advantageous to provide at the N- and C-terminal ends compounds which are not recognized by proteases.




Also forming part of the invention are the nucleotide sequences encoding a polypeptide according to the invention. Described below are ORF nucleotide sequences encoding polypeptides exhibiting particularly preferable characteristics. For each group of preferred ORFS described below, it is to be understood that in addition to the individual ORFs listed, in instances wherein such ORFS are present as part of “combined” ORFs, the “combined” ORFs are also to be included within the preferred group.




More particularly, the subject of the invention is nucleotide sequences, characterized in that they encode a polypeptide of the cellular envelope, preferably of the outer cellular envelope of


Chlamydia pneumoniae


or one of its representative fragments, such as for example the predominant proteins of the outer membrane, the adhesion proteins or the proteins entering into the composition of the Chlamydia wall. Among these sequences, the sequences comprising a nucleotide sequence chosen from the following sequences are most preferred:




ORF15; ORF25; ORF26; ORF27; ORF28; ORF29; ORF30; ORF31; ORF32; ORF33; ORF35; ORF68; ORF124; ORF275; ORF291; ORF294; ORF327; ORF342; ORF364; ORF374; ORF380; ORF414; ORF439; ORF466; ORF467; ORF468; ORF469; ORF470; ORF472; ORF474; ORF476; ORF477; ORF478; ORF479; ORF480; ORF482; ORF485; ORF500; ORF501; ORF503; ORF504; ORF505; ORF506; ORF520; ORF578; ORF580; ORF581; ORF595; ORF596; ORF597; ORF737; ORF830; ORF834; ORF836; ORF893; ORF917; ORF932; ORF976; ORF1035; ORF1045; ORF1090 and one of their representative fragments.




The structure of the cytoplasmic membranes and of the wall of bacteria is dependent on the associated proteins. The structure of the cytoplasmic membrane makes it impermeable to water, to water-soluble substances and to small-sized molecules (ions, small inorganic molecules, peptides or proteins). To enter into or to interfere with a cell or a bacterium, a ligand must establish a special relationship with a protein anchored in the cytoplasmic membrane (the receptor). These proteins which are anchored on the membrane play an important role in metabolism since they control the exchanges in the bacterium. These exchanges apply to molecules of interest for the bacterium (small molecules such as sugars and small peptides) as well as undesirable molecules for the bacterium such as antibiotics or heavy metals.




The double lipid layer structure of the membrane requires the proteins which are inserted therein to have hydrophobic domains of about twenty amino acids forming an alpha helix. Predominantly hydrophobic and potentially transmembrane regions may be predicted from the primary sequence of the proteins, itself deduced from the nucleotide sequence. The presence of one or more putative transmembrane domains raises the possibility for a protein to be associated with the cytoplasmic membrane and to be able to play an important metabolic role therein or alternatively for the protein thus exposed to be able to exhibit potentially protective epitopes.




If the proteins inserted into the membrane exhibit several transmembrane domains capable of interacting with one another via electrostatic bonds, it then becomes possible for these proteins to form pores which go across the membrane which becomes permeable for a number of substances. It should be noted that proteins which do not have transmembrane domains may also be anchored by the intermediacy of fatty acids in the cytoplasmic membrane, it being possible for the breaking of the bond between the protein and its anchor in some cases to be responsible for the release of the peptide outside the bacterium.




Preferably, the invention relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


transmembrane polypeptide or one of its representative fragments, having between 1 and 3 transmembrane domains and in that they comprise a nucleotide sequence chosen from the following sequences:




ORF2; ORF3; ORF6; ORF9; ORF10; ORF11; ORF13; ORF14; ORF16; ORF18; ORF19; ORF20; ORF21; ORF22; ORF25; ORF27; ORF28; ORF29; ORF30; ORF31; ORF32; ORF33; ORF34; ORF35; ORF37; ORF39; ORF41; ORF42; ORF44; ORF45; ORF46; ORF47; ORF48; ORF49; ORF50; ORF53; ORF54; ORF56; ORF57; ORF59; ORF60; ORF61; ORF62; ORF63; ORF64; ORF65; ORF66; ORF69; ORF72; ORF73; ORF74; ORF76; ORF77; ORF78; ORF79; ORF80; ORF82; ORF84; ORF85; ORF86; ORF88; ORF89; ORF90; ORF91; ORF92; ORF93; ORF95; ORF96; ORF98; ORF99; ORF100; ORF101; ORF102; ORF103; ORF104; ORF105; ORF106; ORF107; ORF108; ORF114; ORF117; ORF118; ORF122; ORF123; ORF124; ORF125; ORF129; ORF130; ORF131; ORF132; ORF133; ORF134; ORF135; ORF137; ORF138; ORF139; ORF140; ORF141; ORF142; ORF143; ORF145; ORF146; ORF147; ORF150; ORF151; ORF152; ORF156; ORF157; ORF158; ORF159; ORF160; ORF161; ORF162; ORF164; ORF166; ORF167; ORF170; ORF173; ORF175; ORF176; ORF178; ORF179; ORF180; ORF182; ORF183; ORF184; ORF185; ORF186; ORF187; ORF188; ORF189; ORF190; ORF191; ORF192; ORF194; ORF195; ORF196; ORF197; ORF198; ORF199; ORF200; ORF201; ORF202; ORF205; ORF207; ORF208; ORF209; ORF210; ORF212; ORF215; ORF219; ORF220; ORF224; ORF226; ORF227; ORF228; ORF231; ORF232; ORF233; ORF234; ORF235; ORF236; ORF238; ORF239; ORF240; ORF241; ORF242; ORF244; ORF247; ORF251; ORF252; ORF253; ORF255; ORF256; ORF257; ORF258; ORF260; ORF262; ORF263; ORF266; ORF267; ORF268; ORF269; ORF270; ORF273; ORF274; ORF276; ORF278; ORF279; ORF280; ORF281; ORF282; ORF283; ORF284; ORF286; ORF287; ORF289; ORF290; ORF291; ORF293; ORF294; ORF297; ORF304; ORF305; ORF307; ORF308; ORF309; ORF310; ORF311; ORF313; ORF314; ORF315; ORF316; ORF318; ORF319; ORF320; ORF321; ORF322; ORF323; ORF324; ORF325; ORF326; ORF331; ORF332; ORF336; ORF338; ORF339; ORF341; ORF344; ORF345; ORF346; ORF350; ORF352; ORF353; ORF356; ORF357; ORF358; ORF359; ORF360; ORF362; ORF365; ORF366; ORF367; ORF370; ORF372; ORF373; ORF376; ORF377; ORF378; ORF379; ORF381; ORF382; ORF383; ORF384; ORF385; ORF386; ORF387; ORF390; ORF392; ORF393; ORF394; ORF396; ORF398; ORF399; ORF400; ORF404; ORF408; ORF410; ORF411; ORF413; ORF416; ORF417; ORF418; ORF420; ORF422; ORF424; ORF427; ORF428; ORF429; ORF430; ORF431; ORF433; ORF434; ORF437; ORF440; ORF441; ORF442; ORF443; ORF444; ORF445; ORF447; ORF450; ORF451; ORF452; ORF455; ORF456; ORF459; ORF460; ORF461; ORF462; ORF463; ORF464; ORF465; ORF467; ORF469; ORF471; ORF474; ORF475; ORF476; ORF477; ORF479; ORF482; ORF483; ORF484; ORF485; ORF486; ORF487; ORF488; ORF491; ORF493; ORF494; ORF497; ORF498; ORF499; ORF503; ORF508; ORF509; ORF510; ORF512; ORF514; ORF515; ORF516; ORF517; ORF518; ORF520; ORF521; ORF523; ORF525; ORF527; ORF528; ORF529; ORF530; ORF531; ORF533; ORF534; ORF535; ORF536; ORF537; ORF540; ORF541; ORF543; ORF544; ORF545; ORF546; ORF548; ORF549; ORF551; ORF553; ORF554; ORF555; ORF556; ORF557; ORF558; ORF559; ORF560; ORF562; ORF563; ORF564; ORF565; ORF566; ORF569; ORF571; ORF573; ORF576; ORF577; ORF581; ORF583; ORF584; ORF585; ORF586; ORF588; ORF591; ORF592; ORF594; ORF595; ORF596; ORF597; ORF599; ORF600; ORF603; ORF605; ORF608; ORF614; ORF615; ORF620; ORF621; ORF622; ORF623; ORF624; ORF625; ORF629; ORF630; ORF631; ORF633; ORF634; ORF637; ORF642; ORF644; ORF645; ORF647; ORF648; ORF652; ORF654; ORF655; ORF657; ORF658; ORF659; ORF660; ORF661; ORF664; ORF665; ORF666; ORF667; ORF670; ORF671; ORF672; ORF673; ORF674; ORF676; ORF679; ORF681; ORF684; ORF687; ORF688; ORF689; ORF690; ORF693; ORF694; ORF695; ORF696; ORF697; ORF698; ORF699; ORF700; ORF701; ORF703; ORF705; ORF706; ORF707; ORF708; ORF710; ORF712; ORF715; ORF716; ORF717; ORF718; ORF719; ORF721; ORF722; ORF723; ORF725; ORF726; ORF727; ORF728; ORF729; ORF730; ORF731; ORF733; ORF736; ORF737; ORF738; ORF740; ORF741; ORF742; ORF743; ORF747; ORF748; ORF750; ORF752; ORF754; ORF755; ORF756; ORF757; ORF759; ORF760; ORF761; ORF762; ORF763; ORF764; ORF765; ORF766; ORF767; ORF768; ORF772; ORF774; ORF775; ORF777; ORF781; ORF783; ORF788; ORF791; ORF792; ORF793; ORF794; ORF795; ORF796; ORF797; ORF798; ORF799; ORF802; ORF803; ORF806; ORF807; ORF808; ORF809; ORF810; ORF811; ORF813; ORF814; ORF815; ORF816; ORF817; ORF819; ORF820; ORF821; ORF823; ORF824; ORF827; ORF829; ORF830; ORF831; ORF833; ORF834; ORF835; ORF837; ORF844; ORF845; ORF846; ORF847; ORF848; ORF849; ORF850; ORF851; ORF852; ORF854; ORF855; ORF856; ORF857; ORF859; ORF860; ORF862; ORF865; ORF866; ORF868; ORF869; ORF870; ORF871; ORF872; ORF874; ORF877; ORF878; ORF879; ORF880; ORF881; ORF882; ORF884; ORF885; ORF888; ORF889; ORF890; ORF891; ORF892; ORF894; ORF895; ORF896; ORF897; ORF899; ORF900; ORF902; ORF903; ORF904; ORF905; ORF909; ORF910; ORF912; ORF913; ORF914; ORF915; ORF917; ORF918; ORF919; ORF921; ORF923; ORF924; ORF926; ORF927; ORF928; ORF929; ORF930; ORF931; ORF937; ORF938; ORF939; ORF941; ORF943; ORF948; ORF951; ORF952; ORF953; ORF958; ORF960; ORF963; ORF964; ORF965; ORF968; ORF970; ORF974; ORF975; ORF977; ORF979; ORF980; ORF981; ORF983; ORF984; ORF985; ORF987; ORF989; ORF992; ORF993; ORF997; ORF998; ORF999; ORF1001; ORF1002; ORF1004; ORF1005; ORF1009; ORF1013; ORF1014; ORF1015; ORF1016; ORF1019; ORF1021; ORF1023; ORF1024; ORF1029; ORF1031; ORF1033; ORF1034; ORF1039; ORF1041; ORF1042; ORF1045; ORF1047; ORF1049; ORF1051; ORF1052; ORF1053; ORF1054; ORF1056; ORF1059; ORF1061; ORF1062; ORF1063; ORF1064; ORF1065; ORF1067; ORF1075; ORF1077; ORF1078; ORF1079; ORF1080; ORF1081; ORF1089; ORF1095; ORF1097; ORF1098; ORF1099; ORF1101; ORF1102; ORF1103; ORF1106; ORF1107; ORF1108; ORF1109; ORF1110; ORF1113; ORF1116; ORF1118; ORF1119; ORF1121; ORF1123; ORF1124; ORF1126; ORF1128; ORF1130; ORF1131; ORF1133; ORF1134; ORF1136; ORF1137 and one of their representative fragments.




Preferably, the invention relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


transmembrane polypeptide or one of its representative fragments, having between 4 and 6 transmembrane domains and in that they comprise a nucleotide sequence chosen from the following sequences:




ORF5; ORF7; ORF8; ORF15; ORF36; ORF38; ORF51; ORF55; ORF58; ORF67; ORF70; ORF81; ORF97; ORF110; ORF111; ORF115; ORF119; ORF126; ORF128; ORF148; ORF155; ORF163; ORF165; ORF168; ORF169; ORF171; ORF172; ORF174; ORF177; ORF181; ORF193; ORF203; ORF213; ORF214; ORF216; ORF217; ORF221; ORF222; ORF225; ORF229; ORF243; ORF246; ORF248; ORF254; ORF261; ORF285; ORF288; ORF292; ORF296; ORF298; ORF299; ORF301; ORF303; ORF317; ORF328; ORF329; ORF351; ORF354; ORF355; ORF364; ORF371; ORF374; ORF375; ORF391; ORF395; ORF401; ORF403; ORF405; ORF409; ORF414; ORF419; ORF421; ORF423; ORF425; ORF438; ORF448; ORF453; ORF458; ORF466; ORF468; ORF470; ORF480; ORF489; ORF490; ORF496; ORF501; ORF504; ORF505; ORF506; ORF511; ORF513; ORF519; ORF526; ORF532; ORF538; ORF539; ORF547; ORF550; ORF561; ORF568; ORF570; ORF574; ORF578; ORF579; ORF580; ORF582; ORF589; ORF593; ORF598; ORF601; ORF604; ORF610; ORF613; ORF617; ORF626; ORF632; ORF635; ORF638; ORF640; ORF641; ORF646; ORF649; ORF650; ORF651; ORF686; ORF711; ORF724; ORF732; ORF734; ORF744; ORF745; ORF749; ORF751; ORF769; ORF770; ORF771; ORF773; ORF776; ORF779; ORF780; ORF785; ORF787; ORF789; ORF801; ORF805; ORF812; ORF822; ORF825; ORF826; ORF839; ORF841; ORF843; ORF853; ORF861; ORF875; ORF876; ORF886; ORF893; ORF898; ORF906; ORF907; ORF908; ORF920; ORF922; ORF925; ORF933; ORF935; ORF936; ORF944; ORF946; ORF947; ORF954; ORF959; ORF961; ORF966; ORF967; ORF972; ORF978; ORF995; ORF996; ORF1000; ORF1003; ORF1010; ORF1011; ORF1012; ORF1017; ORF1020; ORF1030; ORF1036; ORF1038; ORF1043; ORF1046; ORF1048; ORF1050; ORF1058; ORF1071; ORF1073; ORF1084; ORF1085; ORF1086; ORF1087; ORF1091; ORF1092; ORF1094; ORF1096; ORF1100; ORF1104; ORF1111; ORF1112; ORF1114; ORF1117; ORF1122; ORF1125 and one of their representative fragments.




Preferably, the invention also relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


transmembrane polypeptide or one of its representative fragments, having at least 7 transmembrane domains and in that they comprise a nucleotide sequence chosen from the following sequences:




ORF17; ORF52; ORF68; ORF83; ORF87; ORF109; ORF112; ORF113; ORF120; ORF121; ORF127; ORF153; ORF204; ORF211; ORF218; ORF223; ORF275; ORF277; ORF295; ORF300; ORF302; ORF306; ORF327; ORF335; ORF342; ORF343; ORF347; ORF349; ORF361; ORF363; ORF369; ORF380; ORF388; ORF389; ORF397; ORF415; ORF432; ORF439; ORF446; ORF449; ORF472; ORF478; ORF500; ORF522; ORF524; ORF567; ORF575; ORF602; ORF606; ORF609; ORF636; ORF639; ORF643; ORF653; ORF668; ORF692; ORF702; ORF704; ORF713; ORF720; ORF778; ORF784; ORF800; ORF836; ORF838; ORF842; ORF864; ORF867; ORF883; ORF901; ORF916; ORF932; ORF934; ORF940; ORF942; ORF950; ORF956; ORF971; ORF973; ORF976; ORF988; ORF994; ORF1018; ORF1028; ORF1035; ORF1037; ORF1044; ORF1055; ORF1057; ORF1068; ORF1069; ORF1070; ORF1072; ORF1082; ORF1088; ORF1105; ORF1132; ORF1135 and one of their representative fragments.




Preferably, the invention relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


surface exposed polypeptide (e.g., an outer membrane protein) or one of its representative fragments, said nucleotide sequences comprising a nucleotide sequence chosen from the following sequences:




ORF 15, ORF 25, ORF 26, ORF 27, ORF 28, ORF 29, ORF 30, ORF 31, ORF 32, ORF 33, ORF 35, ORF 36, ORF 1257, ORF 280, ORF 291, ORF 314, ORF 354, ORF 380, ORF 1266, ORF 466, ORF 467, ORF 468, ORF 469, ORF 470, ORF 472, ORF 474, ORF 476, ORF 477, ORF 478, ORF 479, ORF 480, ORF 482, ORF 483, ORF 485, ORF 486, ORF 500, ORF 501, ORF 503, ORF 504, ORF 505, ORF 506, ORF 507, ORF 1268, ORF 1269, ORF 543, ORF 544, ORF 578, ORF 579, ORF 580, ORF 581, ORF 595, ORF 596, ORF 597, ORF 1271, ORF 633, ORF 637, ORF 699, ORF 706, ORF 737, ORF 744, ORF 1273, ORF 751, ORF 775, ORF 776, ORF 777, ORF 793, ORF 815, ORF 830, ORF 1221, ORF 849, ORF 851, ORF 852, ORF 874, ORF 891, ORF 922, ORF 940, ORF 1231, ORF 1281, ORF 1035, ORF 1079, ORF 1087, ORF 1108, and one of their representative fragments.




Preferably, the invention relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


lipoprotein or one of its representative fragments, said nucleotide sequences comprising a nucleotide sequence chosen from the following sequences:




ORF 3, ORF 10, ORF 11, ORF 16, ORF 1254, ORF 1255, ORF 38, ORF 1256, ORF 62, ORF 85, ORF 1258, ORF 115, ORF 1151, ORF 151, ORF 1259, ORF 173, ORF 1261, ORF 186, ORF 194, ORF 205, ORF 214, ORF 216, ORF 217, ORF 238, ORF 1177, ORF 280, ORF 291, ORF 317, ORF 327, ORF 354, ORF 364, ORF 367, ORF 414, ORF 432, ORF 1192, ORF 460, ORF 1267, ORF 1268, ORF 520, ORF 536, ORF 1270, ORF 576, ORF 597, ORF 603, ORF 609, ORF 637, ORF 1272, ORF 652, ORF 1213, ORF 699, ORF 705, ORF 706, ORF 708, ORF 711, ORF 727, ORF 1274, ORF 800, ORF 814, ORF 825, ORF 829, ORF 830, ORF 831, ORF 844, ORF 849, ORF 1275, ORF 1276, ORF 1277, ORF 872, ORF 878, ORF 880, ORF 891, ORF 892, ORF 1278, ORF 1279, ORF 1280, ORF 941, ORF 942, ORF 1282, ORF 1283, ORF 952, ORF 988, ORF 998, ORF 1009, ORF 1285, ORF 1235, ORF 1028, ORF 1056, ORF 1070, ORF 1287, ORF 1087, ORF 1288, ORF 1289, ORF 1098, ORF 1246, ORF 1291, ORF 1108, ORF 1109, ORF 1112, ORF 1133, and one of their representative fragments.




Preferably, the invention relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


polypeptide involved in lipopolysaccharide (LPS) biosynthesis, said nucleotide sequences comprising a nucleotide sequence chosen from the following sequences: ORF 316, ORF 564, ORF 610, ORF 647, ORF 1211, ORF 688, ORF 924, and one of their representative fragments.




Preferably the invention relates to additional LPS-related nucleotide sequences according to the invention, characterized in that they encode:




(a) a


Chlamydia pneumoniae


KDO (3-deoxy-D-manno-octulosonic acid)-related polypeptide or one of its representative fragments, said nucleotide sequences comprising a nucleotide sequence chosen from the following sequences: ORF 177, ORF 1156, ORF 245, ORF 767, and one of their representative fragments;




(b) a


Chlamydia pneumoniae


phosphomannomutase-related polypeptide or one of its representative fragments, said nucleotide sequences comprising a nucleotide sequence chosen from the following sequences: ORF 74, and one of its representative fragments;




(c) a


Chlamydia pneumoniae


phosphoglucomutase-related polypeptide or one of its representative fragments, said nucleotide sequences comprising a nucleotide sequence chosen from the following sequences: ORF 1286, ORF 1039, and one of their representative fragments; and




(d) a


Chlamydia pneumoniae


lipid A component-related polypeptide or one of its representative fragments, said nucleotide sequences comprising a nucleotide sequence chosen from the following sequences: ORF 689, ORF 690, ORF 691, ORF 1037, and one of their representative fragments.




Preferably, the invention relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


polypeptide containing RGD (Arg-Gly-Asp) attachment sites or one of its representative fragments.




(a) RGD-containing proteins that are outer membrane proteins, are more likely to play a role in cell attachment. ORFs that encoded a protein containing an RGD sequence and also were classified as outer membrane proteins are ORF 468 and its representative fragments.




(a) An RGD-encoding ORF that showed homology to cds1, cds2, and copN type III virulence loci in


Chlamydia psittaci


(Hsia, R. et al. (1997), Type III secretion genes identity a putative virulence locus of Chlamydia. Molecular Microbiology 25:351-359) is ORF 350, and its representative fragments.




(c) The outer membrane of Chlamydia is made of cysteine-rich proteins that form a network of both intra and inter molecular disulfide links. This contributes to the integrity of the membrane since Chlamydia lacks the peptidoglycan layer that other gram-negative bacteria have. Cysteine-rich proteins that have the RGD sequence are also considered to be potential vaccine candidates. Cysteine-rich proteins were defined as proteins that had more than 3.0% cysteine in their primary amino acid sequence, above the mean genomic ORF cysteine content. The corresponding ORFs are: ORF 1290, ORF 1294, ORF 1296, and one of their representative fragments.




(d) The outer membrane of Chlamydia may also contain small proteins that have cysteines in their N- and C-terminus that may contribute to the network formed by disulfide linkages. These proteins may be anchored in the outer membrane via their N-terminus and may have their C-terminus exposed, which then can interact with the host cells. Alternatively, these proteins may be anchored in the outer membrane via both N-and C-terminus and may have regions in the middle that may be exposed which can in turn interact with the host cells. ORFs encoding polypeptides that contain cysteines in their first 30 amino acids and also contain an RGD sequence are:




ORF 105, ORF 106, ORF 114, ORF 170, ORF 171, ORF 1264, ORF 268, ORF 1265, ORF 350, ORF 393, ORF 394, ORF 451, ORF 452, ORF 453, ORF 473, ORF 499, ORF 515, ORF 519, ORF 525, ORF 526, ORF 538, ORF 611, ORF 645, ORF 686, ORF 700, ORF 746, ORF 755, ORF 756, ORF 757, ORF 789, ORF 814, ORF 855, ORF 856, ORF 878, ORF 957, ORF 958, ORF 989, ORF 1290, and one of their representative fragments.




(e) RGD-containing ORFs homologous to RGD-containing ORFs from


Chlamydia trachomatis


are:




ORF 114, ORF 468, ORF 755, ORF 756, ORF 757, ORF 855, ORF 856, ORF 905, ORF 913, ORF 914, ORF 915, and one of their representative fragments.




Preferably, the invention relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


Type III or other, non-type III secreted polypeptide or one of its representative fragments, said nucleotide sequences comprising a nucleotide sequence chosen from the following sequences:




ORF 25, ORF 28, ORF 29, ORF 33, ORF 308, ORF 309, ORF 343, ORF 344, ORF 345, ORF 367, ORF 414, ORF 415, ORF 480, ORF 550, ORF 579, ORF 580, ORF 581, ORF 597, ORF 699, ORF 744, ORF 751, ORF 776, ORF 866, ORF 874, ORF 883, ORF 884, ORF 888, ORF 891, ORF 1293, and one of their representative fragments.




Preferably, the invention relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


cell wall anchored surface polypeptide or one of its representative fragments, said nucleotide sequences comprising a nucleotide sequence chosen from the following sequences: ORF 267, ORF 271, ORF 419, ORF 590, ORF 932, ORF 1292, ORF 1295, and one of their representative fragments.




Preferably, the invention relates to the nucleotide sequences according to the invention, characterized in that they encode


Chlamydia pneumoniae


polypeptides not found in


Chlamydia trachomatis


(Blastp. P>e


−10


), said nucleotide sequences comprising a nucleotide sequence chosen from the following sequences:




ORF 7, ORF 8, ORF 9, ORF 16, ORF 17, ORF 18, ORF 19, ORF 20, ORF 21, ORF 22, ORF 1254, ORF 23, ORF 1255, ORF 24, ORF 1139, ORF 1140, ORF 46, ORF 47, ORF 51, ORF 60, ORF 1256, ORF 61, ORF 62, ORF 63, ORF 64, ORF 1257, ORF 65, ORF 66, ORF 67, ORF 68, ORF 1143, ORF 1145, ORF 83, ORF 84, ORF 1146, ORF 85, ORF 86, ORF 87, ORF 1258, ORF 116, ORF 117, ORF 125, ORF 1148, ORF 143, ORF 1150, ORF 1151, ORF 144, ORF 145, ORF 147, ORF 148, ORF 149, ORF 150, ORF 152, ORF 1259, ORF 162, ORF 166, ORF 1154, ORF 167, ORF 1261, ORF 1156, ORF 1157, ORF 178, ORF 179, ORF 1158, ORF 182, ORF 183, ORF 184, ORF 185, ORF 1159, ORF 186, ORF 1160, ORF 187, ORF 188, ORF 189, ORF 190, ORF 1161, ORF 1162, ORF 191, ORF 192, ORF 194, ORF 195, ORF 1163, ORF 196, ORF 201, ORF 202, ORF 209, ORF 212, ORF 221, ORF 224, ORF 1167, ORF 226, ORF 227, ORF 228, ORF 229, ORF 230, ORF 231, ORF 232, ORF 1169, ORF 1170, ORF 1171, ORF 234, ORF 235, ORF 236, ORF 1172, ORF 243, ORF 251, ORF 252, ORF 1176, ORF 253, ORF 255, ORF 254, ORF 256, ORF 1177, ORF 1178, ORF 262, ORF 263, ORF 1264, ORF 278, ORF 279, ORF 1180, ORF 280, ORF 290, ORF 291, ORF 292, ORF 296, ORF 1181, ORF 297, ORF 298, ORF 300, ORF 1265, ORF 322, ORF 324, ORF 325, ORF 370, ORF 1186, ORF 371, ORF 372, ORF 1187, ORF 373, ORF 378, ORF 1266, ORF 382, ORF 383, ORF 384, ORF 385, ORF 386, ORF 1188, ORF 1189, ORF 391, ORF 392, ORF 398, ORF 400, ORF 403, ORF 1191, ORF 423, ORF 435, ORF 445, ORF 450, ORF 1193, ORF 456, ORF 460, ORF 461, ORF 465, ORF 1196, ORF 471, ORF 473, ORF 475, ORF 481, ORF 484, ORF 487, ORF 488, ORF 489, ORF 490, ORF 491, ORF 492, ORF 493, ORF 494, ORF 495, ORF 496, ORF 497, ORF 498, ORF 499, ORF 502, ORF 1267, ORF 1268, ORF 508, ORF 510, ORF 509, ORF 512, ORF 515, ORF 519, ORF 1197, ORF 521, ORF 1198, ORF 522, ORF 524, ORF 528, ORF 534, ORF 537, ORF 1269, ORF 1270, ORF 548, ORF 551, ORF 557, ORF 1201, ORF 1203, ORF 562, ORF 566, ORF 593, ORF 595, ORF 600, ORF 1271, ORF 604, ORF 611, ORF 612, ORF 614, ORF 616, ORF 625, ORF 627, ORF 628, ORF 629, ORF 631, ORF 641, ORF 1272, ORF 648, ORF 1212, ORF 663, ORF 685, ORF 707, ORF 714, ORF 715, ORF 716, ORF 717, ORF 722, ORF 746, ORF 1273, ORF 761, ORF 764, ORF 770, ORF 1217, ORF 783, ORF 1274, ORF 803, ORF 815, ORF 1220, ORF 835, ORF 1221, ORF 844, ORF 845, ORF 846, ORF 847, ORF 848, ORF 849, ORF 850, ORF 851, ORF 1275, ORF 852, ORF 862, ORF 1276, ORF 1277, ORF 873, ORF 1223, ORF 892, ORF 919, ORF 1225, ORF 1278, ORF 926, ORF 1228, ORF 1229, ORF 1230, ORF 1279, ORF 1281, ORF 1282, ORF 1283, ORF 948, ORF 950, ORF 949, ORF 951, ORF 980, ORF 982, ORF 1233, ORF 999, ORF 1000, ORF 1001, ORF 1002, ORF 1008, ORF 1285, ORF 1235, ORF 1016, ORF 1019, ORF 1027, ORF 1036, ORF 1241, ORF 1048, ORF 1049, ORF 1050, ORF 1053, ORF 1054, ORF 1064, ORF 1076, ORF 1091, ORF 1288, ORF 1093, ORF 1289, ORF 1101, ORF 1103, ORF 1245, ORF 1246, ORF 1247, ORF 1290, ORF 1291, ORF 1115, ORF 1116, ORF 1118, ORF 1120, ORF 1249, ORF 1121, ORF 1250, ORF 1126, ORF 1251, ORF 1127, ORF 1128, ORF 1130, ORF 1129, ORF 1131, ORF 1136, ORF 1253, ORF 1292, ORF 1294, ORF 1295, ORF 1296, and one of their representative fragments.




Preferably, the invention also relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the intermediate metabolism, in particular in the metabolism of sugars and/or of cofactors, such as for example triose phosphate isomerase or pyruvate kinase, and in that they comprise a nucleotide sequence chosen from the following sequences:




ORF2; ORF55; ORF56; ORF69; ORF75; ORF80; ORF100; ORF110; ORF114; ORF120; ORF121; ORF157; ORF160; ORF161; ORF172; ORF180; ORF181; ORF198; ORF200; ORF225; ORF248; ORF249; ORF276; ORF277; ORF318; ORF319; ORF320; ORF323; ORF331; ORF347; ORF375; ORF376; ORF381; ORF393; ORF394; ORF395; ORF396; ORF409; ORF446; ORF447; ORF448; ORF449; ORF513; ORF516; ORF571; ORF647; ORF662; ORF697; ORF718; ORF793; ORF794; ORF808; ORF809; ORF838; ORF839; ORF840; ORF853; ORF854; ORF918; ORF923; ORF929; ORF931; ORF938; ORF939; ORF958; ORF959; ORF960; ORF966; ORF995; ORF1021; ORF1040; ORF1041; ORF1042; ORF1085; ORF1100; ORF1102; ORF1117; ORF1118; ORF1119; ORF1120; ORF1135 and one of their representative fragments.




Preferably, the invention also relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the intermediate metabolism of nucleotides or nucleic acids, such as for example CTP synthetase or GMP synthetase, and in that they comprise a nucleotide sequence chosen from the following sequences:




ORF77; ORF78; ORF138; ORF189; ORF190; ORF233; ORF246; ORF338; ORF412; ORF421; ORF438; ORF607; ORF648; ORF657; ORF740; ORF783; ORF967; ORF989; ORF990; ORF992; ORF1011; ORF1058; ORF1059; ORF1073; ORF1074 and one of their representative fragments.




Preferably, the invention also relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the metabolism of nucleic acids, such as for example DNA polymerases or DNA topoisomerases, and in that they comprise a nucleotide sequence chosen from the following sequences:




ORF14; ORF59; ORF70; ORF71; ORF97; ORF113; ORF137; ORF141; ORF169; ORF285; ORF287; ORF288; ORF313; ORF326; ORF358; ORF411; ORF443; ORF548; ORF569; ORF601; ORF651; ORF654; ORF658; ORF659; ORF664; ORF665; ORF694; ORF698; ORF704; ORF760; ORF762; ORF763; ORF786; ORF787; ORF788; ORF801; ORF802; ORF812; ORF819; ORF822; ORF870; ORF897; ORF898; ORF902; ORF908; ORF916; ORF954; ORF955; ORF961; ORF983; ORF996; ORF1007; ORF1012; ORF1013; ORF1014; ORF1015; ORF1038; ORF1137 and one of their representative fragments.




Preferably, the invention also relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the metabolism of amino acids or polypeptides, such as for example serine hydroxymethyl transferase or the proteins which load amino acids onto transfer RNAs, and in that they comprise a nucleotide sequence chosen from the following sequences:




ORF99; ORF111; ORF127; ORF134; ORF140; ORF174; ORF175; ORF176; ORF353; ORF377; ORF404; ORF523; ORF539; ORF559; ORF561; ORF586; ORF598; ORF609; ORF636; ORF687; ORF700; ORF701; ORF759; ORF790; ORF857; ORF861; ORF904; ORF936; ORF952; ORF962; ORF963; ORF964; ORF965; ORF991; ORF1003; ORF1004; ORF1005; ORF1018; ORF1067; ORF1110; ORF1111; ORF1112; ORF1114; ORF1121; ORF1122; ORF1123; ORF1124; ORF1125 and one of their representative fragments.




Preferably, the invention also relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the metabolism of polypeptides, such as for example protein kinases or proteases, and in that they comprise a nucleotide sequence chosen from the following sequences:




ORF4; ORF44; ORF45; ORF48; ORF54; ORF112; ORF130; ORF155; ORF163; ORF212; ORF257; ORF307; ORF343; ORF405; ORF416; ORF458; ORF540; ORF541; ORF542; ORF543; ORF544; ORF560; ORF594; ORF652; ORF699; ORF723; ORF747; ORF817; ORF827; ORF871; ORF909; ORF910; ORF911; ORF912; ORF1023; ORF1051; ORF1052; ORF1081 and one of their representative fragments.




Preferably, the invention also relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the metabolism of fatty acids, such as for example succinyl-CoA-synthesizing proteins or phosphatidylserine synthetase, and in that they comprise a nucleotide sequence chosen from the following sequences:




ORF76; ORF284; ORF308; ORF309; ORF310; ORF311; ORF312; ORF425; ORF433; ORF565; ORF688; ORF690; ORF691; ORF767; ORF797; ORF894; ORF895; ORF994; ORF1020; ORF1030; ORF1033; ORF1034; ORF1046; ORF1047; ORF1057 and one of their representative fragments.




Preferably, the invention also relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the synthesis of the wall, such as for example KDO transferase, and the proteins responsible for the attachment of certain sugars onto the exposed proteins, and in that they comprise a nucleotide sequence chosen from the following sequences:




ORF49; ORF50; ORF177; ORF178; ORF245; ORF610; ORF972; ORF974; ORF978; ORF1037 and one of their representative fragments.




Preferably, the invention also relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the transcription, translation and/or maturation process, such as for example initiation factors, RNA polymerases or certain chaperone proteins, and in that they comprise a nucleotide sequence chosen from the following sequences:




ORF90; ORF92; ORF131; ORF151; ORF199; ORF333; ORF334; ORF336; ORF379; ORF589; ORF590; ORF619; ORF630; ORF649; ORF739; ORF741; ORF806; ORF821; ORF843; ORF968; ORF971; ORF1061 and one of their representative fragments.




Preferably, the invention also relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


ribosomal polypeptide or one of its representative fragments, such as for example the ribosomal proteins L21, L27 and S10, and in that they comprise a nucleotide sequence chosen from the following sequences:




ORF93; ORF94; ORF95; ORF136; ORF259; ORF332; ORF348; ORF583; ORF584; ORF588; ORF591; ORF592; ORF663; ORF666; ORF667; ORF669; ORF670; ORF671; ORF672; ORF673; ORF674; ORF675; ORF676; ORF677; ORF678; ORF679; ORF680; ORF681; ORF683; ORF684; ORF738; ORF781; ORF1008; ORF1024; ORF1025; ORF1066 and one of their representative fragments.




Preferably, the invention also relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


transport polypeptide or one of its representative fragments, such as for example the proteins for transporting amino acids, sugars and certain oligopeptides, and in that they comprise a nucleotide sequence chosen from the following sequences:




ORF40; ORF41; ORF52; ORF105; ORF106; ORF107; ORF109; ORF133; ORF210; ORF211; ORF214; ORF215; ORF216; ORF217; ORF218; ORF219; ORF220; ORF223; ORF242; ORF260; ORF293; ORF299; ORF366; ORF369; ORF575; ORF602; ORF638; ORF639; ORF640; ORF643; ORF653; ORF702; ORF703; ORF724; ORF732; ORF855; ORF856; ORF901; ORF906; ORF933; ORF942; ORF1043; ORF1086; ORF1105 and one of their representative fragments.




Preferably, the invention also relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the virulence process, such as for example the proteins analogous to the


Escherichia coli


vacB protein, and in that they comprise a nucleotide sequence chosen from the following sequences:




ORF546; ORF550; ORF778; ORF779; ORF886 and one of their representative fragments.




Preferably, the invention also relates to the nucleotide sequences according to the invention, characterized in that they encode a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the secretory system and/or which is secreted, such as for example proteins homologous to proteins in the secretory system of certain bacteria such as the Salmonellae or the Yersiniae, and in that they comprise a nucleotide sequence chosen from the following sequences:




ORF751; ORF874; ORF875; ORF876; ORF883; ORF884; ORF885 and one of their representative fragments.




Preferably, the invention also relates to a nucleotide sequence according to the invention, characterized in that they encode a polypeptide specific to


Chlamydia pneumoniae


or one of its representative fragments (with a Blast E value of >10


−5


), and in that they comprise a nucleotide sequence chosen from the following sequences:




ORF7; ORF8; ORF17; ORF18; ORF19; ORF20; ORF22; ORF23; ORF24; ORF51; ORF60; ORF63; ORF65; ORF66; ORF67; ORF83; ORF84; ORF86; ORF87; ORF125; ORF143; ORF144; ORF179; ORF182; ORF184; ORF185; ORF187; ORF221; ORF252; ORF254;; ORF278; ORF279; ORF387; ORF388; ORF397; ORF1048; ORF1049; ORF1050; ORF1128; ORF1130; ORF1131 and one of their representative fragments.




Also forming part of the invention are polypeptides encoded by the polynucleotides of the invention, as well as fusion polypeptides comprising such polypeptides. In one embodiment, the polypeptides and fusion polypeptides immunoreact with seropositive serum of an individual infected with


Chlamydia pneumoniae.


For example, described below, are polypeptide sequences exhibiting particularly preferable characteristics. For each group of preferred polypeptides described below, it is to be understood that in addition to the individual polypeptides listed, in instances wherein such polypeptides are encoded as part of “combined” ORFs, such “combined” polypeptides are also to be included within the preferred group.




The subject of the invention is also a polypeptide according to the invention, characterized in that it is a polypeptide of the cellular envelope, preferably of the outer cellular envelope, of


Chlamydia pneumoniae


or one of its representative fragments. According to the invention, the said polypeptide is preferably chosen from the polypeptides having the following sequences:




SEQ ID No. 15; SEQ ID No. 25; SEQ ID No. 26; SEQ ID No. 27; SEQ ID No. 28; SEQ ID No. 29; SEQ ID No. 30; SEQ ID No. 31; SEQ ID No. 32; SEQ ID No. 33; SEQ ID No. 35; SEQ ID No. 68; SEQ ID No. 124; SEQ ID No. 275; SEQ ID No. 291; SEQ ID No. 294; SEQ ID No. 327; SEQ ID No. 342; SEQ ID No. 364; SEQ ID No. 374; SEQ ID No. 380; SEQ ID No. 414; SEQ ID No. 439; SEQ ID No. 466; SEQ ID No. 467; SEQ ID No. 468; SEQ ID No. 469; SEQ ID No. 470; SEQ ID No. 472; SEQ ID No. 474; SEQ ID No. 476; SEQ ID No. 477; SEQ ID No. 478; SEQ ID No. 479; SEQ ID No. 480; SEQ ID No. 482; SEQ ID No. 485; SEQ ID No. 500; SEQ ID No. 501; SEQ ID No. 503; SEQ ID No. 504; SEQ ID No. 505; SEQ ID No. 506; SEQ ID No. 520; SEQ ID No. 578; SEQ ID No. 580; SEQ ID No. 581; SEQ ID No. 595; SEQ ID No. 596; SEQ ID No. 597; SEQ ID No. 737; SEQ ID No. 830; SEQ ID No. 834; SEQ ID No. 836; SEQ ID No. 893; SEQ ID No. 917; SEQ ID No. 932; SEQ ID No. 976; SEQ ID No. 1035; SEQ ID No. 1045; SEQ ID No. 1090 and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, characterized in that it is a


Chlamydia pneumoniae


transmembrane polypeptide or one of its representative fragments, having between 1 and 3 transmembrane domains, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 2; SEQ ID No. 3; SEQ ID No. 6; SEQ ID No. 9; SEQ ID No. 10; SEQ ID No. 11; SEQ ID No. 13; SEQ ID No. 14; SEQ ID No. 16; SEQ ID No. 18; SEQ ID No. 19; SEQ ID No. 20; SEQ ID No. 21; SEQ ID No. 22; SEQ ID No. 25; SEQ ID No. 27; SEQ ID No. 28; SEQ ID No. 29; SEQ ID No. 30; SEQ ID No. 31; SEQ ID No. 32; SEQ ID No. 33; SEQ ID No. 34; SEQ ID No. 35; SEQ ID No. 37; SEQ ID No. 39; SEQ ID No. 41; SEQ ID No. 42; SEQ ID No. 44; SEQ ID No. 45; SEQ ID No. 46; SEQ ID No. 47; SEQ ID No. 48; SEQ ID No. 49; SEQ ID No. 50; SEQ ID No. 53; SEQ ID No. 54; SEQ ID No. 56; SEQ ID No. 57; SEQ ID No. 59; SEQ ID No. 60; SEQ ID No. 61; SEQ ID No. 62; SEQ ID No. 63; SEQ ID No. 64; SEQ ID No. 65; SEQ ID No. 66; SEQ ID No. 69;; SEQ ID No. 72; SEQ ID No. 73; SEQ ID No. 74; SEQ ID No. 76; SEQ ID No. 77; SEQ ID No. 78; SEQ ID No. 79; SEQ ID No. 80; SEQ ID No. 82; SEQ ID No. 84; SEQ ID No. 85; SEQ ID No. 86; SEQ ID No. 88; SEQ ID No. 89; SEQ ID No. 90; SEQ ID No. 91; SEQ ID No. 92; SEQ ID No. 93; SEQ ID No. 95; SEQ ID No. 96; SEQ ID No. 98; SEQ ID No. 99; SEQ ID No. 100; SEQ ID No. 101; SEQ ID No. 102; SEQ ID No. 103; SEQ ID No. 104; SEQ ID No. 105; SEQ ID No. 106; SEQ ID No. 107; SEQ ID No. 108; SEQ ID No. 114; SEQ ID No. 117; SEQ ID No. 118; SEQ ID No. 122; SEQ ID No. 123; SEQ ID No. 124; SEQ ID No. 125; SEQ ID No. 129; SEQ ID No. 130; SEQ ID No. 131; SEQ ID No. 132; SEQ ID No. 133; SEQ ID No. 134; SEQ ID No. 135; SEQ ID No. 137; SEQ ID No. 138; SEQ ID No. 139; SEQ ID No. 140; SEQ ID No. 141; SEQ ID No. 142; SEQ ID No. 143; SEQ ID No. 145; SEQ ID No. 146; SEQ ID No. 147; SEQ ID No. 150; SEQ ID No. 151; SEQ ID No. 152; SEQ ID No. 156; SEQ ID No. 157; SEQ ID No. 158; SEQ ID No. 159; SEQ ID No. 160; SEQ ID No. 161; SEQ ID No. 162; SEQ ID No. 164; SEQ ID No. 166; SEQ ID No. 167; SEQ ID No. 170; SEQ ID No. 173; SEQ ID No. 175; SEQ ID No. 176; SEQ ID No. 178; SEQ ID No. 179; SEQ ID No. 180; SEQ ID No. 182; SEQ ID No. 183; SEQ ID No. 184; SEQ ID No. 185; SEQ ID No. 186; SEQ ID No. 187; SEQ ID No. 188; SEQ ID No. 189; SEQ ID No. 190; SEQ ID No. 191; SEQ ID No. 192; SEQ ID No. 194; SEQ ID No. 195; SEQ ID No. 196; SEQ ID No. 197; SEQ ID No. 198; SEQ ID No. 199; SEQ ID No. 200; SEQ ID No. 201; SEQ ID No. 202; SEQ ID No. 205; SEQ ID No. 207; SEQ ID No. 208; SEQ ID No. 209; SEQ ID No. 210; SEQ ID No. 212; SEQ ID No. 215; SEQ ID No. 219; SEQ ID No. 220; SEQ ID No. 224; SEQ ID No. 226; SEQ ID No. 227; SEQ ID No. 228; SEQ ID No. 231; SEQ ID No. 232; SEQ ID No. 233; SEQ ID No. 234; SEQ ID No. 235; SEQ ID No. 236; SEQ ID No. 238; SEQ ID No. 239; SEQ ID No. 240; SEQ ID No. 241; SEQ ID No. 242; SEQ ID No. 244; SEQ ID No. 247; SEQ ID No. 251; SEQ ID No. 252; SEQ ID No. 253; SEQ ID No. 255; SEQ ID No. 256; SEQ ID No. 257; SEQ ID No. 258; SEQ ID No. 260; SEQ ID No. 262; SEQ ID No. 263; SEQ ID No. 266; SEQ ID No. 267; SEQ ID No. 268; SEQ ID No. 269; SEQ ID No. 270; SEQ ID No. 273; SEQ ID No. 274; SEQ ID No. 276; SEQ ID No. 278; SEQ ID No. 279; SEQ ID No. 280; SEQ ID No. 281; SEQ ID No. 282; SEQ ID No. 283; SEQ ID No. 284; SEQ ID No. 286; SEQ ID No. 287; SEQ ID No. 289; SEQ ID No. 290; SEQ ID No. 291; SEQ ID No. 293; SEQ ID No. 294; SEQ ID No. 297; SEQ ID No. 304; SEQ ID No. 305; SEQ ID No. 307; SEQ ID No. 308; SEQ ID No. 309; SEQ ID No. 310; SEQ ID No. 311; SEQ ID No. 313; SEQ ID No. 314; SEQ ID No. 315; SEQ ID No. 316; SEQ ID No. 318; SEQ ID No. 319; SEQ ID No. 320; SEQ ID No. 321; SEQ ID No. 322; SEQ ID No. 323; SEQ ID No. 324; SEQ ID No. 325; SEQ ID No. 326; SEQ ID No. 331; SEQ ID No. 332; SEQ ID No. 336; SEQ ID No. 338; SEQ ID No. 339; SEQ ID No. 341; SEQ ID No. 344; SEQ ID No. 345; SEQ ID No. 346; SEQ ID No. 350; SEQ ID No. 352; SEQ ID No. 353; SEQ ID No. 356; SEQ ID No. 357; SEQ ID No. 358; SEQ ID No. 359; SEQ ID No. 360; SEQ ID No. 362; SEQ ID No. 365; SEQ ID No. 366; SEQ ID No. 367; SEQ ID No. 370; SEQ ID No. 372; SEQ ID No. 373; SEQ ID No. 376; SEQ ID No. 377; SEQ ID No. 378; SEQ ID No. 379; SEQ ID No. 381; SEQ ID No. 382; SEQ ID No. 383; SEQ ID No. 384; SEQ ID No. 385; SEQ ID No. 386; SEQ ID No. 387; SEQ ID No. 390; SEQ ID No. 392; SEQ ID No. 393; SEQ ID No. 394; SEQ ID No. 396; SEQ ID No. 398; SEQ ID No. 399; SEQ ID No. 400; SEQ ID No. 404; SEQ ID No. 408; SEQ ID No. 410; SEQ ID No. 411; SEQ ID No. 413; SEQ ID No. 4 16; SEQ ID No. 41 7; SEQ ID No. 41 8; SEQ ID No. 420; SEQ ID No. 422; SEQ ID No. 424; SEQ ID No. 427; SEQ ID No. 428; SEQ ID No. 429; SEQ ID No. 430; SEQ ID No. 431; SEQ ID No. 433; SEQ ID No. 434; SEQ ID No. 437; SEQ ID No. 440; SEQ ID No. 441; SEQ ID No. 442; SEQ ID No. 443; SEQ ID No. 444; SEQ ID No. 445; SEQ ID No. 447; SEQ ID No. 450; SEQ ID No. 451; SEQ ID No. 452; SEQ ID No. 455; SEQ ID No. 456; SEQ ID No. 459; SEQ ID No. 460; SEQ ID No. 461; SEQ ID No. 462; SEQ ID No. 463; SEQ ID No. 464; SEQ ID No. 465; SEQ ID No. 467; SEQ ID No. 469; SEQ ID No. 471; SEQ ID No. 474; SEQ ID No. 475; SEQ ID No. 476; SEQ ID No. 477; SEQ ID No. 479; SEQ ID No. 482; SEQ ID No. 483; SEQ ID No. 484; SEQ ID No. 485; SEQ ID No. 486; SEQ ID No. 487; SEQ ID No. 488; SEQ ID No. 491; SEQ ID No. 493; SEQ ID No. 494; SEQ ID No. 497; SEQ ID No. 498; SEQ ID No. 499; SEQ ID No. 503; SEQ ID No. 508; SEQ ID No. 509; SEQ ID No. 510; SEQ ID No. 512; SEQ ID No. 514; SEQ ID No. 515; SEQ ID No. 516; SEQ ID No. 517; SEQ ID No. 518; SEQ ID No. 520; SEQ ID No. 521; SEQ ID No. 523; SEQ ID No. 525; SEQ ID No. 527; SEQ ID No. 528; SEQ ID No. 529; SEQ ID No. 530; SEQ ID No. 531; SEQ ID No. 533; SEQ ID No. 534; SEQ ID No. 535; SEQ ID No. 536; SEQ ID No. 537; SEQ ID No. 540; SEQ ID No. 541; SEQ ID No. 543; SEQ ID No. 544; SEQ ID No. 545; SEQ ID No. 546; SEQ ID No. 548; SEQ ID No. 549; SEQ ID No. 551; SEQ ID No. 553; SEQ ID No. 554; SEQ ID No. 555; SEQ ID No. 556; SEQ ID No. 557; SEQ ID No. 558; SEQ ID No. 559; SEQ ID No. 560; SEQ ID No. 562; SEQ ID No. 563; SEQ ID No. 564; SEQ ID No. 565; SEQ ID No. 566; SEQ ID No. 569; SEQ ID No. 571; SEQ ID No. 573; SEQ ID No. 576; SEQ ID No. 577; SEQ ID No. 581; SEQ ID No. 583; SEQ ID No. 584; SEQ ID No. 585; SEQ ID No. 586; SEQ ID No. 588; SEQ ID No. 591; SEQ ID No. 592; SEQ ID No. 594; SEQ ID No. 595; SEQ ID No. 596; SEQ ID No. 597; SEQ ID No. 599; SEQ ID No. 600; SEQ ID No. 603; SEQ ID No. 605; SEQ ID No. 608; SEQ ID No. 614; SEQ ID No. 615; SEQ ID No. 620; SEQ ID No. 621; SEQ ID No. 622; SEQ ID No. 623; SEQ ID No. 624; SEQ ID No. 625; SEQ ID No. 629; SEQ ID No. 630; SEQ ID No. 631; SEQ ID No. 633; SEQ ID No. 634; SEQ ID No. 637; SEQ ID No. 642; SEQ ID No. 644; SEQ ID No. 645; SEQ ID No. 647; SEQ ID No. 648; SEQ ID No. 652; SEQ ID No. 654; SEQ ID No. 655; SEQ ID No. 657; SEQ ID No. 658; SEQ ID No. 659; SEQ ID No. 660; SEQ ID No. 661; SEQ ID No. 664; SEQ ID No. 665; SEQ ID No. 666; SEQ ID No. 667; SEQ ID No. 670; SEQ ID No. 671; SEQ ID No. 672; SEQ ID No. 673; SEQ ID No. 674; SEQ ID No. 676; SEQ ID No. 679; SEQ ID No. 681; SEQ ID No. 684; SEQ ID No. 687; SEQ ID No. 688; SEQ ID No. 689; SEQ ID No. 690; SEQ ID No. 693; SEQ ID No. 694; SEQ ID No. 695; SEQ ID No. 696; SEQ ID No. 697; SEQ ID No. 698; SEQ ID No. 699; SEQ ID No. 700; SEQ ID No. 701; SEQ ID No. 703; SEQ ID No. 705; SEQ ID No. 706; SEQ ID No. 707; SEQ ID No. 708; SEQ ID No. 710; SEQ ID No. 712; SEQ ID No. 715; SEQ ID No. 716; SEQ ID No. 717; SEQ ID No. 718; SEQ ID No. 719; SEQ ID No. 721; SEQ ID No. 722; SEQ ID No. 723; SEQ ID No. 725; SEQ ID No. 726; SEQ ID No. 727; SEQ ID No. 728; SEQ ID No. 729; SEQ ID No. 730; SEQ ID No. 731; SEQ ID No. 733; SEQ ID No. 736; SEQ ID No. 737; SEQ ID No. 738; SEQ ID No. 740; SEQ ID No. 741; SEQ ID No. 742; SEQ ID No. 743; SEQ ID No. 747; SEQ ID No. 748; SEQ ID No. 750; SEQ ID No. 752; SEQ ID No. 754; SEQ ID No. 755; SEQ ID No. 756; SEQ ID No. 757; SEQ ID No. 759; SEQ ID No. 760; SEQ ID No. 761; SEQ ID No. 762; SEQ ID No. 763; SEQ ID No. 764; SEQ ID No. 765; SEQ ID No. 766; SEQ ID No. 767; SEQ ID No. 768; SEQ ID No. 772; SEQ ID No. 774; SEQ ID No. 775; SEQ ID No. 777; SEQ ID No. 781; SEQ ID No. 783; SEQ ID No. 788; SEQ ID No. 791; SEQ ID No. 792; SEQ ID No. 793; SEQ ID No. 794; SEQ ID No. 795; SEQ ID No. 796; SEQ ID No. 797; SEQ ID No. 798; SEQ ID No. 799; SEQ ID No. 802; SEQ ID No. 803; SEQ ID No. 806; SEQ ID No. 807; SEQ ID No. 808; SEQ ID No. 809; SEQ ID No. 810; SEQ ID No. 811; SEQ ID No. 813; SEQ ID No. 814; SEQ ID No. 815; SEQ ID No. 816; SEQ ID No. 817; SEQ ID No. 819; SEQ ID No. 820; SEQ ID No. 821; SEQ ID No. 823; SEQ ID No. 824; SEQ ID No. 827; SEQ ID No. 829; SEQ ID No. 830; SEQ ID No. 831; SEQ ID No. 833; SEQ ID No. 834; SEQ ID No. 835; SEQ ID No. 837; SEQ ID No. 844; SEQ ID No. 845 ; SEQ ID No. 8 46; SEQ ID No. 8 47 ; SEQ ID No. 848; SEQ ID No. 849; SEQ ID No. 850; SEQ ID No. 851; SEQ ID No. 852; SEQ ID No. 854; SEQ ID No. 855; SEQ ID No. 856; SEQ ID No. 857; SEQ ID No. 859; SEQ ID No. 860; SEQ ID No. 862; SEQ ID No. 865; SEQ ID No. 866; SEQ ID No. 868; SEQ ID No. 869; SEQ ID No. 870; SEQ ID No. 871; SEQ ID No. 872; SEQ ID No. 874; SEQ ID No. 877; SEQ ID No. 878; SEQ ID No. 879; SEQ ID No. 880; SEQ ID No. 881; SEQ ID No. 882; SEQ ID No. 884; SEQ ID No. 885; SEQ ID No. 888; SEQ ID No. 889; SEQ ID No. 890; SEQ ID No. 891; SEQ ID No. 892; SEQ ID No. 894; SEQ ID No. 895; SEQ ID No. 896; SEQ ID No. 897; SEQ ID No. 899; SEQ ID No. 900; SEQ ID No. 902; SEQ ID No. 903; SEQ ID No. 904; SEQ ID No. 905; SEQ ID No. 909; SEQ ID No. 910; SEQ ID No. 912; SEQ ID No. 913; SEQ ID No. 914; SEQ ID No. 915; SEQ ID No. 917; SEQ ID No. 918; SEQ ID No. 919; SEQ ID No. 921; SEQ ID No. 923; SEQ ID No. 924; SEQ ID No. 926; SEQ ID No. 927; SEQ ID No. 928; SEQ ID No. 929; SEQ ID No. 930; SEQ ID No. 931; SEQ ID No. 937; SEQ ID No. 938; SEQ ID No. 939; SEQ ID No. 941; SEQ ID No. 943; SEQ ID No. 948; SEQ ID No. 951; SEQ ID No. 952; SEQ ID No. 953; SEQ ID No. 958; SEQ ID No. 960; SEQ ID No. 963; SEQ ID No. 964; SEQ ID No. 965; SEQ ID No. 968; SEQ ID No. 970; SEQ ID No. 974; SEQ ID No. 975; SEQ ID No. 977; SEQ ID No. 979; SEQ ID No. 980; SEQ ID No. 981; SEQ ID No. 983; SEQ ID No. 984; SEQ ID No. 985; SEQ ID No. 987; SEQ ID No. 989; SEQ ID No. 992; SEQ ID No. 993; SEQ ID No. 997; SEQ ID No. 998; SEQ ID No. 999; SEQ ID No. 1001; SEQ ID No. 1002; SEQ ID No. 1004; SEQ ID No. 1005; SEQ ID No. 1009; SEQ ID No. 1013; SEQ ID No. 1014; SEQ ID No. 1015; SEQ ID No. 1016; SEQ ID No. 1019; SEQ ID No. 1021; SEQ ID No. 1023; SEQ ID No. 1024; SEQ ID No. 1029; SEQ ID No. 1031; SEQ ID No. 1033; SEQ ID No. 1034; SEQ ID No. 1039; SEQ ID No. 1041; SEQ ID No. 1042; SEQ ID No. 1045; SEQ ID No. 1047; SEQ ID No. 1049; SEQ ID No. 1051; SEQ ID No. 1052; SEQ ID No. 1053; SEQ ID No. 1054; SEQ ID No. 1056; SEQ ID No. 1059; SEQ ID No. 1061; SEQ ID No. 1062; SEQ ID No. 1063; SEQ ID No. 1064; SEQ ID No. 1065; SEQ ID No. 1067; SEQ ID No. 1075; SEQ ID No. 1077; SEQ ID No. 1078; SEQ ID No. 1079; SEQ ID No. 1080; SEQ ID No. 1081; SEQ ID No. 1089; SEQ ID No. 1095; SEQ ID No. 1097; SEQ ID No. 1098; SEQ ID No. 1099; SEQ ID No. 1101; SEQ ID No. 1102; SEQ ID No. 1103; SEQ ID No. 1106; SEQ ID No. 1107; SEQ ID No. 1108; SEQ ID No. 1109; SEQ ID No. 1110; SEQ ID No. 1113; SEQ ID No. 1116; SEQ ID No. 1118; SEQ ID No. 1119; SEQ ID No. 1121; SEQ ID No. 1123; SEQ ID No. 1124; SEQ ID No. 1126; SEQ ID No. 1128; SEQ ID No. 1130; SEQ ID No. 1131; SEQ ID No. 1133; SEQ ID No. 1134; SEQ ID No. 1136; SEQ ID No. 1137 and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, characterized in that it is a


Chlamydia pneumoniae


transmembrane polypeptide or one of its representative fragments, having between 4 and 6 transmembrane domains, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 5; SEQ ID No. 7; SEQ ID No. 8; SEQ ID No. 15; SEQ ID No. 36; SEQ ID No. 38; SEQ ID No. 51; SEQ ID No. 55; SEQ ID No. 58; SEQ ID No. 67; SEQ ID No. 70; SEQ ID No. 81; SEQ ID No. 97; SEQ ID No. 110; SEQ ID No. 111; SEQ ID No. 115; SEQ ID No. 119; SEQ ID No. 126; SEQ ID No. 128; SEQ ID No. 148; SEQ ID No. 155; SEQ ID No. 163; SEQ ID No. 165; SEQ ID No. 168; SEQ ID No. 169; SEQ ID No. 171; SEQ ID No. 172; SEQ ID No. 174; SEQ ID No. 177; SEQ ID No. 181; SEQ ID No. 193; SEQ ID No. 203; SEQ ID No. 213; SEQ ID No. 214; SEQ ID No. 216; SEQ ID No. 217; SEQ ID No. 221; SEQ ID No. 222; SEQ ID No. 225; SEQ ID No. 229; SEQ ID No. 243; SEQ ID No. 246; SEQ ID No. 248; SEQ ID No. 254; SEQ ID No. 261; SEQ ID No. 285; SEQ ID No. 288; SEQ ID No. 292; SEQ ID No. 296; SEQ ID No. 298; SEQ ID No. 299; SEQ ID No. 301; SEQ ID No. 303; SEQ ID No. 317; SEQ ID No. 328; SEQ ID No. 329; SEQ ID No. 351; SEQ ID No. 354; SEQ ID No. 355; SEQ ID No. 364; SEQ ID No. 371; SEQ ID No. 374; SEQ ID No. 375; SEQ ID No. 391; SEQ ID No. 395; SEQ ID No. 401; SEQ ID No. 403; SEQ ID No. 405; SEQ ID No. 409; SEQ ID No. 414; SEQ ID No. 419; SEQ ID No. 421; SEQ ID No. 423; SEQ ID No. 425; SEQ ID No. 438; SEQ ID No. 448; SEQ ID No. 453; SEQ ID No. 458; SEQ ID No. 466; SEQ ID No. 468; SEQ ID No. 470; SEQ ID No. 480; SEQ ID No. 489; SEQ ID No. 490; SEQ ID No. 496; SEQ ID No. 501; SEQ ID No. 504; SEQ ID No. 505; SEQ ID No. 506; SEQ ID No. 511; SEQ ID No. 513; SEQ ID No. 519; SEQ ID No. 526; SEQ ID No. 532; SEQ ID No. 538; SEQ ID No. 539; SEQ ID No. 547; SEQ ID No. 550; SEQ ID No. 561; SEQ ID No. 568; SEQ ID No. 570; SEQ ID No. 574; SEQ ID No. 578; SEQ ID No. 579; SEQ ID No. 580; SEQ ID No. 582; SEQ ID No. 589; SEQ ID No. 593; SEQ ID No. 598; SEQ ID No. 601; SEQ ID No. 604; SEQ ID No. 610; SEQ ID No. 613; SEQ ID No. 617; SEQ ID No. 626; SEQ ID No. 632; SEQ ID No. 635; SEQ ID No. 638; SEQ ID No. 640; SEQ ID No. 641; SEQ ID No. 646; SEQ ID No. 649; SEQ ID No. 650; SEQ ID No. 651; SEQ ID No. 686; SEQ ID No. 711; SEQ ID No. 724; SEQ ID No. 732; SEQ ID No. 734; SEQ ID No. 744; SEQ ID No. 745; SEQ ID No. 749; SEQ ID No. 751; SEQ ID No. 769; SEQ ID No. 770; SEQ ID No. 771; SEQ ID No. 773; SEQ ID No. 776; SEQ ID No. 779; SEQ ID No. 780; SEQ ID No. 785; SEQ ID No. 787; SEQ ID No. 789; SEQ ID No. 801; SEQ ID No. 805; SEQ ID No. 812; SEQ ID No. 822; SEQ ID No. 825; SEQ ID No. 826; SEQ ID No. 839; SEQ ID No. 841; SEQ ID No. 843; SEQ ID No. 853; SEQ ID No. 861; SEQ ID No. 875; SEQ ID No. 876; SEQ ID No. 886; SEQ ID No. 893; SEQ ID No. 898; SEQ ID No. 906; SEQ ID No. 907; SEQ ID No. 908; SEQ ID No. 920; SEQ ID No. 922; SEQ ID No. 925; SEQ ID No. 933; SEQ ID No. 935; SEQ ID No. 936; SEQ ID No. 944; SEQ ID No. 946; SEQ ID No. 947; SEQ ID No. 954; SEQ ID No. 959; SEQ ID No. 961; SEQ ID No. 966; SEQ ID No. 967; SEQ ID No. 972; SEQ ID No. 978; SEQ ID No. 995; SEQ ID No. 996; SEQ ID No. 1000; SEQ ID No. 1003; SEQ ID No. 1010; SEQ ID No. 1011; SEQ ID No. 1012; SEQ ID No. 1017; SEQ ID No. 1020; SEQ ID No. 1030; SEQ ID No. 1036; SEQ ID No. 1038; SEQ ID No. 1043; SEQ ID No. 1046; SEQ ID No. 1048; SEQ ID No. 1050; SEQ ID No. 1058; SEQ ID No. 1071; SEQ ID No. 1073; SEQ ID No. 1084; SEQ ID No. 1085; SEQ ID No. 1086; SEQ ID No. 1087; SEQ ID No. 1091; SEQ ID No. 1092; SEQ ID No. 1094; SEQ ID No. 1096; SEQ ID No. 1100; SEQ ID No. 1104; SEQ ID No. 1111; SEQ ID No. 1112; SEQ ID No. 1114; SEQ ID No. 1117; SEQ ID No. 1122; SEQ ID No. 1125 and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, characterized in that it is a


Chlamydia pneumoniae


transmembrane polypeptide or one of its representative fragments, having at least 7 transmembrane domains, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 17; SEQ ID No. 52; SEQ ID No. 68; SEQ ID No. 83; SEQ ID No. 87; SEQ ID No. 109 ; SEQ ID No. 112; SEQ ID No. 113; SEQ ID No. 120; SEQ ID No. 121; SEQ ID No. 127; SEQ ID No. 153; SEQ ID No. 204; SEQ ID No. 211; SEQ ID No. 218; SEQ ID No. 223; SEQ ID No. 275; SEQ ID No. 277; SEQ ID No. 295; SEQ ID No. 300; SEQ ID No. 302; SEQ ID No. 306; SEQ ID No. 327; SEQ ID No. 335; SEQ ID No. 342; SEQ ID No. 343; SEQ ID No. 347; SEQ ID No. 349; SEQ ID No. 361; SEQ ID No. 363; SEQ ID No. 369; SEQ ID No. 380; SEQ ID No. 388; SEQ ID No. 389; SEQ ID No. 397; SEQ ID No. 415; SEQ ID No. 432; SEQ ID No. 439; SEQ ID No. 446; SEQ ID No. 449; SEQ ID No. 472; SEQ ID No. 478; SEQ ID No. 500; SEQ ID No. 522; SEQ ID No. 524; SEQ ID No. 567; SEQ ID No. 575; SEQ ID No. 602; SEQ ID No. 606; SEQ ID No. 609; SEQ ID No. 636; SEQ ID No. 639; SEQ ID No. 643; SEQ ID No. 653; SEQ ID No. 668; SEQ ID No. 692; SEQ ID No. 702; SEQ ID No. 704; SEQ ID No. 713; SEQ ID No. 720; SEQ ID No. 778; SEQ ID No. 784; SEQ ID No. 800; SEQ ID No. 836; SEQ ID No. 838; SEQ ID No. 842; SEQ ID No. 864; SEQ ID No. 867; SEQ ID No. 883; SEQ ID No. 901; SEQ ID No. 916; SEQ ID No. 932; SEQ ID No. 934; SEQ ID No. 940; SEQ ID No. 942; SEQ ID No. 950; SEQ ID No. 956; SEQ ID No. 971; SEQ ID No. 973; SEQ ID No. 976; SEQ ID No. 988; SEQ ID No. 994; SEQ ID No. 1018; SEQ ID No. 1028; SEQ ID No. 1035; SEQ ID No. 1037; SEQ ID No. 1044; SEQ ID No. 1055; SEQ ID No. 1057; SEQ ID No. 1068; SEQ ID No. 1069; SEQ ID No. 1070; SEQ ID No. 1072; SEQ ID No. 1082; SEQ ID No. 1088; SEQ ID No. 1105; SEQ ID No. 1132; SEQ ID No. 1135 and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, in that it is a


Chlamydia pneumoniae


surface exposed polypeptide or one of its representative fragments, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 15, SEQ ID No. 25, SEQ ID No. 26, SEQ ID No. 27, SEQ ID No. 28, SEQ ID No. 29, SEQ ID No. 30, SEQ ID No. 31, SEQ ID No. 32, SEQ ID No. 33, SEQ ID No. 35, SEQ ID No. 36, SEQ ID No. 1257, SEQ ID No. 280, SEQ ID No. 291, SEQ ID No. 314, SEQ ID No. 354, SEQ ID No. 380, SEQ ID No. 1266, SEQ ID No. 466, SEQ ID No. 467, SEQ ID No. 468, SEQ ID No. 469, SEQ ID No. 470, SEQ ID No. 472, SEQ ID No. 474, SEQ ID No. 476, SEQ ID No. 477, SEQ ID No. 478, SEQ ID No. 479, SEQ ID No. 480, SEQ ID No. 482, SEQ ID No. 483, SEQ ID No. 485, SEQ ID No. 486, SEQ ID No. 500, SEQ ID No. 501, SEQ ID No. 503, SEQ ID No. 504, SEQ ID No. 505, SEQ ID No. 506, SEQ ID No. 507, SEQ ID No. 1268, SEQ ID No. 1269, SEQ ID No. 543, SEQ ID No. 544, SEQ ID No. 578, SEQ ID No. 579, SEQ ID No. 580, SEQ ID No. 581, SEQ ID No. 595, SEQ ID No. 596, SEQ ID No. 597, SEQ ID No. 1271, SEQ ID No. 633, SEQ ID No. 637, SEQ ID No. 699, SEQ ID No. 706, SEQ ID No. 737, SEQ ID No. 744, SEQ ID No. 1273, SEQ ID No. 751, SEQ ID No. 775, SEQ ID No. 776, SEQ ID No. 777, SEQ ID No. 793, SEQ ID No. 815, SEQ ID No. 830, SEQ ID No. 1221, SEQ ID No. 849, SEQ ID No. 851, SEQ ID No. 852, SEQ ID No. 874, SEQ ID No. 891, SEQ ID No. 922, SEQ ID No. 940, SEQ ID No. 1231, SEQ ID No. 1281, SEQ ID No. 1035, SEQ ID No. 1079, SEQ ID No. 1087, SEQ ID No. 1108, and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, characterized in that it is a


Chlamydia pneumoniae


lipoprotein or one of its representative fragments, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 3, SEQ ID No. 10, SEQ ID No. 11, SEQ ID No. 16, SEQ ID No. 1254, SEQ ID No. 1255, SEQ ID No. 38, SEQ ID No. 1256, SEQ ID No. 62, SEQ ID No. 85, SEQ ID No. 1258, SEQ ID No. 115, SEQ ID No. 1151, SEQ ID No. 151, SEQ ID No. 1259, SEQ ID No. 173, SEQ ID No. 1261, SEQ ID No. 186, SEQ ID No. 194, SEQ ID No. 205, SEQ ID No. 214, SEQ ID No. 216, SEQ ID No. 217, SEQ ID No. 238, SEQ ID No. 1177, SEQ ID No. 280, SEQ ID No. 291, SEQ ID No. 317, SEQ ID No. 327, SEQ ID No. 354, SEQ ID No. 364, SEQ ID No. 367, SEQ ID No. 414, SEQ ID No. 432, SEQ ID No. 1192, SEQ ID No. 460, SEQ ID No. 1267, SEQ ID No. 1268, SEQ ID No. 520, SEQ ID No. 536, SEQ ID No. 1270, SEQ ID No. 576, SEQ ID No. 597, SEQ ID No. 603, SEQ ID No. 609, SEQ ID No. 637, SEQ ID No. 1272, SEQ ID No. 652, SEQ ID No. 1213, SEQ ID No. 699, SEQ ID No. 705, SEQ ID No. 706, SEQ ID No. 708, SEQ ID No. 711, SEQ ID No. 727, SEQ ID No. 1274, SEQ ID No. 800, SEQ ID No. 814, SEQ ID No. 825, SEQ ID No. 829, SEQ ID No. 830, SEQ ID No. 831, SEQ ID No. 844, SEQ ID No. 849, SEQ ID No. 1275, SEQ ID No. 1276, SEQ ID No. 1277, SEQ ID No. 872, SEQ ID No. 878, SEQ ID No. 880, SEQ ID No. 891, SEQ ID No. 892, SEQ ID No. 1278, SEQ ID No. 1279, SEQ ID No. 1280, SEQ ID No. 941, SEQ ID No. 942, SEQ ID No. 1282, SEQ ID No. 1283, SEQ ID No. 952, SEQ ID No. 988, SEQ ID No. 998, SEQ ID No. 1009, SEQ ID No. 1285, SEQ ID No. 1235, SEQ ID No. 1028, SEQ ID No. 1056, SEQ ID No. 1070, SEQ ID No. 1287, SEQ ID No. 1087, SEQ ID No. 1288, SEQ ID No. 1289, SEQ ID No. 1098, SEQ ID No. 1246, SEQ ID No. 1291, SEQ ID No. 1108, SEQ ID No. 1109, SEQ ID No. 1112, SEQ ID No. 1133, and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, in that it is a


Chlamydia pneucmoniae


polypeptide involved in lipopolysaccharide (LPS) biosynthesis, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 316, SEQ ID No. 564, SEQ ID No. 610, SEQ ID No. 647, SEQ ID No. 1211, SEQ ID No. 688, SEQ ID No. 924, and one of their representative fragments.




Preferably, the invention relates to additional LPS-related polypeptides according to the invention, in that it is:




(a) a


Chlamydia pneumoniae


KDO (3-deoxy-D-manno-octylosonic acid)-related polypeptide or one of its representative fragments, and in that it is chosen from the polypeptides having the following sequences: SEQ ID No. 177, SEQ ID No. 1156, SEQ ID No. 245, SEQ ID No. 767, and one of their representative fragments;




(b) a


Chlamydia pneumoniae


phosphomannomutase-related polypeptide or one of its representative fragments, and in that it is chosen from the polypeptides having the following sequences: SEQ ID No. 74, and its representative fragment;




(c) a


Chlamydia pneumoniae


phosphoglucomutase-related polypeptide or one of its representative fragments, and in that it is chosen from the polypeptides having the following sequences: SEQ ID No. 1286, SEQ ID No. 1039, and its representative fragment; and




(d) a


Chlamydia pneumoniae


lipid A component-related polypeptide or one of its representative fragments, and in that it is chosen from the polypeptides having the following sequences: SEQ ID No. 689, SEQ ID No. 690, SEQ ID No. 691, SEQ ID No. 1037, and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, in that it is a


Chlamydia pneumoniae


polypeptide or one of its representative fragments that contains an RGD sequence and is also an outer membrane protein, and in that it is chosen from the polypeptides having the following sequences: SEQ ID No. 468 and its representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, in that it is a


Chlamydia pneumoniae


polypeptide or one of its representative fragments that contains an RGD sequence that shows homology to cds1, cds2, and copN type III virulence loci in


Chlamydia Psitacci,


and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 350 and its representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, in that it is a


Chlamydia pneumoniae


polypeptide or one of its representative fragments that is cysteine-rich and contains RGD sequence, and in that it is chosen from the polypeptides having the following sequences: SEQ ID No. 1290, SEQ ID No. 6846, SEQ ID No. 6848, and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, in that it is a


Chlamydia pneumoniae


outer membrane polypeptide that contains cysteines in their first 30 amino acids and also contain an RGD sequence, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 105, SEQ ID No. 106, SEQ ID No. 114, SEQ ID No. 170, SEQ ID No. 171, SEQ ID No. 1264, SEQ ID No. 268, SEQ ID No. 1265, SEQ ID No. 350, SEQ ID No. 393, SEQ ID No. 394, SEQ ID No. 451, SEQ ID No. 452, SEQ ID No. 453, SEQ ID No. 473, SEQ ID No. 499, SEQ ID No. 515, SEQ ID No. 519, SEQ ID No. 525, SEQ ID No. 526, SEQ ID No. 538, SEQ ID No. 611, SEQ ID No. 645, SEQ ID No. 686, SEQ ID No. 700, SEQ ID No. 746, SEQ ID No. 755, SEQ ID No. 756, SEQ ID No. 757, SEQ ID No. 789, SEQ ID No. 814, SEQ ID No. 855, SEQ ID No. 856, SEQ ID No. 878, SEQ ID No. 957, SEQ ID No. 958, SEQ ID No. 989, SEQ ID No. 1290, and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, in that it is a


Chlamydia pneumoniae


polypeptide or one of its representative fragments that contains RGD sequences homologous to


Chlamydia trachomatis


polypeptides containing RGD sequences, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 114, SEQ ID No. 468, SEQ ID No. 755, SEQ ID No. 756, SEQ ID No. 757, SEQ ID No. 855, SEQ ID No. 856, SEQ ID No. 905, SEQ ID No. 913, SEQ ID No. 914, SEQ ID No. 915, and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, in that it is a


Chlamydia pneumoniae


Type III and non-Type III secreted polypeptide or one of its representative fragments, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 25, SEQ ID No. 28, SEQ ID No. 29, SEQ ID No. 33, SEQ ID No. 308, SEQ ID No. 309, SEQ ID No. 343, SEQ ID No. 344, SEQ ID No. 345, SEQ ID No. 367, SEQ ID No. 414, SEQ ID No. 415, SEQ ID No. 480, SEQ ID No. 550, SEQ ID No. 579, SEQ ID No. 580, SEQ ID No. 581, SEQ ID No. 597, SEQ ID No. 699, SEQ ID No. 744, SEQ ID No. 751, SEQ ID No. 776, SEQ ID No. 866, SEQ ID No. 874, SEQ ID No. 883, SEQ ID No. 884, SEQ ID No. 888, SEQ ID No. 891, SEQ ID No. 6845, and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, in that it is a


Chlamydia pneumoniae


cell wall anchored surface polypeptide or one of its representative fragments, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 267, SEQ ID No. 271, SEQ ID No. 419, SEQ ID No. 590, SEQ ID No. 932, SEQ ID No. 6844, SEQ ID No. 6847, and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, in that it is a


Chlamydia pneumoniae


polypeptide or one of its representative fragments not found in


Chlamydia trachomatis


(Blastp P>e


−10


), and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 7, SEQ ID No. 8, SEQ ID No. 9, SEQ ID No. 16, SEQ ID No. 17, SEQ ID No. 18, SEQ ID No. 19, SEQ ID No. 20, SEQ ID No. 21, SEQ ID No. 22, SEQ ID No. 1254, SEQ ID No. 23, SEQ ID No. 1255, SEQ ID No. 24, SEQ ID No. 1139, SEQ ID No. 1140, SEQ ID No. 46, SEQ ID No. 47, SEQ ID No. 51, SEQ ID No. 60, SEQ ID No. 1256, SEQ ID No. 61, SEQ ID No. 62, SEQ ID No. 63, SEQ ID No. 64, SEQ ID No. 1257, SEQ ID No. 65, SEQ ID No. 66, SEQ ID No. 67, SEQ ID No. 68, SEQ ID No. 1143, SEQ ID No. 1145, SEQ ID No. 83, SEQ ID No. 84, SEQ ID No. 1146, SEQ ID No. 85, SEQ ID No. 86, SEQ ID No. 87, SEQ ID No. 1258, SEQ ID No. 116, SEQ ID No. 117, SEQ ID No. 125, SEQ ID No. 1148, SEQ ID No. 143, SEQ ID No. 1150, SEQ ID No. 1151, SEQ ID No. 144, SEQ ID No. 145, SEQ ID No. 147, SEQ ID No. 148, SEQ ID No. 149, SEQ ID No. 150, SEQ ID No. 152, SEQ ID No. 1259, SEQ ID No. 162, SEQ ID No. 166, SEQ ID No. 1154, SEQ ID No. 167, SEQ ID No. 1261, SEQ ID No. 1156, SEQ ID No. 1157, SEQ ID No. 178, SEQ ID No. 179, SEQ ID No. 1158, SEQ ID No. 182, SEQ ID No. 183, SEQ ID No. 184, SEQ ID No. 185, SEQ ID No. 1159, SEQ ID No. 186, SEQ ID No. 1160, SEQ ID No. 187, SEQ ID No. 188, SEQ ID No. 189, SEQ ID No. 190, SEQ ID No. 1161, SEQ ID No. 1162, SEQ ID No. 191, SEQ ID No. 192, SEQ ID No. 194, SEQ ID No. 195, SEQ ID No. 1163, SEQ ID No. 196, SEQ ID No. 201, SEQ ID No. 202, SEQ ID No. 209, SEQ ID No. 212, SEQ ID No. 221, SEQ ID No. 224, SEQ ID No. 1167, SEQ ID No. 226, SEQ ID No. 227, SEQ ID No. 228, SEQ ID No. 229, SEQ ID No. 230, SEQ ID No. 231, SEQ ID No. 232, SEQ ID No. 1169, SEQ ID No. 1170, SEQ ID No. 1171, SEQ ID No. 234, SEQ ID No. 235, SEQ ID No. 236, SEQ ID No. 1172, SEQ ID No. 243, SEQ ID No. 251, SEQ ID No. 252, SEQ ID No. 1176, SEQ ID No. 253, SEQ ID No. 255, SEQ ID No. 254, SEQ ID No. 256, SEQ ID No. 1177, SEQ ID No. 1178, SEQ ID No. 262, SEQ ID No. 263, SEQ ID No. 1264, SEQ ID No. 278, SEQ ID No. 279, SEQ ID No. 1180, SEQ ID No. 280, SEQ ID No. 290, SEQ ID No. 291, SEQ ID No. 292, SEQ ID No. 296, SEQ ID No. 1181, SEQ ID No. 297, SEQ ID No. 298, SEQ ID No. 300, SEQ ID No. 1265, SEQ ID No. 322, SEQ ID No. 324, SEQ ID No. 325, SEQ ID No. 370, SEQ ID No. 1186, SEQ ID No. 371, SEQ ID No. 372, SEQ ID No. 1187, SEQ ID No. 373, SEQ ID No. 378, SEQ ID No. 1266, SEQ ID No. 382, SEQ ID No. 383, SEQ ID No. 384, SEQ ID No. 385, SEQ ID No. 386, SEQ ID No. 1188, SEQ ID No. 1189, SEQ ID No. 391, SEQ ID No. 392, SEQ ID No. 398, SEQ ID No. 400, SEQ ID No. 403, SEQ ID No. 1191, SEQ ID No. 423, SEQ ID No. 435, SEQ ID No. 445, SEQ ID No. 450, SEQ ID No. 1193, SEQ ID No. 456, SEQ ID No. 460, SEQ ID No. 461, SEQ ID No. 465, SEQ ID No. 1196, SEQ ID No. 471, SEQ ID No. 473, SEQ ID No. 475, SEQ ID No. 481, SEQ ID No. 484, SEQ ID No. 487, SEQ ID No. 488, SEQ ID No. 489, SEQ ID No. 490, SEQ ID No. 491, SEQ ID No. 492, SEQ ID No. 493, SEQ ID No. 494, SEQ ID No. 495, SEQ ID No. 496, SEQ ID No. 497, SEQ ID No. 498, SEQ ID No. 499, SEQ ID No. 502, SEQ ID No. 1267, SEQ ID No. 1268, SEQ ID No. 508, SEQ ID No. 510, SEQ ID No. 509, SEQ ID No. 512, SEQ ID No. 515, SEQ ID No. 519, SEQ ID No. 1197, SEQ ID No. 521, SEQ ID No. 1198, SEQ ID No. 522, SEQ ID No. 524, SEQ ID No. 528, SEQ ID No. 534, SEQ ID No. 537, SEQ ID No. 1269, SEQ ID No. 1270, SEQ ID No. 548, SEQ ID No. 551, SEQ ID No. 557, SEQ ID No. 1201, SEQ ID No. 1203, SEQ ID No. 562, SEQ ID No. 566, SEQ ID No. 593, SEQ ID No. 595, SEQ ID No. 600, SEQ ID No. 1271, SEQ ID No. 604, SEQ ID No. 611, SEQ ID No. 612 , SEQ ID No. 614, SEQ ID No. 616, SEQ ID No. 625, SEQ ID No. 627, SEQ ID No. 628, SEQ ID No. 629, SEQ ID No. 631, SEQ ID No. 641, SEQ ID No. 1272, SEQ ID No. 648, SEQ ID No. 1212, SEQ ID No. 663, SEQ ID No. 685, SEQ ID No. 707, SEQ ID No. 714, SEQ ID No. 715, SEQ ID No. 716, SEQ ID No. 717, SEQ ID No. 722, SEQ ID No. 746, SEQ ID No. 1273, SEQ ID No. 761, SEQ ID No. 764, SEQ ID No. 770, SEQ ID No. 1217, SEQ ID No. 783, SEQ ID No. 1274, SEQ ID No. 803, SEQ ID No. 815, SEQ ID No. 1220, SEQ ID No. 835, SEQ ID No. 1221, SEQ ID No. 844, SEQ ID No. 845, SEQ ID No. 846, SEQ ID No. 847, SEQ ID No. 848, SEQ ID No. 849, SEQ ID No. 850, SEQ ID No. 851, SEQ ID No. 1275, SEQ ID No. 852, SEQ ID No. 862, SEQ ID No. 1276, SEQ ID No. 1277, SEQ ID No. 873, SEQ ID No. 1223, SEQ ID No. 892, SEQ ID No. 919, SEQ ID No. 1225, SEQ ID No. 1278, SEQ ID No. 926, SEQ ID No. 1228, SEQ ID No. 1229, SEQ ID No. 1230, SEQ ID No. 1279, SEQ ID No. 1281, SEQ ID No. 1282, SEQ ID No. 1283, SEQ ID No. 948, SEQ ID No. 950, SEQ ID No. 949, SEQ ID No. 951, SEQ ID No. 980, SEQ ID No. 982, SEQ ID No. 1233, SEQ ID No. 999, SEQ ID No. 1000, SEQ ID No. 1001, SEQ ID No. 1002, SEQ ID No. 1008, SEQ ID No. 1285, SEQ ID No. 1235, SEQ ID No. 1016, SEQ ID No. 1019, SEQ ID No. 1027, SEQ ID No. 1036, SEQ ID No. 1241, SEQ ID No. 1048, SEQ ID No. 1049, SEQ ID No. 1050, SEQ ID No. 1053, SEQ ID No. 1054, SEQ ID No. 1064, SEQ ID No. 1076, SEQ ID No. 1091, SEQ ID No. 1288, SEQ ID No. 1093, SEQ ID No. 1289, SEQ ID No. 1101, SEQ ID No. 1103, SEQ ID No. 1245, SEQ ID No. 1246, SEQ ID No. 1247, SEQ ID No. 1290, SEQ ID No. 1291, SEQ ID No. 1115, SEQ ID No. 1116, SEQ ID No. 1118, SEQ ID No. 1120, SEQ ID No. 1249, SEQ ID No. 1121, SEQ ID No. 1250, SEQ ID No. 1126, SEQ ID No. 1251, SEQ ID No. 1127, SEQ ID No. 1128, SEQ ID No. 1130, SEQ ID No. 1129, SEQ ID No. 1131, SEQ ID No. 1136, SEQ ID No. 1253, SEQ ID No. 6844, SEQ ID No. 6846, SEQ ID No. 6847, SEQ ID No. 6848, and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, characterized in that it is a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the intermediate metabolism, in particular in the metabolism of sugars and/or of cofactors, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 2; SEQ ID No. 55; SEQ ID No. 56; SEQ ID No. 69; SEQ ID No. 75; SEQ ID No. 80; SEQ ID No. 100; SEQ ID No. 110; SEQ ID No. 114; SEQ ID No. 120; SEQ ID No. 121; SEQ ID No. 157; SEQ ID No. 160; SEQ ID No. 161; SEQ ID No. 172; SEQ ID No. 180; SEQ ID No. 181; SEQ ID No. 198; SEQ ID No. 200; SEQ ID No. 225; SEQ ID No. 248; SEQ ID No. 249; SEQ ID No. 276; SEQ ID No. 277; SEQ ID No. 318; SEQ ID No. 319; SEQ ID No. 320; SEQ ID No. 323; SEQ ID No. 331; SEQ ID No. 347; SEQ ID No. 375; SEQ ID No. 376; SEQ ID No. 381; SEQ ID No. 393; SEQ ID No. 394; SEQ ID No. 395; SEQ ID No. 396; SEQ ID No. 409; SEQ ID No. 446; SEQ ID No. 447; SEQ ID No. 448; SEQ ID No. 449; SEQ ID No. 513; SEQ ID No. 516; SEQ ID No. 571; SEQ ID No. 647; SEQ ID No. 662; SEQ ID No. 697; SEQ ID No. 718; SEQ ID No. 793; SEQ ID No. 794; SEQ ID No. 808; SEQ ID No. 809; SEQ ID No. 838; SEQ ID No. 839; SEQ ID No. 840; SEQ ID No. 853; SEQ ID No. 854; SEQ ID No. 918; SEQ ID No. 923; SEQ ID No. 929; SEQ ID No. 931; SEQ ID No. 938; SEQ ID No. 939; SEQ ID No. 958; SEQ ID No. 959; SEQ ID No. 960; SEQ ID No. 966; SEQ ID No. 995; SEQ ID No. 1021; SEQ ID No. 1040; SEQ ID No. 1041; SEQ ID No. 1042; SEQ ID No. 1085; SEQ ID No. 1100; SEQ ID No. 1 102; SEQ ID No. 1117; SEQ ID No. 1118; SEQ ID No. 1119; SEQ ID No. 1120; SEQ ID No. 1135 and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, characterized in that it is a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the intermediate metabolism of nucleotides or nucleic acids, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 77; SEQ ID No. 78; SEQ ID No. 138; SEQ ID No. 189; SEQ ID No. 190; SEQ ID No. 233; SEQ ID No. 246; SEQ ID No. 338; SEQ ID No. 412; SEQ ID No. 421; SEQ ID No. 438; SEQ ID No. 607; SEQ ID No. 648; SEQ ID No. 657; SEQ ID No. 740; SEQ ID No. 783; SEQ ID No. 967; SEQ ID No. 989; SEQ ID No. 990; SEQ ID No. 992; SEQ ID No. 1011; SEQ ID No. 1058; SEQ ID No. 1059; SEQ ID No. 1073; SEQ ID No. 1074 and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, characterized in that it is a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the metabolism of nucleic acids, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 14; SEQ ID No. 59; SEQ ID No. 70; SEQ ID No. 71; SEQ ID No. 97; SEQ ID No. 113; SEQ ID No. 137; SEQ ID No. 141; SEQ ID No. 169; SEQ ID No. 285; SEQ ID No. 287; SEQ ID No. 288; SEQ ID No. 313; SEQ ID No. 326; SEQ ID No. 358; SEQ ID No. 411; SEQ ID No. 443; SEQ ID No. 548; SEQ ID No. 569; SEQ ID No. 601; SEQ ID No. 651; SEQ ID No. 654; SEQ ID No. 658; SEQ ID No. 659; SEQ ID No. 664; SEQ ID No. 665; SEQ ID No. 694; SEQ ID No. 698; SEQ ID No. 704; SEQ ID No. 760; SEQ ID No. 762; SEQ ID No. 763; SEQ ID No. 786; SEQ ID No. 787; SEQ ID No. 788; SEQ ID No. 801; SEQ ID No. 802; SEQ ID No. 812; SEQ ID No. 819; SEQ ID No. 822; SEQ ID No. 870; SEQ ID No. 897; SEQ ID No. 898; SEQ ID No. 902; SEQ ID No. 908; SEQ ID No. 916; SEQ ID No. 954; SEQ ID No. 955; SEQ ID No. 961; SEQ ID No. 983; SEQ ID No. 996; SEQ ID No. 1007; SEQ ID No. 1012; SEQ ID No. 1013; SEQ ID No. 1014; SEQ ID No. 1015; SEQ ID No. 1038; SEQ ID No. 1137 and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, characterized in that it is a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the metabolism of amino acids or polypeptides, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 99; SEQ ID No. 111; SEQ ID No. 127; SEQ ID No. 134; SEQ ID No. 140; SEQ ID No. 174; SEQ ID No. 175; SEQ ID No. 176; SEQ ID No. 353; SEQ ID No. 377; SEQ ID No. 404; SEQ ID No. 523; SEQ ID No. 539; SEQ ID No. 559; SEQ ID No. 561; SEQ ID No. 586; SEQ ID No. 598; SEQ ID No. 609; SEQ ID No. 636; SEQ ID No. 687; SEQ ID No. 700; SEQ ID No. 701; SEQ ID No. 759; SEQ ID No. 790; SEQ ID No. 857; SEQ ID No. 861; SEQ ID No. 904; SEQ ID No. 936; SEQ ID No. 952; SEQ ID No. 962; SEQ ID No. 963; SEQ ID No. 964; SEQ ID No. 965; SEQ ID No. 991; SEQ ID No. 1003; SEQ ID No. 1004; SEQ ID No. 1005; SEQ ID No. 1018; SEQ ID No. 1067; SEQ ID No. 1110; SEQ ID No. 1111; SEQ ID No. 1112; SEQ ID No. 1114; SEQ ID No. 1121; SEQ ID No. 1122; SEQ ID No. 1123; SEQ ID No. 1124; SEQ ID No. 1125 and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, characterized in that it is a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the metabolism of polypeptides, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 4; SEQ ID No. 44; SEQ ID No. 45; SEQ ID No. 48; SEQ ID No. 54; SEQ ID No. 112; SEQ ID No. 130; SEQ ID No. 155; SEQ ID No. 163; SEQ ID No. 212; SEQ ID No. 257; SEQ ID No. 307; SEQ ID No. 343; SEQ ID No. 405; SEQ ID No. 416; SEQ ID No. 458; SEQ ID No. 540; SEQ ID No. 541; SEQ ID No. 542; SEQ ID No. 543; SEQ ID No. 544; SEQ ID No. 560; SEQ ID No. 594; SEQ ID No. 652; SEQ ID No. 699; SEQ ID No. 723; SEQ ID No. 747; SEQ ID No. 817; SEQ ID No. 827; SEQ ID No. 871; SEQ ID No. 909; SEQ ID No. 910; SEQ ID No. 911; SEQ ID No. 912; SEQ ID No. 1023; SEQ ID No. 1051; SEQ ID No. 1052; SEQ ID No. 1081 and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, characterized in that it is a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the metabolism of fatty acids, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 76; SEQ ID No. 284; SEQ ID No. 308; SEQ ID No. 309; SEQ ID No. 310; SEQ ID No. 311; SEQ ID No. 312; SEQ ID No. 425; SEQ ID No. 433; SEQ ID No. 565; SEQ ID No. 688; SEQ ID No. 690; SEQ ID No. 691; SEQ ID No. 767; SEQ ID No. 797; SEQ ID No. 894; SEQ ID No. 895; SEQ ID No. 994; SEQ ID No. 1020; SEQ ID No. 1030; SEQ ID No. 1033; SEQ ID No. 1034; SEQ ID No. 1046; SEQ ID No. 1047; SEQ ID No. 1057 and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, characterized in that it is a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the synthesis of the wall, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 49; SEQ ID No. 50; SEQ ID No. 177; SEQ ID No. 178; SEQ ID No. 245; SEQ ID No. 610; SEQ ID No. 972; SEQ ID No. 974; SEQ ID No. 978; SEQ ID No. 1037 and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, characterized in that it is a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the transcription, translation and/or maturation process, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 90; SEQ ID No. 92; SEQ ID No. 131; SEQ ID No. 151; SEQ ID No. 199; SEQ ID No. 333; SEQ ID No. 334; SEQ ID No. 336; SEQ ID No. 379; SEQ ID No. 589; SEQ ID No. 590; SEQ ID No. 619; SEQ ID No. 630; SEQ ID No. 649; SEQ ID No. 739; SEQ ID No. 741; SEQ ID No. 806; SEQ ID No. 821; SEQ ID No. 843; SEQ ID No. 968; SEQ ID No. 971; SEQ ID No. 1061 and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, characterized in that it is a


Chlamydia pneumoniae


ribosomal polypeptide or one of its representative fragments, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 93; SEQ ID No. 94; SEQ ID No. 95; SEQ ID No. 136; SEQ ID No. 259; SEQ ID No. 332; SEQ ID No. 348; SEQ ID No. 583; SEQ ID No. 584; SEQ ID No. 588; SEQ ID No. 591; SEQ ID No. 592; SEQ ID No. 663; SEQ ID No. 666; SEQ ID No. 667; SEQ ID No. 669; SEQ ID No. 670; SEQ ID No. 671; SEQ ID No. 672; SEQ ID No. 673; SEQ ID No. 674; SEQ ID No. 675; SEQ ID No. 676; SEQ ID No. 677; SEQ ID No. 678; SEQ ID No. 679; SEQ ID No. 680; SEQ ID No. 681; SEQ ID No. 683; SEQ ID No. 684; SEQ ID No. 738; SEQ ID No. 781; SEQ ID No. 1008; SEQ ID No. 1024; SEQ ID No. 1025; SEQ ID No. 1066 and one of their representative fragments.




Preferably, the invention also relates to a polypeptide according to the invention, characterized in that it is a


Chlamydia pneumoniae


transport polypeptide or one of its representative fragments, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 40; SEQ ID No. 41; SEQ ID No. 52; SEQ ID No. 105; SEQ ID No. 106; SEQ ID No. 107; SEQ ID No. 109; SEQ ID No. 133; SEQ ID No. 210; SEQ ID No. 211; SEQ ID No. 214; SEQ ID No. 215; SEQ ID No. 216; SEQ ID No. 217; SEQ ID No. 218; SEQ ID No. 219; SEQ ID No. 220; SEQ ID No. 223; SEQ ID No. 242; SEQ ID No. 260; SEQ ID No. 293; SEQ ID No. 299; SEQ ID No. 366; SEQ ID No. 369; SEQ ID No. 575; SEQ ID No. 602; SEQ ID No. 638; SEQ ID No. 639; SEQ ID No. 640; SEQ ID No. 643; SEQ ID No. 653; SEQ ID No. 702; SEQ ID No. 703; SEQ ID No. 724; SEQ ID No. 732; SEQ ID No. 855; SEQ ID No. 856; SEQ ID No. 901; SEQ ID No. 906; SEQ ID No. 933; SEQ ID No. 942; SEQ ID No. 1043; SEQ ID No. 1086; SEQ ID No. 1105 and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, characterized in that it is a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the virulence process, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 546; SEQ ID No. 550; SEQ ID No. 778; SEQ ID No. 779; SEQ ID No. 886 and one of their representative fragments.




Preferably, the invention relates to a polypeptide according to the invention, characterized in that it is a


Chlamydia pneumoniae


polypeptide or one of its representative fragments which is involved in the secretory system and/or which is secreted, and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 751; SEQ ID No. 874; SEQ ID No. 875; SEQ ID No. 876; SEQ ID No. 883; SEQ ID No. 884; SEQ ID No. 885 and one of their representative fragments.




The secreted polypeptides, including the Type III and other, non-Type III secreted polypeptides, of the present invention, as well as the corresponding nucleotide sequences, may be detected by techniques known to persons skilled in the art, such as for example the techniques using cloning combined with vectors allowing the expression of the said polypeptides fused to export markers such as the luc gene for luciferase or the PhoA gene for alkaline phosphatase.




Preferably, the invention relates to a polypeptide according to the invention, characterized in that it is a polypeptide specific to


Chlamydia pneumoniae


or one of its representative fragments(with a Blast E value of >10


−5


), and in that it is chosen from the polypeptides having the following sequences:




SEQ ID No. 7; SEQ ID No. 8; SEQ ID No. 17; SEQ ID No. 18; SEQ ID No. 19; SEQ ID No. 20; SEQ ID No. 22; SEQ ID No. 23; SEQ ID No. 24; SEQ ID No. 51; SEQ ID No. 60; SEQ ID No. 63; SEQ ID No. 65; SEQ ID No. 66; SEQ ID No. 67; SEQ ID No. 83; SEQ ID No. 84; SEQ ID No. 86; SEQ ID No. 87; SEQ ID No. 125; SEQ ID No. 143; SEQ ID No. 144; SEQ ID No. 179; SEQ ID No. 182; SEQ ID No. 184; SEQ ID No. 185; SEQ ID No. 187; SEQ ID No. 221; SEQ ID No. 252; SEQ ID No. 254;; SEQ ID No. 278; SEQ ID No. 279; SEQ ID No. 387; SEQ ID No. 388; SEQ ID No. 397; SEQ ID No. 1048; SEQ ID No. 1049; SEQ ID No. 1050; SEQ ID No. 1128; SEQ ID No. 1130; SEQ ID No. 1131 and one of their representative fragments.




In general, in the present invention, the functional group to which a polypeptide of the invention belongs, as well as its corresponding nucleotide sequence, may be determined either by comparative analogy with sequences already known, or by the use of standard techniques of biochemistry, of cytology combined with the techniques of genetic engineering such as immunoaffinity, localization by immunolabelling, differential extraction, measurement of enzymatic activity, study of the activity inducing or repressing expression or the study of expression in


E. coli.






It is clearly understood, on the one hand, that, in the present invention, the nucleotide sequences (ORF) and the amino acid sequences (SEQ ID No. 2 to SEQ ID No. 1291 and SEQ ID No. 6844 to SEQ ID No. 684) which are listed by functional group, are not exhaustive within the group considered. Moreover, it is also clearly understood that, in the present invention, a nucleotide sequence (ORF) or an amino acid sequence mentioned within a given functional group may also be part of another group taking into account, for example, the interrelationship between the groups listed. Accordingly, and as an example of this interrelationship, an exported and/or secreted polypeptide as well as its coding nucleotide sequence may also be involved in the


Chlamydia pneumoniae


virulence process by modifying the defense mechanism of the infected host cell, or a transmembrane polypeptide or its coding nucleotide sequence is also part of the polypeptides or coding nucleotide sequences of the cellular envelope.




The subject of the present invention is also the nucleotide and/or polypeptide sequences according to the invention, characterized in that the said sequences are recorded on a medium, called recording medium, whose type and nature facilitate the reading, the analysis and the exploitation of the said sequences. These media may of course also contain other information extracted from the present invention, such as in particular the analogies with already known sequences, such as those mentioned in Table 1 of the present description, and/or may contain, in addition, information relating to the nucleotide and/or polypeptide sequences of other microorganisms so as to facilitate the comparative analysis and the exploitation of the results obtained.




Among these recording media, computer-readable media, such as magnetic, optical, electrical and hybrid media such as, for example, floppy disks, CD-ROMs or recording cassettes, are preferred in particular.




The invention also relates to nucleotide sequences which can be used as primer or probe, characterized in that the said sequences are chosen from the nucleotide sequences according to the invention.




The invention relates, in addition, to the use of a nucleotide sequence according to the invention, as primer or probe, for the detection and/or amplification of nucleic acid sequences.




The nucleotide sequences according to the invention may thus be used to amplify nucleotide sequences, in particular by the PCR technique (polymerase chain reaction) (Erlich, 1989; Innis et al., 1990; Rolfs et al., 1991, and White et al., 1997).




These oligodeoxyribonucleotide or oligoribonucleotide primers correspond to representative nucleotide fragments, and are advantageously at least 8 nucleotides, preferably at least 12 nucleotides, 15 nucleotides and still more preferably at least 20 nucleotides long.




Other techniques for amplifying the target nucleic acid may be advantageously used as alternatives to PCR.




The nucleotide sequences of the invention, in particular the primers according to the invention, may also be used in other methods for amplifying a target nucleic acid, such as:




the TAS (Transcription-based Amplification System) technique described by Kwoh et al. in 1989;




the 3SR (Self-Sustained Sequence Replication) technique described by Guatelli et al. in 1990;




the NASBA (Nucleic Acid Sequence Based Amplification) technique described by Kievitis et al. in 1991;




the SDA (Strand Displacement Amplification) technique (Walker et al., 1992);




the TMA (Transcription Mediated Amplification) technique.




The polynucleotides of the invention may also be used in techniques for amplifying or for modifying the nucleic acid serving as probe, such as:




the LCR (Ligase Chain Reaction) technique described by Landegren et al. in 1988 and perfected by Barany et al. in 1991, which uses a thermostable ligase;




the RCR (Repair Chain Reaction) technique described by Segev in 1992;




the CPR (Cycling Probe Reaction) technique described by Duck et al. in 1990;




the Q-beta-replicase amplification technique described by Miele et al. in 1983 and perfected in particular by Chu et al. in 1986, Lizardi et al. in 1988, and then by Burg et al. as well as by Stone et al. in 1996.




The invention also relates to the nucleotide sequences of fragments which can be obtained by amplification with the aid of at least one primer according to the invention. The present invention encompasses both hybridization probes and primers. In general, the complementary probes should be of a length sufficient to form a stable hybrid complex with the target sequences . Primers, while complementary to the target sequences need not form stable hybridization complexes with the target sequences alone. Rather, primers form stable complexes with the target sequences in the presence of polymerase to permit extension of the primer.




In the case where the target polynucleotide to be detected is possibly an RNA, for example an mRNA, it will be possible to use, prior to the use of an amplification reaction with the aid of at least one primer according to the invention or to the use of a method of detection with the aid of at least one probe of the invention, a reverse transcriptase-type enzyme so as to obtain a cDNA from the RNA contained in the biological sample. The cDNA obtained will then serve as target for the primer(s) or the probe(s) used in the amplification or detection method according to the invention.




The detection probe will be chosen so that it hybridizes with the target sequence or the amplicon generated from the target sequence. Such a detection probe will advantageously have as sequence a sequence of at least 12 nucleotides, in particular of at least 20 nucleotides, and preferably at least 100 nucleotides.




The invention also comprises the nucleotide sequences which can be used as probe or primer according to the invention, characterized in that they are labelled with a radioactive compound or with a nonradioactive compound.




The nonlabelled nucleotide sequences may be used directly as probes or primers; however, the sequences are generally labelled with a radioactive element (


32


P,


35


S,


3


H,


125


I) or with a nonradioactive molecule (biotin, acetylaminofluorene, digoxigenin, 5-bromo-deoxyuridine, fluorescein) so as to obtain probes which can be used in numerous applications.




Examples of nonradioactive labelling of nucleotide sequences are described, for example, in French patent No. 78,10975 or by Urdea et al. or by Sanchez-Pescador et al. in 1988.




In the latter case, one of the labelling methods described in patents FR-2 422 956 and FR-2 518 755 may also be used.




The invention also relates to the nucleotide sequences of fragments which can be obtained by hybridization with the aid of at least one probe according to the invention.




The hybridization technique may be performed in various ways (Matthews et al., 1988). The most common method consists in immobilizing the nucleic acid extracted from


Chlamydia pneumoniae


cells on a support (such as nitrocellulose, nylon, polystyrene) and in incubating, under well-defined conditions, the target nucleic acid immobilized with the probe. After hybridization, the excess probe is removed and the hybrid molecules formed are detected by the appropriate method (measurement of the radioactivity, of the fluorescence or of the enzymatic activity linked to the probe).




The invention also comprises the nucleotide sequences according to the invention, characterized in that they are covalently or noncovalently immobilized on a support.




According to another advantageous embodiment of the nucleic sequences according to the invention, the latter may be used immobilized on a support and may thus serve to capture, through specific hybridization, the target nucleic acid obtained from the biological sample to be tested. If necessary, the solid support is separated from the sample and the hybridization complex formed between the so-called capture probe and the target nucleic acid is then detected by means of a second probe, called detection probe, labelled with an easily detectable element.




The nucleotide sequences according to the invention may also be used in new analytical systems, DNA chips, which allow sequencing, the study of mutations and of the expression of genes, and which are currently of interest given their very small size and their high capacity in terms of number of analyses.




The principle of the operation of these chips is based on molecular probes, most often oligonucleotides, which are attached onto a miniaturized surface, generally of the order of a few square centimetres. During an analysis, a sample containing fragments of a target nucleic acid to be analysed, for example DNA or RNA labelled, for example, after amplification, is deposited onto the DNA chip in which the support has been coated beforehand with probes. Bringing the labelled target sequences into contact with the probes leads to the formation, through hybridization, of a duplex according to the rule of pairing defined by J. D. Watson and F. Crick. After a washing step, analysis of the surface of the chip allows the effective hybridizations to be located by means of the signals emitted by the labels tagging the target. A hybridization fingerprint results from this analysis which, by appropriate computer processing, will make it possible to determine information such as the presence of specific fragments in the sample, the determination of sequences and the presence of mutations.




The chip consists of a multitude of molecular probes, precisely organized or arrayed on a solid support whose surface is miniaturized. It is at the centre of a system where other elements (imaging system, microcomputer) allow the acquisition and interpretation of a hybridization fingerprint.




The hybridization supports are provided in the form of flat or porous surfaces (pierced with wells) composed of various materials. The choice of a support is determined by its physicochemical properties, or more precisely, by the relationship between the latter and the conditions under which the support will be placed during the synthesis or the attachment of the probes or during the use of the chip. It is therefore necessary, before considering the use of a particular support (R. S. Matson et al., 1994), to consider characteristics such as its stability to pH, its physical strength, its reactivity and its chemical stability as well as its capacity to nonspecifically bind nucleic acids. Materials such as glass, silicon and polymers are commonly used. Their surface is, in a first step, called “functionalization”, made reactive towards the groups which it is desired to attach thereon. After the functionalization, so-called spacer molecules are grafted onto the activated surface. Used as intermediates between the surface and the probe, these molecules of variable size render unimportant the surface properties of the supports, which often prove to be problematic for the synthesis or the attachment of the probes and for the hybridization.




Among the hybridization supports, there may be mentioned glass which is used, for example, in the method of in situ synthesis of oligonucleotides by photochemical addressing developed by the company Affymetrix (E. L. Sheldon, 1993), the glass surface being activated by silane. Genosensor Consortium (P. Mérel, 1994) also uses glass slides carrying wells 3 mm apart, this support being activated with epoxysilane.




Polymers or silicon may also be mentioned among these hybridization supports. For example, the Andrein Mirzabekov team has developed a chip consisting of polyacrylamide squares polymerized on a silanized glass surface (G. Yershov et al., 1996). Several teams use silicon, in particular the IFOS laboratory of Ecole Centrale of Lyon which uses a silicon semiconductor substrate which is p-doped by introducing it into its crystalline structure atoms whose valency is different from that of silicon. Various types of metals, in particular gold and platinum, may also be used as support (Genosensor Consortium (K. Beattie et al., 1993)).




The probes according to the invention may be synthesized directly in situ on the supports of the DNA chips. This in situ synthesis may be carried out by photochemical addressing (developed by the company Affymax (Amsterdam, Holland) and exploited industrially by its subsidiary Affymetrix (United States)) or based on the VLSIPS (very large scale immobilized polymer synthesis) technology (S. P. A. Fodor et al., 1991) which is based on a method of photochemically directed combinatory synthesis and the principle of which combines solid-phase chemistry, the use of photolabile protecting groups and photolithography.




The probes according to the invention may be attached to the DNA chips in various ways such as electrochemical addressing, automated addressing or the use of probe printers (T. Livache et al., 1994; G. Yershov et al., 1996; J. Derisi et al., 1996, and S. Borman, 1996).




The revealing of the hybridization between the probes of the invention, deposited or synthesized in situ on the supports of the DNA chips, and the sample to be analysed, may be determined, for example, by measurement of fluorescent signals, by radioactive counting or by electronic detection.




The use of fluorescent molecules such as fluorescein constitutes the most common method of labelling the samples. It allows direct or indirect revealing of the hybridization and allows the use of various fluorochromes.




Affymetrix currently provides an apparatus or a scanner designed to read its Gene Chip™ chips. It makes it possible to detect the hybridizations by scanning the surface of the chip in confocal microscopy (R. J. Lipshutz et al., 1995). Other methods of detecting fluorescent signals have been tested: coupling of an epifluorescence microscope and a CCD camera (G. Yershov et al., 1996), the use of an optical fibre collecting system (E. L. Sheldon, 1993). A conventional method consists in carrying out an end labelling, with phosphorus 32, of the target sequences, by means of an appropriate apparatus, the Phosphorimager (marketed by Molecular Dynamics). The electronic detection is based on the principle that the hybridization of two nucleic acid molecules is accompanied by physical phenomena which can be quantified under certain conditions (system developed by Ecole Centrale of Lyon and called GEN-FET (GEN field effect transistor)). Genosensor Consortium and the company Beckman Instruments who are developing an electronic chip or Permittivity Chips™ may also be mentioned (K. Beattie et al., 1993).




The nucleotide sequences according to the invention may thus be used in DNA chips to carry out the analysis of mutations. This analysis is based on the production of chips capable of analysing each base of a nucleotide sequence according to the invention.




The nucleotide sequences according to the invention may also be used in DNA chips to carry out the analysis of the expression of the


Chlamydia pneumoniae


genes. This analysis of the expression of


Chlamydia pneumoniae


genes is based on the use of chips where probes of the invention, chosen for their specificity to characterize a given gene, are present (D. J. Lockhart et al., 1996; D. D. Shoemaker et al., 1996). For the methods of analysis of gene expression using the DNA chips, reference may, for example, be made to the methods described by D. J. Lockhart et al. (1996) and Sosnowsky et al. (1997) for the synthesis of robes in situ or for the addressing and the attachment of previously synthesized probes. The target sequences to be analysed are labelled and in general fragmented into sequences of about 50 to 100 nucleotides before being hybridized onto the chip. After washing as described, for example, by D. J. Lockhart et al. (1996) and application of different electric fields (Sosnowsky et al., 1997), the labelled compounds are detected and quantified, the hybridizations being carried out at least in duplicate. Comparative analyses of the signal intensities obtained with respect to the same probe for different samples and/or for different probes with the same sample, determine the differential expression of RNA or of DNA derived from the sample.




The nucleotide sequences according to the invention may, in addition, be used in DNA chips where other nucleotide probes specific for other microorganisms are also present, and may allow the carrying out of a serial test allowing rapid identification of the presence of a microorganism in a sample.




Accordingly, the subject of the invention is also the nucleotide sequences according to the invention, characterized in that they are immobilized on a support of a DNA chip.




The DNA chips, characterized in that they contain at least one nucleotide sequence according to the invention, immobilized on the support of the said chip, also form part of the invention.




The said chips will preferably contain several probes or nucleotide sequences of the invention of different length and/or corresponding to different genes so as to identify, with greater certainty, the specificity of the target sequences or the desired mutation in the sample to be analysed.




Accordingly, the analyses carried out by means of primers and/or probes according to the invention, immobilized on supports such as DNA chips, will make it possible, for example, to identify, in samples, mutations linked to variations such as intraspecies variations. These variations may be correlated or associated with pathologies specific to the variant identified and will make it possible to select the appropriate treatment.




The invention thus comprises a DNA chip according to the invention, characterized in that it contains, in addition, at least one nucleotide sequence of a microorganism different from


Chlamydia pneumoniae,


immobilized on the support of the said chip; preferably, the different microorganism will be chosen from an associated microorganism, a bacterium of the Chlamydia family, and a variant of the species


Chlamydia pneumoniae.






Another subject of the present invention is a vector for the cloning and/or the expression of a sequence, characterized in that it contains a nucleotide sequence according to the invention. Among the said vectors according to the invention, the vectors containing a nucleotide sequence encoding a polypeptide of the cellular, preferably outer, envelope of


Chlamydia pneumoniae


or one of its representative fragments, are preferred. In a specific embodiment, the vectors contain a nucleotide sequence encoding a


Chlamydia pneumoniae


secreted polypeptide or one of its representative fragments or encoding a transport polypeptide, a surface exposed polypeptide, a lipoprotein or one of its representative fragments, a polypeptide involved in lipopolysaccharide (LPS) biosynthesis, a Type III and non-Type III secreted polypeptide, a polypeptide containing RGD attachment sites, a cell wall anchored surface polypeptide, a polypeptide not found in


Chlamydia trachomatis,


a ribosomal polypeptide or a polypeptide involved in secretion, transcription, translation, maturation of proteins, a polypeptide involved in the synthesis of the wall, a polypeptide involved in the virulence, a polypeptide involved in the intermediate metabolism, in particular in the metabolism of sugars and/or of cofactors, a polypeptide involved in the metabolism of nucleotides, of amino acids, of nucleic acids or of fatty acids of


Chlamydia pneumoniae


or one of their representative fragments, or a polypeptide specific to


Chlamydia pneumoniae.






According to the invention, the vectors comprise the elements necessary to allow the expression and/or the secretion of the said nucleotide sequences in a given host cell, and form part of the invention. The vector should, in this case, comprise a promoter, signals for initiation and for termination of translation, as well as appropriate regions for regulation of transcription. It should be capable of being stably maintained in the host cell and may optionally possess particular signals specifying the secretion of the translated protein. These different elements are chosen according to the host cell used. To this effect, the nucleotide sequences according to the invention may be inserted into autonomously-replicating vectors within the chosen host, or integrative vectors in the chosen host.




Any of the standard methods known to those skilled in the art for the insertion of DNA fragments into a vector may be used to construct expression vectors containing a chimeric gene consisting of appropriate transcriptional/translational control signals and the protein coding sequences. These methods may include in vitro recombinant DNA and synthetic techniques and in vivo recombinants (genetic recombination).




Expression of a polypeptide, peptide or derivative, or analogs thereof encoded by a polynucleotide sequence in SEQ ID No. 1 or ORFs contained within SEQ ID No. 1 may be regulated by a second nucleic acid sequence so that the protein or peptide is expressed in a host transformed with the recombinant DNA molecule. For example, expression of a protein or peptide may be controlled by any promoter/enhancer element known in the art. Promoters which may be used to control expression include, but are not limited to, the CMV promoter, the SV40 early promoter region (Bernoist and Chambon, 1981, Nature 290:304-310), the promoter contained in the 3′ long terminal repeat of Rous sarcoma virus (Yamamoto, et al., 1980, Cell 22:787-797), the herpes thymidine kinase promoter (Wagner et al., 1981, Proc. Natl. Acad. Sci. U.S.A. 78:1441-1445), the regulatory sequences of the metallothionein gene (Brinster et al., 1982, Nature 296:39-42); prokaryotic expression vectors such as the $-lactamase promoter (Villa-Kamaroff, et al., 1978, Proc. Natl. Acad. Sci. U.S.A. 75:3727-3731), or the tac promoter (DeBoer, et al., 1983, Proc. Natl. Acad. Sci. U.S.A. 80:21-25); see also “Useful proteins from recombinant bacteria” in Scientific American, 1980, 242:74-94; plant expression vectors comprising the nopaline synthetase promoter region (Herrera-Estrella et al., 1983, Nature 303:209-213) or the cauliflower mosaic virus 35S RNA promoter (Gardner, et al., 1981, Nucl. Acids Res. 9:2871), and the promoter of the photosynthetic enzyme ribulose biphosphate carboxylase (Herrera-Estrella et al., 1984, Nature 310:115-120); promoter elements from yeast or other fungi such as the Gal 4 promoter, the ADC (alcohol dehydrogenase) promoter, PGK (phosphoglycerol kinase) promoter, alkaline phosphatase promoter, and the following animal transcriptional control regions, which exhibit tissue specificity and have been utilized in transgenic animals: elastase I gene control region which is active in pancreatic acinar cells (Swift et al., 1984, Cell 38:639-646; Ornitz et al., 1986, Cold Spring Harbor Symp. Quant. Biol. 50:399-409; MacDonald, 1987, Hepatology 7:425-515); insulin gene control region which is active in pancreatic beta cells (Hanahan, 1985, Nature 315:115-122), immunoglobulin gene control region which is active in lymphoid cells (Grosschedl et al., 1984, Cell 38:647-658; Adames et al., 1985, Nature 318:533-538; Alexander et al., 1987, Mol. Cell. Biol. 7:1436-1444), mouse mammary tumor virus control region which is active in testicular, breast, lymphoid and mast cells (Leder et al., 1986, Cell 45:485-495), albumin gene control region which is active in liver (Pinkert et al., 1987, Genes and Devel. 1:268-276), alpha-fetoprotein gene control region which is active in liver (Krumlauf et al., 1985, Mol. Cell. Biol. 5:1639-1648; Hammer et al., 1987, Science 235:53-58; alpha 1-antitrypsin gene control region which is active in the liver (Kelsey et al., 1987, Genes and Devel. 1:161-171), beta-globin gene control region which is active in myeloid cells (Mogram et al., 1985, Nature 315:338-340; Kollias et al., 1986, Cell 46:89-94; myelin basic protein gene control region which is active in oligodendrocyte cells in the brain (Readhead et al., 1987, Cell 48:703-712); myosin light chain-2 gene control region which is active in skeletal muscle (Sani, 1985, Nature 314:283-286), and gonadotropic releasing hormone gene control region which is active in the hypothalamus (Mason et al., 1986, Science 234:1372-1378).




The vectors according to the invention are, for example, vectors of plasmid or viral origin. In a specific embodiment, a vector is used that comprises a promoter operably linked to a protein or peptide-encoding a nucleic acid sequence in SEQ ID No. 1, or ORFs contained within SEQ ID No. 1, one or more origins of replication, and, optionally, one or more selectable markers (e.g., an antibiotic resistance gene). Expression vectors comprise regulatory sequences that control gene expression, including gene expression in a desired host cell. Preferred vectors for the expression of the polypeptides of the invention include the pET-type plasmid vectors (Promega) or pBAD plasmid vectors (Invitrogen). Furthermore, the vectors according to the invention are useful for transforming host cells so as to clone or express the nucleotide sequences of the invention.




Expression can also be achieved using targeted homologous recombination to activate


Chlamydia pneumoniae


genes present in the cloned genomic DNA. A heterologous regulatory element may be inserted into a stable cell line or cloned microorganism, such that it is operatively linked with an endogenous


Chlamydia pneumoniae


gene present in the cloned genome, using techniques, such as targeted homologous recombination, which are well known to those of skill in the art (See, e.g., Chappel, U.S. Pat. No. 4,215,051 and Skoultchi, WO 91/06667 each of which is incorporated herein in its entirety).




Expression vector/host cell systems containing inserts of polynucleotide sequences in SEQ ID No. 1 or ORFs within SEQ ID No. 1, which encode polypeptides, peptides or derivatives, or analogs thereof, can be identified by three general approaches: (a) nucleic acid hybridization, (b) presence or absence of “marker” gene functions, and (c) expression of inserted sequences. In the first approach, the presence of a polynucleotide sequence inserted in an expression vector can be detected by nucleic acid hybridization using probes comprising sequences that are homologous to an inserted polynucleotide sequence. In the second approach, the recombinant vector/host system can be identified and selected based upon the presence or absence of certain “marker” gene functions (e.g., thymidine kinase activity, resistance to antibiotics, transformation phenotype, occlusion body formation in baculovirus, etc.) caused by the insertion of a polynucleotide sequence in the vector. For example, if the polynucleotide sequence in SEQ ID No. 1 or ORFs within SEQ ID No. 1 is inserted within the marker gene sequence of the vector, recombinants containing the insert can be identified by the absence of the marker gene function. In the third approach, recombinant expression vectors can be identified by assaying the product of the polynucleotide sequence expressed by the recombinant. Such assays can be based, for example, on the physical or functional properties of the expressed polypeptide in in vitro assay systems, e.g., binding with antibody, promotion of cell proliferation.




Once a particular recombinant DNA molecule is identified and isolated, several methods known in the art may be used to propagate it. The clones identified may be introduced into an appropriate host cell by standard methods, such as for example lipofection, electroporation, and heat shock. Once a suitable host system and growth conditions are established, recombinant expression vectors can be propagated and prepared in quantity.




The invention also encompasses the host cells transformed by a vector according to the invention. These cells may be obtained by introducing into host cells a nucleotide sequence inserted into a vector as defined above, and then culturing the said cells under conditions allowing the replication and/or the expression of the transfected nucleotide sequence.




The host cell may be chosen from eukaryotic or prokaryotic systems, such as for example bacterial cells (Olins and Lee, 1993), but also yeast cells (Buckholz, 1993), as well as animal cells, in particular cultures of mammalian cells (Edwards and Aruffo, 1993), and in particular Chinese hamster ovary (CHO) cells, but also insect cells in which methods using baculoviruses for example may be used (Luckow, 1993).




Furthermore, a host cell strain may be chosen which modulates the expression of the inserted sequences, or modifies and processes the gene product in the specific fashion desired. Expression from certain promoters can be elevated in the presence of certain inducers; thus, expression of the genetically engineered polypeptide may be controlled. Furthermore, different host cells have characteristic and specific mechanisms for the translational and post-translational processing and modification (e.g., glycosylation, phosphorylation) of proteins. Appropriate cell lines or host systems can be chosen to ensure the desired modification and processing of the foreign protein expressed. For example, expression in a bacterial system can be used to produce an unglycosylated core protein product. Expression in yeast will produce a glycosylated product. Expression in mammalian cells can be used to ensure “native” glycosylation of a heterologous protein. Furthermore, different vector/host expression systems may effect processing reactions to different extents.




A preferred host cell for the expression of the proteins of the invention consists of prokaryotic cells, such as Gram bacteria. A further preferred host cell according to the invention is a bacterium belonging to the Chlamydia family, more preferably belonging to the species


Chlamydia pneumoniae


or chosen from a microorganism associated with the species


Chlamydia pneumoniae.






In other specific embodiments, the polypeptides, peptides or derivatives, or analogs thereof may be expressed as a fusion, or chimeric protein product (comprising the protein, fragment, analog, or derivative joined via a peptide bond to a heterologous protein sequence (of a different protein)). Such a chimeric product can be made by ligating the appropriate nucleic acid sequences encoding the desired amino acid sequences to each other by methods known in the art, in the proper coding frame, and expressing the chimeric product by methods commonly known in the art. Alternatively, such a chimeric product may be made by protein synthetic techniques, e.g., by use of a peptide synthesizer.




Genomic sequences can be cloned and expressed as translational gene products (i.e., peptides, polypeptides, and proteins) or transcriptional gene products (i.e., antisense and ribozymes).




The invention further relates to the intracellular production of an antisense nucleic acid sequence of SEQ ID No. 1 by transcription from an exogenous sequence. For example, a vector can be introduced in vivo such that it is taken up by a cell, within which cell the vector or a portion thereof is transcribed, producing an antisense nucleic acid (RNA) of the invention. Such a vector would contain a sequence encoding an antisense nucleic acid. Such a vector can remain episomal or become chromosomally integrated, as long as it can be transcribed to produce the desired antisense RNA. Such vectors can be constructed by recombinant DNA technology methods standard in the art. Vectors can be plasmid, viral, or others known in the art, used for replication and expression in mammalian cells. Expression of the sequence encoding the an antisense RNA can be by any promoter known in the art to act in mammalian, preferably human, cells. Such promoters can be inducible or constitutive. Such promoters include but are not limited to: the CMV promoter, the SV40 early promoter region (Bernoist and Chambon, 1981, Nature 290:304-310), the promoter contained in the 3N long terminal repeat of Rous sarcoma virus (Yamamoto et al., 1980, Cell 22:787-797), the herpes thymidine kinase promoter (Wagner et al., 1981, Proc. Natl. Acad. Sci. U.S.A. 78:1441-1445), the regulatory sequences of the metallothionein gene (Brinster et al., 1982, Nature 296:39-42), etc.




In a specific embodiment, the antisense oligonucleotide comprises catalytic RNA, or a ribozyme (see, e.g., PCT International Publication WO 90/11364, published Oct. 4, 1990; Sarver et al., 1990, Science 247:1222-1225). In another embodiment, the oligonucleotide is a 2N-0-methylribonucleotide (Inoue et al., 1987, Nucl. Acids Res. 15:6131-6148), or a chimeric RNA-DNA analog (Inoue et al., 1987, FEBS Lett. 215:327-330).




In another embodiment, the antisense nucleic acids of the invention comprise a sequence complementary to at least a portion of an RNA transcript of a polynucleotide sequence in SEQ ID No. 1. However, absolute complementarity, although preferred, is not required. A sequence “complementary to at least a portion of an RNA,” as referred to herein, means a sequence having sufficient complementarity to be able to hybridize with the RNA, forming a stable duplex; in the case of double-stranded antisense nucleic acid sequence, a single strand of the duplex DNA may thus be tested, or triplex formation may be assayed. The ability to hybridize will depend on both the degree of complementarity and the length of the antisense nucleic acid. Generally, the longer the hybridizing nucleic acid, the more base mismatches with an RNA transcribed from SEQ ID No. 1 may contain and still form a stable duplex (or triplex, as the case may be). One skilled in the art can ascertain a tolerable degree of mismatch by use of standard procedures to determine the melting point of the hybridized complex.




The invention also relates to the animals, except humans, comprising one of the above-described transformed cells according to the invention.




The production of transgenic animals according to the invention overexpressing one or more of the


Chlamydia pneumoniae


genes will be preferably carried out on rats, mice or rabbits according to methods well known to persons skilled in the art such as viral or nonviral transfections. The transgenic animals overexpressing one or more of the said genes may be obtained by transfection of multiple copies of the said genes under the control of a powerful promoter of a ubiquitous nature, or which is selective for one type of tissue. The transgenic animals may also be obtained by homologous recombination on embryonic stem cells, transfer of these stem cells to embryos, selection of the chimeras affected at the level of the reproductive lines, and growth of the said chimeras.




The transformed cells as well as the transgenic animals according to the invention can be used in methods of preparing the recombinant polypeptide.




It is now possible to produce recombinant polypeptides in a relatively large quantity by genetic engineering using the cells transformed with expression vectors according to the invention or using transgenic animals according to the invention.




The methods of preparing a polypeptide of the invention in recombinant form, characterized in that they use a vector and/or a cell transformed with a vector according to the invention and/or a transgenic animal comprising one of the said transformed cells according to the invention, are themselves included in the present invention.




Among the said methods of preparing a polypeptide of the invention in recombinant form, the methods of preparation using a vector, and/or a cell transformed with the said vector and/or a transgenic animal comprising one of the said transformed cells, containing a nucleotide sequence encoding a polypeptide of the cellular envelope of


Chlamydia pneumoniae


or one of its representative fragments, more preferably encoding a polypeptide of the outer cellular envelope of


Chlamydia pneumoniae


or one of its fragment, are preferred.




Among the said methods of preparing a polypeptide of the invention in recombinant form, the methods of preparation using a vector, and/or a cell transformed with the said vector and/or a transgenic animal comprising one of the said transformed cells, containing a nucleotide sequence encoding a


Chlamydia pneumoniae


secreted polypeptide or one of its representative fragments or encoding a transport polypeptide, a surface exposed polypeptide, a lipoprotein or one of its representative fragments, a polypeptide involved in lipopolysaccharide biosynthesis, a Type III or other secreted polypeptide, a polypeptide containing RGD attachment sites, a cell wall anchored surface polypeptide, a polypeptide not found in


Chlamydia trachomatis,


a ribosomal polypeptide or a polypeptide involved in secretion, transcription, translation, maturation of proteins, a polypeptide involved in the synthesis of the wall, a polypeptide involved in the virulence, a polypeptide involved in the intermediate metabolism, in particular in the metabolism of sugars and/or of cofactors, a polypeptide involved in the metabolism of nucleotides, of amino acids, of nucleic acids or of fatty acids of


Chlamydia pneumoniae


or one of their representative fragments, or a polypeptide specific to


Chlamydia pneumoniae,


are also preferred.




The recombinant polypeptides obtained as indicated above may be provided either in glycosylated or non-glycosylated form and may or may not have the natural tertiary structure.




A preferred variant consists in producing a recombinant polypeptide fused to a “carrier” protein (chimeric protein). The advantage of this system is that it allows a stabilization and a reduction in proteolysis of the recombinant product, an increase in solubility during renaturation in vitro and/or a simplification of purification when the fusion partner has affinity for a specific ligand.




More particularly, the invention relates to a method of preparing a polypeptide of the invention comprising the following steps:




a) culture of the transformed cells under conditions allowing the expression of a recombinant polypeptide having a nucleic acid sequence according to the invention;




b) where appropriate, recovery of the said recombinant polypeptide.




When the method of preparing a polypeptide of the invention uses a transgenic animal according to the invention, the recombinant polypeptide is then extracted from the said animal.




The subject of the invention is also a polypeptide capable of being obtained by a method of the invention as described above.




The invention also comprises a method of preparing a synthetic polypeptide, characterized in that it uses an amino acid sequence of polypeptides according to the invention.




The invention also relates to a synthetic polypeptide obtained by a method according to the invention.




Polypeptides according to the invention may also be prepared by conventional techniques in the field of peptide synthesis under conditions suitable to produce the polypeptides encoded by the polynucleotide of the invention.




This synthesis may be carried out in and recovered from a homogeneous solution or on a solid phase.




For example, the synthesis technique in a homogeneous solution described by Houbenweyl in 1974 may be used.




This method of synthesis consists in successively condensing, in pairs, the successive amino acids in the required order, or in condensing amino acids and fragments previously formed and already containing several amino acids in the appropriate order, or alternatively several fragments thus previously prepared, it being understood that care will have been taken to protect beforehand all the reactive functional groups carried by these amino acids or fragments, with the exception of the amine functional groups of one and the carboxyl functional groups of the other or vice versa, which should normally take part in the formation of the peptide bonds, in particular after activation of the carboxyl functional group, according to methods well known in peptide synthesis.




According to another preferred technique of the invention, the one described by Merrifield is used.




To manufacture a peptide chain according to the Merrifield method, a highly porous polymer resin is used, onto which the first C-terminal amino acid of the chain is attached. This amino acid is attached onto a resin via its carboxyl group and its amine functional group is protected. The amino acids which will constitute the peptide chain are thus attached, one after another, onto the amine group, each time deprotected beforehand, of the portion of the peptide chain already formed, and which is attached to the resin. When the entire peptide chain desired is formed, the protecting groups are removed from the various amino acids constituting the peptide chain and the peptide is detached from the resin with the aid of an acid.




The invention relates, in addition, to hybrid (fusion) polypeptides having at least one polypeptide or one of its representative fragments according to the invention, and a sequence of a polypeptide capable of eliciting an immune response in humans or animals.




Advantageously, the antigenic determinant is such that it is capable of eliciting a humoral and/or cellular response. An antigenic determinant may be identified by screening expression libraries of the


Chlamydia pneumoniae


genome with antibodies contained in the serum of patients infected with a bacterium belonging to the species


Chlamydia pneumoniae.


An antigenic determinant may comprise a polypeptide or one of its representative fragments according to the invention, in glycosylated form, used in order to obtain immunogenic compositions capable of inducing the synthesis of antibodies directed against multiple epitopes. The said polypeptides or their glycosylated fragments also form part of the invention.




These hybrid molecules may consist, in part, of a carrier molecule for polypeptides or for their representative fragments according to the invention, combined with a portion which may be immunogenic, in particular an epitope of the diphtheria toxin, the tetanus toxin, a hepatitis B virus surface antigen (patent FR 79 21811), the poliomyelitis virus VP1 antigen or any other viral or bacterial toxin or antigen.




The methods of synthesizing the hybrid molecules include the methods used in genetic engineering to construct hybrid nucleotide sequences encoding the desired polypeptide sequences. Reference may be advantageously made, for example, to the technique for producing genes encoding fusion proteins described by Minton in 1984.




The said hybrid nucleotide sequences encoding a hybrid polypeptide as well as the hybrid polypeptides according to the invention, characterized in that they are recombinant polypeptides obtained by the expression of the said hybrid nucleotide sequences, also form part of the invention.




The invention also comprises the vectors characterized in that they contain one of the said hybrid nucleotide sequences. The host cells transformed by the said vectors, the transgenic animals comprising one of the said transformed cells as well as the methods of preparing recombinant polypeptides using the said vectors, the said transformed cells and/or the said transgenic animals of course also form part of the invention.




The polypeptides according to the invention, the antibodies according to the invention described below and the nucleotide sequences according to the invention may advantageously be used in in vitro and/or in vivo methods for the detection and/or the identification of bacteria belonging to the species


Chlamydia pneumoniae,


in a biological sample (biological tissue or fluid) which is likely to contain them. These methods, depending on the specificity of the polypeptides, of the antibodies and of the nucleotide sequences according to the invention which will be used, may in particular detect and/or identify the bacterial variants belonging to the species


Chlamydia pneumoniae


as well as the associated microorganisms capable of being detected by the polypeptides, the antibodies and the nucleotide sequences according to the invention which will be chosen. It may, for example, be advantageous to choose a polypeptide, an antibody or a nucleotide sequence according to the invention, which is capable of detecting any bacterium of the Chlamydia family by choosing a polypeptide, an antibody and/or a nucleotide sequence according to the invention which is specific to the family or, on the contrary, it will be most particularly advantageous to target a variant of the species


Chlamydia pneumoniae,


which is responsible, for example, for the induction or the worsening of pathologies specific to the targeted variant, by choosing a polypeptide, an antibody and/or a nucleotide sequence according to the invention which is specific to the said variant.




The polypeptides according to the invention may advantageously be used in a method for the detection and/or the identification of bacteria belonging to the species


Chlamydia pneumoniae


or to an associated microorganism, in a biological sample (biological tissue or fluid) which is likely to contain them, characterized in that it comprises the following steps:




a) bringing this biological sample into contact with a polypeptide or one of its representative fragments according to the invention (under conditions allowing an immunological reaction between the said polypeptide and the antibodies which may be present in the biological sample);




b) detecting the antigen-antibody complexes which may be formed.




Preferably, the biological sample consists of a fluid, for example a human or animal serum, blood or biopsies.




Any conventional procedure may be used to carry out such a detection of the antigen-antibody complexes which may be formed.




By way of example, a preferred method uses immunoenzymatic procedures based on the ELISA technique, immunofluorescence procedures or radioimmunological procedures (RIA), and the like.




Accordingly, the invention also relates to the polypeptides according to the invention, labelled with the aid of a suitable label such as a label of the enzymatic, fluorescent or radioactive type.




Such methods comprise, for example, the following steps:




deposition of defined quantities of a polypeptide composition according to the invention into the wells of a microtitre plate,




introduction, into the said wells, of increasing dilutions of serum, or of a different biological sample as defined above, which has to be analysed,




incubation of the microplate,




introduction, into the wells of the microtitre plate, of labelled antibodies directed against human or animal immunoglobulins, these antibodies having been labelled with the aid of an enzyme selected from those which are capable of hydrolyzing a substrate, thereby modifying the absorption of the radiation of the latter, at least at a defined wavelength, for example at 550 nm,




detection, by comparison with a control, of the quantity of substrate hydrolyzed.




The invention also relates to a kit or set for the detection and/or the identification of bacteria belonging to the species


Chlamydia pneumoniae


or to an associated microorganism, characterized in that it comprises the following components:




a polypeptide according to the invention,




where appropriate, the reagents for constituting the medium appropriate for the immunological or specific reaction,




the reagents allowing the detection of the antigen-antibody complexes produced by the immunological reaction between the polypeptide(s) of the invention and the antibodies which may be present in the biological sample, it being possible for these reagents also to carry a label, or to be capable of being recognized in turn by a labelled reagent, more particularly in the case where the polypeptide according to the invention is not labelled,




where appropriate, a reference biological sample (negative control) free of antibodies recognized by a polypeptide according to the invention,




where appropriate, a reference biological sample (positive control) containing a predetermined quantity of antibodies recognized by a polypeptide according to the invention.




According to the invention, the polypeptides, peptides, fusion proteins or other derivatives, or analogs thereof encoded by a polynucleotide sequence in SEQ ID No. 1, may be used as an immunogen to generate antibodies which immunospecifically bind such an immunogen. Such antibodies may include, but are not limited to, polyclonal and monoclonal antibodies, humanized or chimeric antibodies, single chain antibodies, Fab fragments, F(ab′)


2


fragments, fragments produced by a Fab expression library, anti-idiotypic (anti-Id) antibodies, and epitope-binding fragments of any of the above. In a specific embodiment, the antibody to a polypeptide, peptide or other derivative, or analog thereof encoded by a polynucleotide sequence in SEQ ID No. 1 is a bispecific antibody (see generally, e.g. Fanger and Drakeman, 1995,


Drug News and Perspectives


8: 133-137). Such a bispecific antibody is genetically engineered to recognize both (1) an epitope and (2) one of a variety of “trigger” molecules, e.g. Fc receptors on myeloid cells, and CD3 and CD2 on T cells, that have been identified as being able to cause a cytotoxic T-cell to destroy a particular target. Such bispecific antibodies can be prepared either by chemical conjugation, hybridoma, or recombinant molecular biology techniques known to the skilled artisan.




Various procedures known in the art may be used for the production of polyclonal antibodies to a polypeptide, peptide or other derivative, or analog thereof encoded by a polynucleotide sequence in SEQ ID No. 1. For the production of antibody, various host animals can be immunized by injection with a polypeptide, or peptide or other derivative, or analog thereof, including but not limited to rabbits, mice, rats, etc. Various adjuvants, depending on the host species, may be used to increase the immunological response, including but not limited to Stimulon™ QS-21 (Aquila Biopharmaceuticals, Inc., Framingham, Mass.), MPL™ (3-O-deacylated monophosphoryl lipid A; RIBI ImmunoChem Research, Inc., Hamilton, Mont.), aluminum phosphate, IL-12 (Genetics Institute, Cambridge, Mass.), Freund's (complete and incomplete), mineral gels such as aluminum hydroxide, surface active substances such as lysolecithin, pluronic polyols, polyanions, peptides, oil emulsions, keyhole limpet hemocyanins, dinitrophenol, BCG (bacille Calmette-Guerin), and corynebacterium parvum. Alternatively, polyclonal antibodies may be prepared by purifying, on an affinity column onto which a polypeptide according to the invention has been previously attached, the antibodies contained in the serum of patients infected with a bacterium belonging to the species


Chlamydia pneumoniae.






For preparation of monoclonal antibodies directed toward a polypeptide, peptide or other derivative, or analog, any technique which provides for the production of antibody molecules by continuous cell lines in culture may be used. For example, the hybridoma technique originally developed by Kohler and Milstein (1975, Nature 256:495-497), as well as the trioma technique, the human B-cell hybridoma technique (Kozbor et al., 1983, Immunology Today 4:72), and the EBV-hybridoma technique to produce human monoclonal antibodies (Cole et al., 1985, in Monoclonal Antibodies and Cancer Therapy, Alan R. Liss, Inc., pp. 77-96). In an additional embodiment of the invention, monoclonal antibodies can be produced in germ-free animals utilizing technology described in PCT/US90/02545. In another embodiment of the invention, transgenic non-human animals can be used for the production of human antibodies utilizing technology described in WO 98/24893 and WO 96/33735. According to the invention, human antibodies may be used and can be obtained by using human hybridomas (Cote et al., 1983, Proc. Natl. Acad. Sci. U.S.A. 80:2026-2030) or by transforming human B cells with EBV virus in vitro (Cole et al., 1985, in


Monoclonal Antibodies and Cancer Therapy,


Alan R. Liss, pp. 77-96). In fact, according to the invention, techniques developed for the production of “chimeric antibodies” (Morrison et al., 1984, PROC. NATL. ACAD. SCI. U.S.A. 81:6851-6855; Neuberger et al., 1984, Nature 312:604-608; Takeda et al., 1985, Nature 314:452-454) by splicing the genes from a mouse antibody molecule specific for a polypeptide, peptide or other derivative, or analog together with genes from a human antibody molecule of appropriate biological activity can be used; such antibodies are within the scope of this invention.




According to the invention, techniques described for the production of single chain antibodies (U.S. Pat. No. 4,946,778) can be adapted to produce polypeptide or peptide-specific single chain antibodies. An additional embodiment of the invention utilizes the techniques described for the construction of Fab expression libraries (Huse et al., 1989, Science 246:1275-1281) to allow rapid and easy identification of monoclonal Fab fragments with the desired specificity for polypeptides, derivatives, or analogs.




Antibody fragments which contain the idiotype of the molecule can be generated by known techniques. For example, such fragments include but are not limited to: the F(ab′)


2


fragment which can be produced by pepsin digestion of the antibody molecule; the Fab′ fragments which can be generated by reducing the disulfide bridges of the F(ab′)


2


fragment, the Fab fragments which can be generated by treating the antibody molecule with papain and a reducing agent, and Fv fragments.




In addition, techniques have been developed for the production of chimerized (See, e.g., Boss, M. et al., U.S. Pat. No. 4,816,397; and Cabilly, S. et al., U.S. Pat. No. 5,585,089 each of which is incorporated herein by reference in its entirety) humanized antibodies (See, e.g., Queen, U.S. Pat. No. 5,585,089, which is incorporated herein by reference in its entirety.) An immunoglobulin light or heavy chain variable region consists of a “framework” region interrupted by three hypervariable regions, referred to as complementarily determining regions (CDRs). The extent of the framework region and CDRs have been precisely defined (See, “Sequences of Proteins of Immunological Interest”, Kabat, E. et al., U.S. Department of Health and Human Services (1983). Briefly, humanized antibodies are antibody molecules from non-human species having one or more CDRs from the non-human species and a framework from a human immunoglobulin molecule.




The antibodies of the invention may also be labelled in the same manner as described above for the nucleic probes of the invention such as an enzymatic, fluorescent or radioactive type labelling.




The invention relates, in addition, to a method for the detection and/or the identification of bacteria belonging to the species


Chlamydia pneumoniae


or to an associated microorganism in a biological sample, characterized in that it comprises the following steps:




a) bringing the biological sample (biological tissue or fluid) into contact with a mono- or polyclonal antibody according to the invention (under conditions allowing an immunological reaction between the said antibodies and the polypeptides of the bacterium belonging to the species


Chlamydia pneumoniae


or to an associated microorganism which may be present in the biological sample, that is, under conditions suitable for the formation of immune complexes);




b) detecting the antigen-antibody complex which may be formed.




Also falling within the scope of the invention is a kit or set for the detection and/or the identification of bacteria belonging to the species


Chlamydia pneumoniae


or to an associated microorganism, characterized in that it comprises the following components:




a polyclonal or monoclonal antibody according to the invention, labeled where appropriate;




where appropriate, a reagent for constituting the medium appropriate for carrying out the immunological reaction;




a reagent allowing the detection of the antigen-antibody complexes produced by the immunological reaction, it being possible for this reagent also to carry a label, or to be capable of being recognized in turn by a labelled reagent, more particularly in the case where the said monoclonal or polyclonal antibody is not labelled;




where appropriate, reagents for carrying out the lysis of the cells in the sample tested.




The principle of the DNA chip which was explained above may also be used to produce protein “chips” on which the support has been coated with a polypeptide or an antibody according to the invention, or arrays thereof, in place of the DNA. These protein “chips” make it possible, for example, to analyze the biomolecular interactions (BIA) induced by the affinity capture of target analytes onto a support coated, for example, with proteins, by surface plasma resonance (SPR). Reference may be made, for example, to the techniques for coupling proteins onto a solid support which are described in EP 524 800 or to the methods describing the use of biosensor-type protein chips such as the BIAcore-type technique (Pharmacia) (Arlinghaus et al., 1997, Krone et al., 1997, Chatelier et al., 1995). These polypeptides or antibodies according to the invention, capable of specifically binding antibodies or polypeptides derived from the sample to be analysed, may thus be used in protein chips for the detection and/or the identification of proteins in samples. The said protein chips may in particular be used for infectious diagnosis and may preferably contain, per chip, several polypeptides and/or antibodies of the invention of different specificity, and/or polypeptides and/or antibodies capable of recognizing microorganisms different from


Chlamydia pneumoniae.






Accordingly, the subject of the present invention is also the polypeptides and the antibodies according to the invention, characterized in that they are immobilized on a support, in particular of a protein chip.




The protein chips, characterized in that they contain at least one polypeptide or one antibody according to the invention immobilized on the support of the said chip, also form part of the invention.




The invention comprises, in addition, a protein chip according to the invention, characterized in that it contains, in addition, at least one polypeptide of a microorganism different from


Chlamydia pneumoniae


or at least one antibody directed against a compound of a microorganism different from


Chlamydia pneumoniae,


immobilized on the support of the said chip.




The invention also relates to a kit or set for the detection and/or the identification of bacteria belonging to the species


Chlamydia pneumoniae


or to an associated microorganism, or for the detection and/or the identification of a microorganism characterized in that it comprises a protein chip according to the invention.




The subject of the present invention is also a method for the detection and/or the identification of bacteria belonging to the species


Chlamydia pneumoniae


or to an associated microorganism in a biological sample, characterized in that it uses a nucleotide sequence according to the invention.




More particularly, the invention relates to a method for the detection and/or the identification of bacteria belonging to the species


Chlamydia pneumoniae


or to an associated microorganism in a biological sample, characterized in that it comprises the following steps:




a) where appropriate, isolation of the DNA from the biological sample to be analysed, or optionally production of a cDNA from the RNA in the biological sample;




b) specific amplification of the DNA of bacteria belonging to the species


Chlamydia pneumoniae


or to an associated microorganism with the aid of at least one primer according to the invention;




c) detection of the amplification products.




These may be detected, for example, by the molecular hybridization technique using a nucleic probe according to the invention. This probe will be advantageously labelled with a nonradioactive (cold probe) or radioactive element.




For the purposes of the present invention, “DNA in the biological sample” or “DNA contained in the biological sample” will be understood to mean either the DNA present in the biological sample considered, or optionally the cDNA obtained after the action of a reverse transcriptase-type enzyme on the RNA present in the said biological sample.




Another aim of the present invention consists in a method according to the invention, characterized in that it comprises the following steps:




a) bringing a nucleotide probe according to the invention into contact with a biological sample, the DNA contained in the biological sample having, where appropriate, been previously made accessible to hybridization, under conditions allowing the hybridization of the probe to complementary base pairs of the DNA of a bacterium belonging to the species


Chlamydia pneumoniae


or to an associated microorganism;




b) detecting the hybridization complex formed between the nucleotide probe and the DNA in the biological sample.




The present invention also relates to a method according to the invention, characterized in that it comprises the following steps:




a) bringing a nucleotide probe immobilized on a support according to the invention into contact with a biological sample, the DNA in the sample having, where appropriate, been previously made accessible to hybridization, under conditions allowing the hybridization of the probe to the DNA of a bacterium belonging to the species


Chlamydia pneumoniae


or to an associated microorganism;




b) bringing the hybrid formed between the nucleotide probe immobilized on a support and the DNA contained in the biological sample, where appropriate after removal of the DNA in the biological sample which has not hybridized with the probe, into contact with a labelled nucleotide probe according to the invention;




c) detecting the new hybrid formed in step b).




According to an advantageous embodiment of the method for the detection and/or the identification defined above, it is characterized in that, prior to step a), the DNA in the biological sample is primer-extended and/or amplified beforehand with the aid of at least one primer according to the invention.




The invention relates, in addition, to a kit or set for the detection and/or the identification of bacteria belonging to the species


Chlamydia pneumoniae


or to an associated microorganism, characterized in that it comprises the following components:




a) a nucleotide probe according to the invention;




b) where appropriate, the reagents necessary for carrying out a hybridization reaction;




c) where appropriate, at least one primer according to the invention as well as the reagents (e.g., polymerase and/or deoxynucleotide triphosphates) necessary for a DNA amplification reaction.




The invention also relates to a kit or set for the detection and/or the identification of bacteria belonging to the species


Chlamydia pneumoniae


or to an associated microorganism, characterized in that it comprises the following components:




a) a nucleotide probe, called capture probe, according to the invention;




b) an oligonucleotide probe, called detection probe, according to the invention;




c) where appropriate, at least one primer according to the invention as well as the reagents (e.g., polymerase and/or deoxynucleotide triphosphates) necessary for a DNA amplification reaction.




The invention also relates to a kit or set for the detection and/or the identification of bacteria belonging to the species


Chlamydia pneumoniae


or to an associated microorganism, characterized in that it comprises the following components:




a) at least one primer according to the invention;




b) where appropriate, the reagents necessary for carrying out a DNA amplification reaction;




c) where appropriate, a component which makes it possible to check the sequence of the amplified fragment, more particularly an oligonucleotide probe according to the invention.




The invention relates, in addition, to a kit or set for the detection and/or the identification of bacteria belonging to the species


Chlamydia pneumoniae


or to an associated microorganism, or for the detection and/or the identification of a microorganism characterized in that it comprises a DNA chip according to the invention.




The invention also relates to a method or to a kit or set according to the invention for the detection and/or the identification of bacteria belonging to the species


Chlamydia pneumoniae,


characterized in that the said primer and/or the said probe according to the invention are chosen from the nucleotide sequences specific to the species


Chlamydia pneumoniae,


in that the said polypeptides according to the invention are chosen from the polypeptides specific to the species


Chlamydia pneumoniae


and in that the said antibodies according to the invention are chosen from the antibodies directed against the polypeptides according to the invention chosen from the polypeptides specific to the species


Chlamydia pneumoniae.






Preferably, the said method or the said kit or set above according to the invention, for the detection and/or the identification of bacteria belonging to the species


Chlamydia pneumoniae


is characterized in that the said primer and/or the said probe or the said polypeptides are chosen from the nucleotide sequences or polypeptides according to the invention which have been identified as being specific to the species


Chlamydia pneumoniae


and in that the said antibodies according to the invention are chosen from the antibodies directed against the polypeptides according to the invention chosen from the polypeptides identified as being specific to the species


Chlamydia pneumoniae.






The invention relates, in addition, to a method or a kit or set according to the invention for the diagnosis of predispositions to, or of a condition caused by, cardiovascular diseases, preferably linked to the presence of atheroma, which are induced or worsened by a


Chlamydia pneumoniae


infection.




The invention also relates to a method or a kit or set according to the invention for the diagnosis of predispositions to, or of conditions caused by, respiratory diseases induced or worsened by a


Chlamydia pneumoniae


infection; preferably, the said respiratory disease is asthma.




According to another aspect, the subject of the invention is the use of polypeptides according to the invention, of cells transformed with a vector according to the invention and/or of transformed animals according to the invention, for the biosynthesis or the biodegradation of organic or inorganic compounds.




As has been mentioned above, the nucleotide sequences of the invention were identified by homology with sequences known to encode, for example, polypeptides or fragments of enzymatic polypeptides involved in the biosynthesis or the biodegradation of organic or inorganic molecules.




It is thus possible to use the said polypeptides of the invention in a similar manner for the biosynthesis or the biodegradation of organic or inorganic compounds of industrial or therapeutic interest (called compounds of interest).




Among these polypeptides, there may be mentioned in particular the enzymes involved in metabolism, such as the proteolytic enzymes, amino transferases, glucose metabolism, or the enzymes which may be used in the biosynthesis of sugars, amino acids, fatty acids, polypeptides, nucleotides, nucleic acids or any other organic or inorganic compound or in the biodegradation of organic or inorganic compounds.




Among these polypeptides, there may be mentioned, in addition, the mutated or modified enzymes corresponding to mutated or modified polypeptides according to the invention which may also be used for the biosynthesis or the biodegradation of organic or inorganic compounds at the industrial level, such as, for example, the production of compounds of interest, the reprocessing of manufacturing residues applied to the food industries, to the papermaking industry or to the chemical and pharmaceutical industries.




The methods of biosynthesis or biodegradation of organic or inorganic compounds, characterized in that they use a polypeptide or one of its representative fragments according to the invention, transformed cells according to the invention and/or a transformed animal according to the invention, also form part of the invention.




The invention relates, in addition, to the use of a nucleotide sequence according to the invention, of a polypeptide according to the invention, of an antibody according to the invention, of a cell according to the invention, and/or of a transformed animal according to the invention, for the selection of an organic or inorganic compound capable of modulating, regulating, inducing or inhibiting the expression of genes, and/or of modifying the cellular replication of eukaryotic or prokaryotic cells or capable of inducing, inhibiting or worsening the pathologies linked to an infection by


Chlamydia pneumoniae


or one of its associated microorganisms.




The invention also comprises screening assays that comprise methods of selecting compounds capable of binding to a polypeptide, fusion polypeptide or one of its representative fragments according to the invention, capable of binding to a nucleotide sequence according to the invention, or capable of recognizing an antibody according to the invention, and/or capable of modulating, regulating, inducing or inhibiting the expression of genes, and/or of modifying the growth or the cellular replication of eukaryotic or prokaryotic cells, or capable of inducing, inhibiting or worsening, in an animal or human organism, the pathologies linked to an infection by


Chlamydia pneumoniae


or one of its associated microorganisms, characterized in that it comprises the following steps:




a) bringing the said compound into contact with the said polypeptide, the said nucleotide sequence, with a transformed cell according to the invention and/or administering the said compound to a transformed animal according to the invention;




b) determining the capacity of the said compound to bind with the said polypeptide or the said nucleotide sequence, or to modulate, regulate, induce or inhibit the expression of genes, or to modulate growth or cellular replication, or to induce, inhibit or worsen in the said transformed animal, the pathologies linked to an infection by


Chlamydia pneumoniae


or one of its associated microorganisms.




The transformed cells and/or animals according to the invention may advantageously serve as a model and may be used in methods for studying, identifying and/or selecting compounds capable of being responsible for pathologies induced or worsened by


Chlamydia pneumoniae,


or capable of preventing and/or of treating these pathologies such as, for example, cardiovascular or respiratory diseases. In particular, the transformed host cells, in particular bacteria of the Chlamydia family whose transformation with a vector according to the invention may, for example, increase or inhibit its infectivity, or modulate the pathologies usually induced or worsened by the infection, may be used to infect animals in which the onset of pathologies will be monitored. These nontransformed animals, infected for example with transformed Chlamydia bacteria, may serve as a study model. In the same manner, the transformed animals according to the invention may, for example, exhibit predispositions to cardiovascular and/or respiratory diseases and thus be used in methods for selecting compounds capable of preventing and/or of treating the said diseases. The said methods using the said transformed cells and/or transformed animals form part of the invention.




The compounds capable of being selected may be organic compounds such as polypeptides or carbohydrates or any other organic or inorganic compounds already known, or new organic compounds produced using molecular modeling techniques and obtained by chemical or biochemical synthesis, these techniques being known to persons skilled in the art.




The said selected compounds may be used to modulate the growth and/or the cellular replication of


Chlamydia pneumoniae


or any other associated microorganism and thus to control infection by these microorganisms. The said compounds according to the invention may also be used to modulate the growth and/or the cellular replication of all eukaryotic or prokaryotic cells, in particular tumour cells and infectious microorganisms, for which the said compounds will prove active, the methods which make it possible to determine the said modulations being well known to persons skilled in the art.




Compound capable of modulating the growth of a microorganism is understood to designate any compound which makes it possible to act, to modify, to limit and/or to reduce the development, the growth, the rate of proliferation and/or the viability of the said microorganism.




This modulation may be achieved, for example, by an agent capable of binding to a protein and thus of inhibiting or of potentiating its biological activity, or capable of binding to a membrane protein of the outer surface of a microorganism and of blocking the penetration of the said microorganism into the host cell or of promoting the action of the immune system of the infected organism directed against the said microorganism. This modulation may also be achieved by an agent capable of binding to a nucleotide sequence of a DNA or RNA of a microorganism and of blocking, for example, the expression of a polypeptide whose biological or structural activity is necessary for the growth or for the reproduction of the said microorganism.




Associated microorganism is understood to designate in the present invention any microorganism whose gene expression may be modulated, regulated, induced or inhibited, or whose growth or cellular replication may also be modulated by a compound of the invention. Associated microorganism is also understood to designate in the present invention any microorganism containing nucleotide sequences or polypeptides according to the invention. These microorganisms may, in some cases, contain polypeptides or nucleotide sequences identical or homologous to those of the invention may also be detected and/or identified by the detection and/or identification methods or kit according to the invention and may also serve as a target for the compounds of the invention.




The invention relates to the compounds capable of being selected by a method of selection according to the invention.




The invention also relates to a pharmaceutical composition comprising a compound chosen from the following compounds:




a nucleotide sequence according to the invention;




a polypeptide according to the invention;




a vector according to the invention;




an antibody according to the invention; and




a compound capable of being selected by a method of selection according to the invention, optionally in combination with a pharmaceutically acceptable vehicle.




An effective quantity is understood to designate a sufficient quantity of the said compound or antibody, or of a polypeptide of the invention, which makes it possible to modulate the growth of


Chlamydia pneumoniae


or of an associated microorganism.




The invention also relates to a pharmaceutical composition comprising one or more polypeptides according to the invention and/or one or more fusion polypeptides according to the invention. Such compositions further comprise a pharmaceutically acceptable carrier or vehicle. Pharmaceutical compositions include compositions that comprise a polypeptide or fusion polypeptide that immunoreacts with seropositive serum of an individual infected with


Chlamydia pneumoniae.


In one embodiment, a pharmaceutical composition according to the invention can be utilized for the prevention or the treatment of an infection by a bacterium belonging to the species


Chlamydia pneumoniae


or by an associated microorganism.




The invention relates, in addition, to an immunogenic composition or a vaccine composition, characterized in that it comprises one or more polypeptides according to the invention and/or one or more hybrid (fusion) polypeptides according to the invention. Such compositions further comprise a pharmaceutically acceptable carrier or vehicle. Immunogenic compositions or fusion polypeptide include compositions that comprise a polypeptide that immunoreacts with seropositive serum of an individual infected with


Chlamydia pneumoniae.






Immunogenic or vaccine compositions can also comprise DNA immunogenic or vaccine compositions comprising polynucleotide sequences of the invention operatively associated with a regulatory sequence that controls gene expression. Such compositions can include compositions that direct expression of a neutralizing epitope of


Chlamydia pneumoniae.






The invention also comprises the use of a transformed cell according to the invention, for the preparation of a vaccine composition.




The invention also relates to a vaccine composition, characterized in that it contains a nucleotide sequence according to the invention, a vector according to the invention and/or a transformed cell according to the invention.




The invention also relates to the vaccine compositions according to the invention, for the prevention or the treatment of an infection by a bacterium belonging to the species


Chlamydia pneumoniae


or by an associated microorganism.




The invention also relates to the use of DNA encoding polypeptides of


Chlamydia pneumoniae,


in particular antigenic determinants, to be formulated as vaccine compositions. In accordance with this aspect of the invention, the DNA of interest is engineered into an expression vector under the control of regulatory elements, which will promote expression of the DNA, i.e., promoter or enhancer elements. In one preferred embodiment, the promoter element may be cell-specific and permit substantial transcription of the DNA only in predetermined cells. The DNA may be introduced directly into the host either as naked DNA (U.S. Pat. No. 5,679,647 incorporated herein by reference in their entirety) or formulated in compositions with other agents which may facilitate uptake of the DNA including viral vectors, i.e., adenovirus vectors, or agents which facilitate immunization, such as bupivicaine and other local anesthetics (U.S. Pat. No. 5,593,972 incorporated herein by reference in their entirety), saponins (U.S. Pat. No. 5,739,118 incorporated herein by reference in their entirety) and cationic polyamines (published international application WO 96/10038 incorporated herein by reference in their entirety).




The DNA sequence encoding the antigenic polypeptide and regulatory element may be inserted into a stable cell line or cloned microorganism, using techniques, such as targeted homologous recombination, which are well known to those of skill in the art, and described e.g., in Chappel, U.S. Pat. No. 4,215,051; Skoultchi, WO 91/06667 each of which is incorporated herein by reference in its entirety.




Such cell lines and microorganisms may be formulated for vaccine purposes. In yet another embodiment, the DNA sequence encoding the antigenic polypeptide and regulatory element may be delivered to a mammalian host and introduced into the host genome via homologous recombination (See, Chappel, U.S. Pat. No. 4,215,051; Skoultchi, WO 91/06667 each of which is incorporated herein by reference in its entirety.




Preferably, the immunogenic and/or vaccine compositions according to the invention intended for the prevention and/or the treatment of an infection by


Chlamydia pneumoniae


or by an associated microorganism will be chosen from the immunogenic and/or vaccine compositions comprising a polypeptide or one of its representative fragments corresponding to a protein, or one of its representative fragments, of the cellular envelope of


Chlamydia pneumoniae.


The vaccine compositions comprising nucleotide sequences will also preferably comprise nucleotide sequences encoding a polypeptide or one of its representative fragments corresponding to a protein, or one of its representative fragments, of the cellular envelope of


Chlamydia pneumoniae.






Among these preferred immunogenic and/or vaccine compositions, the most preferred are those comprising a polypeptide or one of its representative fragments, or a nucleotide sequence or one of its representative fragments hose sequences are chosen from the nucleotide or amino acid sequences identified in this functional group and listed above.




The polypeptides of the invention or their representative fragments entering into the immunogenic compositions according to the invention may be selected by techniques known to persons skilled in the art, such as for example on the capacity of the said polypeptides to stimulate T cells, which results, for example, in their proliferation or the secretion of interleukins, and which leads to the production of antibodies directed against the said polypeptides.




In mice, in which a weight dose of the vaccine composition comparable to the dose used in humans is administered, the antibody reaction is tested by collecting serum followed by a study of the formation of a complex between the antibodies present in the serum and the antigen of the vaccine composition, according to the customary techniques.




According to the invention, the said vaccine compositions will be preferably in combination with a pharmaceutically acceptable vehicle and, where appropriate, with one or more appropriate immunity adjuvants.




Various types of vaccines are currently available for protecting humans against infectious diseases: attenuated live microorganisms (


M. bovis


—BCG for tuberculosis), inactivated microorganisms (influenza virus), acellular extracts (


Bordetella pertussis


for whooping cough), recombinant proteins (hepatitis B virus surface antigen), polysaccharides (pneumococci). Experiments are underway on vaccines prepared from synthetic peptides or from genetically modified microorganisms expressing heterologous antigens. Even more recently, recombinant plasmid DNAs carrying genes encoding protective antigens were proposed as an alternative vaccine strategy. This type of vaccination is carried out with a particular plasmid derived from an


E. coli


plasmid which does not replicate in vivo and which encodes only the vaccinal protein. Animals were immunized by simply injecting the naked plasmid DNA into the muscle. This technique leads to the expression of the vaccine protein in situ and to a cell-type (CTL) and a humoral type (antibody) immune response. This double induction of the immune response is one of the main advantages of the technique of vaccination with naked DNA.




The vaccine compositions of the present invention can be evaluated in in vitro and in vivo animal models prior to host, e.g., human, administration. For example, in vitro neutralization assays such as those described by Peterson et al. (1988) can be utilized. The assay described by Peterson et al. (1988) is suitable for testing vaccine compositions directed toward either


Chlamydia pneumoniae


or


Chlamydia trachomatis.






Briefly, hyper-immune antisera is diluted in PBS containing 5% guinea pig serum, as a complement source. Chlamydiae (10


4


IFU; inclusion-forming units) are added to the antisera dilutions. The antigen-antibody mixtures are incubated at 37° C. for 45 minutes and inoculated into duplicate confluent Hep-2 or HeLa cell monolayers contained in glass vials (e.g., 15 by 45 mm), which have been washed twice with PBS prior to inoculation. The monolayer cells are infected by centrifugation at 1000×g for 1 hour followed by stationary incubation at 37E for 1 hour. Infected monolayers are incubated for 48 or 72 hours, fixed and stained with a Chlamydiae specific antibody, such as anti-MOMP for


C.trachomatis,


etc. IFUs are counted in ten fields at a magnification of 200×. Neutralization titer is assigned based on the dilution that gives 50% inhibition as compared to control monolayers/IFU.




The efficacy of vaccine compositions can be determined in vivo by challenging animal models of


Chlamydia pneumoniae


infection, e.g., mice or rabbits, with the vaccine compositions. For example, in vivo vaccine composition challenge studies can be performed in the murine model of


Chlamydia pneumonia


infection described by Moazed et al. (1997). Briefly, male homozygous apoE deficient and/or C57 BL/6J mice are immunized with vaccine compositions. Post-vaccination, the mice are mildly sedated by subcutaneous injection of a mixture of ketamine and xylazine, and inoculated intranasally with a total volume of 0.03-0.05 ml of organisms suspended in SPG medium or with SPG alone. The inoculations of


Chlamydia pneumoniae


are approximately 3×10


7


IFU/mouse. The mice are inoculated with


Chlamydia pneumoniae


at 8, 10, and 12 weeks of age. Tissues are then collected from the lung, spleen, heart, etc. at 1-20 weeks after the first inoculation. The presence of organisms is scored using PCR, histology and immunocytochemistry, or by quantitative culture/IFU after tissue homogenization.




Alternatively, in vivo vaccine composition challenge studies can be performed in the rabbit model of


Chlamydia pneumoniae


described by Laitinen et al. (1997). Briefly, New Zealand white rabbits (5 months old) are immunized with the vaccine compositions. Post-vaccination, the rabbits are sedated with Hypnorm, 0.3 ml/Kg of body weight, intramuscularly, and inoculated intranasally with a total of 0.5 ml of


Chlamydia pneumoniae


suspended in SPG medium or with SPG alone. The inoculations of


Chlamydia pneumoniae


are approximately 3×10


7


IFU/rabbit. The rabbits are reinfected in the same manner and with the same dose 3 weeks after the primary inoculation. Tissues are then collected 2 weeks after the primary infection and 1, 2, and 4 weeks after the reinfection. The presence of


Chlamydia pneumoniae


is scored using PCR, histology and immunocytochemistry, or by quantitative culture/IFU after tissue homogenization.




The vaccine compositions comprising nucleotide sequences or vectors into which the said sequences are inserted are in particular described in International Application No. WO 90/11092 and also in International Application No. WO 95/11307.




The nucleotide sequence constituting the vaccine composition according to the invention may be injected into the host after having been coupled to compounds which promote the penetration of this polynucleotide inside the cell or its transport up to the cell nucleus. The resulting conjugates may be encapsulated into polymeric microparticles, as described in International Application No. WO 94/27238 (Medisorb Technologies International).




According to another embodiment of the vaccine composition according to the invention, the nucleotide sequence, preferably a DNA, is complexed with the DEAE-dextran (Pagano et al., 1967) or with nuclear proteins (Kaneda et al., 1989), with lipids (Felgner et al., 1987) or encapsulated into liposomes (Fraley et al., 1980) or alternatively introduced in the form of a gel facilitating its transfection into the cells (Midoux et al., 1993, Pastore et al., 1994). The polynucleotide or the vector according to the invention may also be in suspension in a buffer solution or may be combined with liposomes.




Advantageously, such a vaccine will be prepared in accordance with the technique described by Tacson et al. or Huygen et al. in 1996 or alternatively in accordance with the technique described by Davis et al. in International Application No. WO 95/11307.




Such a vaccine may also be prepared in the form of a composition containing a vector according to the invention, placed under the control of regulatory elements allowing its expression in humans or animals. It is possible, for example, to use, as vector for the in vivo expression of the polypeptide antigen of interest, the plasmid pcDNA3 or the plasmid pcDNA1/neo, both marketed by Invitrogen® & D Systems, Abingdon, United Kingdom). It is also possible to use the plasmid V1Jns.tPA, described by Shiver et al. in 1995. Such a vaccine will advantageously comprise, in addition to the recombinant vector, a saline solution, for example a sodium chloride solution.




The immunogenic compositions of the invention can also be utilized as part of methods for immunization, wherein such methods comprise administering to a host, e.g., a human host, an immunizing amount of the immunogenic compositions of the invention. In a preferred embodiment, the method of immunizing is a method of immunizing against


Chlamydia pneumoniae.






A pharmaceutically acceptable vehicle is understood to designate a compound or a combination of compounds entering into a pharmaceutical or vaccine composition which does not cause side effects and which makes it possible, for example, to facilitate the administration of the active compound, to increase its life and/or its efficacy in the body, to increase its solubility in solution or alternatively to enhance its preservation. These pharmaceutically acceptable vehicles are well known and will be adapted by persons skilled in the art according to the nature and the mode of administration of the active compound chosen.




As regards the vaccine formulations, these may comprise appropriate immunity adjuvants which are known to persons skilled in the art, such as, for example, aluminum hydroxide, a representative of the family of muramyl peptides such as one of the peptide derivatives of N-acetyl-muramyl, a bacterial lysate, or alternatively incomplete Freund's adjuvant, Stimulon™ QS-21 (Aquila Biopharmaceuticals, Inc., Framingham, Mass.), MPL™ (3-O-deacylated monophosphoryl lipid A; RIBI ImmunoChem Research, Inc., Hamilton, Mont.), aluminum phosphate, IL-12 (Genetics Institute, Cambridge, Mass.).




Preferably, these compounds will be administered by the systemic route, in particular by the intravenous route, by the intranasal, intramuscular, intradermal or subcutaneous route, or by the oral route. More preferably, the vaccine composition comprising polypeptides according to the invention will be administered several times, spread out over time, by the intradermal or subcutaneous route.




Their optimum modes of administration, dosages and galenic forms may be determined according to criteria which are generally taken into account in establishing a treatment adapted to a patient, such as for example the patient's age or body weight, the seriousness of his general condition, tolerance of the treatment and the side effects observed.




The invention comprises the use of a composition according to the invention for the treatment or the prevention of cardiovascular diseases, preferably linked to the presence of atheroma, which are induced or worsened by


Chlamydia pneumoniae.






Finally, the invention comprises the use of a composition according to the invention for the treatment or the prevention of respiratory diseases which are induced or worsened by the presence of


Chlamydia pneumoniae,


preferably asthma.




Other characteristics and advantages of the invention appear in the following examples and figures:











LEGEND TO THE FIGURES




FIG.


1


: Line for the production of


Chlamydia pneumoniae


sequences




FIG.


2


: Analysis of the sequences and assembling




FIG.


3


: Finishing techniques





FIG. 3



a


): Assembly map





FIG. 3



b


): Determination and use of the orphan ends of the contigs











EXAMPLES




Experimental Procedures




Cells




The


Chlamydia pneumoniae


strain (CM1) used by the inventors is obtained from ATCC (American Culture Type Collection) where it has the reference number ATCC 1360-VR.




It is cultured on HeLa 229 cells, obtained from the American Type Culture Collection, under the reference ATCC CCL-2.1.




Culture of the Cells




The HeLa ATCC CCL-2.1 cells are cultured in 75-ml cell culture flasks (Corning). The culture medium is Dulbecco's modified cell culture medium (Gibco BRL No. 04101965) supplemented with MEM amino acids (Gibco BRL—No. 04301140) L (5 ml per 500 ml of medium) and 5% foetal calf serum (Gibco BRL No. 10270 batch 40G8260K) without antibiotics or antifungals.




The cell culture stock is maintained in the following manner. The cell cultures are examined under an inverted microscope. 24 hours after confluence, each cellular lawn is washed with PBS (Gibco BRL No. 04114190), rinsed and then placed for 5 min in an oven in the presence of 3 ml of trypsine (Gibco BRL No. 25200056). The cellular lawn is then detached and then resuspended in 120 ml of culture medium, the whole is stirred in order to make the cellular suspension homogeneous. 30 ml of this suspension are then distributed per cell culture flask. The flasks are kept in a CO


2


oven (5%) for 48 hours at a temperature of 37° C. The cell stock is maintained so as to have available daily 16 flasks of subconfluent cells. It is these subconfluent cells which will be used so as to be infected with Chlamydia. 25-ml cell culture flasks are also used, these flasks are prepared in a similar manner but the volumes used for maintaining the cells are the following: 1 ml of trypsine, 28 ml of culture medium to resuspend the cells, 7 ml of culture medium are used per 25-ml flask.




Infection of the Cells with Chlamydia




Initially, the Chlamydiae are obtained frozen from ATCC (−70° C.), in suspension in a volume of 1 ml. This preparation is slowly thawed, 500 ml are collected and brought into contact with subconfluent cells, which are obtained as indicated above, in a 25-ml cell culture flask, containing 1 ml of medium, so as to cover the cells. The flask is then centrifuged at 2000 rpm in a “swing” rotor for microtitre plates, the centrifuge being maintained at a temperature of 35° C. After centrifugation, the two flasks are placed in an oven at 35° C. for three hours. 6 ml of culture medium containing cycloheximide (1 mg/ml) are then added and the flask is stored at 35° C. After 72 hours, the level of infection is evaluated by direct immunofluorescence and by the cytopathogenic effect caused to the cells.




Direct Immunofluorescence




Starting with infected cells, which were obtained as indicated above, a cellular smear is deposited with a Pasteur pipette on a microscope slide. The cellular smear is fixed with acetone for 10 minutes; after draining the acetone, the smear is covered with 30 ml of murine monoclonal antibodies directed against MOMP (major outer membrane protein) of Chlamydia (Syva, Biomérieux) labelled with fluorescein isothiocyanate. The whole is then incubated in a humid chamber at a temperature of 37° C. The slides are then rinsed with water, slightly dried, and then after depositing a drop of mounting medium, a coverslip is mounted before reading. The reading is carried out with the aid of a fluorescence microscope equipped with the required filters (excitation at 490 nm, emission at 520 nm).




Harvesting of the


Chlamydia pneumoniae






After checking the infection by direct immunofluorescence, carried out as indicated above, the culture flasks are opened under a sterile cabinet, sterile glass beads with a diameter of the order of a millimeter are placed in the flask. The flask is closed and then vigorously stirred while being maintained horizontally, the cellular lawn at the bottom, so that the glass beads can have a mechanical action on the cellular lawn. Most of the cells are thus detached or broken; the effect of the stirring is observed under an optical microscope so as to ensure proper release of Chlamydiae.




Large-scale Infection of the Cell Cultures




The product of the Chlamydiae harvest (culture medium and cellular debris) is collected with a pipette, and distributed into three cell culture flasks containing subconfluent HeLa ATCC CCL-2.1 cells, obtained as indicated above. The cells thus inoculated are placed under gentle stirring (swing) in an oven at 35° C. After one hour, the flasks are kept horizontally in an oven so that the culture medium covers the cells for 3 hours. 30 ml of culture medium containing actydione (1 mg/ml) are then added to each of the flasks. The culture flasks are then stored at 35° C. for 72 hours. The cells thus infected are examined under an optical microscope after 24 hours, the cytopathogenic effect is evaluated by the appearance of cytoplasmic inclusions which are visible under an inverted optical microscope. After 72 hours, the vacuoles containing the Chlamydiae occupy the cytoplasm of the cell and push the cell nucleus sideways. At this stage, numerous cells are spontaneously destroyed and have left free elementary bodies in the culture medium. The Chlamydiae are harvested as described above and are either frozen at −80° C. or used for another propagation.




Purification of the Chlamydiae




The product of the Chlamydia harvests is stored at −80° C. and thawed on a water bath at room temperature. After thawing, each tube is vigorously stirred for one minute and immersed for one minute in an ultrasound tank (BRANSON 1200); the tubes are then stirred by inverting before being centrifuged for 5 min at 2000 rpm. The supernatant is carefully removed and kept at cold temperature (ice). The supernatant is vigorously stirred and then filtered on nylon filters having pores of 5 microns in diameter on a support (Nalgene) allowing a delicate vacuum to be established under the nylon filter. For each filtration, three nylon filters are superposed; these filters are replaced after every 40 ml of filtrate. Two hundred milliliters of filtration product are kept at cold temperature, and then after stirring by inverting, are centrifuged at 10,000 rpm for 90 min, the supernatant is removed and the pellet is taken up in 10 ml of 10 mM Tris, vigorously vortexed and then centrifuged at 10,000 rpm for 90 min. The supernatant is removed and the pellet is taken up in a buffer (20 mM Tris pH 8.0, 50 mM KCl, 5 mM MgCl


2


) to which 800 units of DNAse I (Boehringer) are added. The whole is kept at 37° C. for one hour. One ml of 0.5 M EDTA is then added, the whole is vortexed and frozen at −20° C.




Preparation of the DNA




The Chlamydiae purified above are thawed and subjected to a proteinase K (Boehringer) digestion in a final volume of 10 ml. The digestion conditions are the following: 0.1 mg/ml proteinase K, 0.1×SDS at 55° C., stirring every 10 min. The product of digestion is then subjected to a double extraction with phenol-chloroform, two volumes of ethanol are added and the DNA is directly recovered with a Pasteur pipette having one end in the form of a hook. The DNA is dried on the edge of the tube and then resuspended in 500 ml of 2 mM Tris pH 7.5. The DNA is stored at 4° C. for at least 24 hours before being used for the cloning.




Cloning of the DNA




After precipitation, the DNA is quantified by measuring the optical density at 260 nm. Thirty mg of Chlamydia DNA are distributed into 10 tubes of 1.5 ml and diluted in 300 ml of water. Each of the tubes is subjected to 10 applications of ultrasound lasting for 0.5 sec in a sonicator (unisonix XL2020). The contents of the 10 tubes are then grouped and concentrated by successive extractions with butanol (Sigma B1888) in the following manner: two volumes of butanol are added to the dilute DNA mixture. After stirring, the whole is centrifuged for five minutes at 2500 rpm and the butanol is removed. This operation is repeated until the volume of the aqueous phase is less than 1 ml. The DNA is then precipitated in the presence of ethanol and of 0.5 M sodium acetate pH 5.4, and then centrifuged for thirty minutes at 15,000 rpm at cold temperature (4° C.). The pellet is washed with 75% ethanol, centrifuged for five minutes at 15,000 rpm and dried at room temperature. A tenth of the preparation is analysed on a 0.8% agarose gel. Typically, the size of the DNA fragments thus prepared is between 200 and 8000 base pairs.




To allow the cloning of the DNA obtained, the ends are repaired. The DNA is distributed in an amount of 10 mg/tube, in the following reaction medium: 100 ml final volume, 1×buffer (Biolabs 201L), 0.5 ml BSA 0.05 mg/ml, 0.1 mM DATP, 0.1 mM each of dGTP, dCTP or dTTP, 60,000 IU T4 DNA polymerase. The reaction is incubated for thirty minutes at 16° C. The contents of each of the tubes are then grouped before carrying out an extraction with phenol-chloroform and then precipitating the aqueous phase as described above. After this step, the DNA thus prepared is phosphorylated. For that, the DNA is distributed into tubes in an amount of 10 mg per tube, and then in a final volume of 50 ml, the reaction is prepared in the following manner: 1 mM ATP, 1×kinase buffer, 10 IU T4 polynucleotide kinase (Biolabs 201L). The preparation is incubated for thirty minutes at 37° C. The contents of the tubes are combined and a phenol-chloroform extraction and then a precipitation are carried out in order to precipitate the DNA. The latter is then suspended in 1 ml of water and then the DNA fragments are separated according to their size on a 0.8% agarose gel (1×TAE). The DNA is subjected to an electric field of 5 V/cm and then visualized on a UV table. The fragments whose size varies between 1200 and 2000 base pairs are selected by cutting out the gel. The gel fragment thus isolated is placed in a tube and then the DNA is purified with the Qiaex kit (20021 Qiagen), according to the procedure provided by the manufacturer.




Preparation of the Vector




14 mg of the cloning vector pGEM-5Zf (Proméga P2241) are diluted in a final volume of 150 ml and are subjected to digestion with the restriction enzyme EcoRV 300 IU (Biolabs 195S) according to the protocol and with the reagents provided by the manufacturer. The whole is placed at 37° C. for 150 min and then distributed in the wells of a 0.8% agarose gel subjected to an electric field of 5 V/cm. The linearized vector is visualized on a UV table, isolated by cutting out the gel and then purified by the Qiaex kit (Qiagen 20021) according to the manufacturer's recommendations. The purification products are grouped in a tube, the volume is measured and then half the volume of phenol is added and the whole is vigorously stirred for 1 min. Half the volume of chloroform-isoamyl alcohol 24:1 is added and vigorously stirred for 1 min. The whole is centrifuged at 15,000 rpm for 5 min at 4° C., the aqueous phase is recovered and transferred into a tube. The DNA is precipitated in the presence of 0.3 M sodium acetate, pH 5.4 and 3 volumes of ethanol and placed at −20° C. for 1 hour. The DNA is then centrifuged at 15,000 rpm for 30 min at 4° C., the supernatant is removed while preserving the pellet, washed twice with 70% ethanol. After drying at room temperature, the DNA is suspended in 25 ml of water.




Phosphorylation of the Vector




25 ml of the vector prepared in the preceding step are diluted in a final volume of 500 ml of the following reaction mixture:




After repair, the DNA is subjected to a phenol-chloroform extraction and a precipitation, the pellet is then taken up in 10 ml of water, the DNA is quantified by measuring the optical density at 260 nm. The quantified DNA is ligated into the vector PGEm-5Zf(+) prepared by the restriction enzyme EcoRV and dephosphorylated (see preparation of the vector). The ligation is carried out under three conditions which vary in the ratio between the number of vector molecules and the number of insert molecules. Typically, an equimolar ratio, a ratio of 1:3 and a ratio of 3:1 are used for the ligations which are, moreover, carried out under the following conditions: vector PGEm-5Zf(+) 25 ng, cut DNA, ligation buffer in a final volume of 20 ml with T4 DNA ligase (Amersham E70042X); the whole is then placed in a refrigerator overnight and then a phenol-chloroform extraction and a precipitation are carried out in a conventional manner. The pellet is taken up in 5 ml of water.




Transformation of the Bacteria




Plating of the Bacteria




Petri dishes containing LB Agar medium containing ampicillin (50 mg/ml), Xgal (280 mg/ml) [5-bromo-4-chloro-indolyl-beta-D-galactopyranoside (Sigma B-4252)], IPTG (140 mg/ml) [isopropyl-beta-D-thiogalactoside (Sigma I-6758)] are used, 50 and 100 ml of bacteria are plated for each of the ligations. The Petri dishes are placed upside down at 37° C. for 15 to 16 hours in an oven. The number of “recombinant” positive clones is evaluated by counting the white colonies and the blue colonies which are thought to contain the vector alone.




Evaluation of the “recombinant” positive clones




Ninety-four white colonies and two blue colonies are collected with the aid of sterile cones and are deposited at the bottom of the wells of plates designed for carrying out the amplification techniques. 30 ml of the following reaction mixture are added to each well: 1.7 mM MgCl


2


, 0.2 mM each of dTP, dCTP, dGTP and dTTP, two synthetic oligonucleotides corresponding to sequences flanking the cloning site on either side and orienting the synthesis of the DNA in a convergent manner (0.5 mM RP and PU primers, 1 U TAQ polymerase (GibcoBRL 18038-026)).




The colonies thus prepared are subjected to a temperature of 94° C. for 5 min and then to 30 thermal cycles composed of the following steps: 94° C. for 40 s, 50° C. for 30 s, 72° C. for 180 s. The reaction is then kept for 7 min at 72° C. and then kept at 4° C.




The amplification products are deposited on an agarose gel (0.8%), stained with ethidium bromide, subjected to electrophoresis, and then analysed on an ultraviolet table. The presence of an amplification fragment having a size greater than 500 base pairs indicates the presence of an insert. The bacterial clones are then prepared so as to study the sequence of their insert.




Sequencing




To sequence the inserts of the clones obtained as above, these were amplified by PCR on bacteria cultures carried out overnight using the primers for the vectors flanking the inserts. The sequence of the ends of these inserts (on average 500 bases on each side) was determined by automated fluorescent sequencing on an ABI 377 sequencer, equipped with the ABI Prism DNA Sequencing Analysis software (version 2.1.2).




Analysis of the Sequences




The sequences obtained by sequencing in a high-yield line (

FIG. 1

) are stored in a database; this part of the production is independent of any treatment of the sequences. The sequences are extracted from the database, avoiding all the regions of inadequate quality, that is to say the regions for which uncertainties are observed on the sequence at more than 95%. After extraction, the sequences are introduced into a processing line, the diagram of which is described in FIG.


2


. In a first path of this processing line, the sequences are assembled by the Gap4 software from R. Staden (Bonfield et al., 1995) (OS UNIX/SUN Solaris); the results obtained by this software are kept in the form of two files which will be used for a subsequent processing. The first of these files provides information on the sequence of each of the contigs obtained. The second file represents all the clones participating in the composition of all the contigs as well as their positions on the respective contigs.




The second processing path uses a sequence assembler (TIGR-Asmg assembler UNIX/SUN Solaris); the results of this second processing path are kept in the form of a file in the TIGR-Asmg format which provides information on the relationship existing between the sequences selected for the assembly. This assembler is sometimes incapable of linking contigs whose ends overlap over several hundreds of base pairs.




The results obtained from these two assemblers are compared with the aid of the BLAST program, each of the contigs derived from one assembly path being compared with the contigs derived from the other path.




For the two processing paths, the strict assembly parameters are fixed (95% homology, 30 superposition nucleotides). These parameters avoid 3 to 5% of the clones derived from eukaryotic cells being confused with sequences obtained from the clones derived from


Chlamydia pneumoniae.


The eukaryotic sequences are however preserved during the course of this project; the strategy introduced, which is described below, will be designed, inter alia, not to be impeded by these sequences derived from contaminating clones.




The results of these two assemblers are processed in a software developed for this project. This software operates on a Windows NT platform and receives, as data, the results derived from the STADEN software and/or the results derived from the TIGR-Asmg assembler, the software, results, after processing of the data, in the determination of an assembly map which gives the proximity relationship and the orientation of the contigs in relation to one another (

FIG. 3



a


). Using this assembly map, the software determines all the primers necessary for finishing the project. This treatment, which will be detailed below, has the advantage of distinguishing the isolated sequences derived from the contaminations, by the DNA eukaryotic cells, of the small-sized sequences clearly integrated into the project by the relationships which they establish with contigs. In order to allow, without any risk of error, the arrangement and the orientation of the contigs in relation to one another, a statistical evaluation of the accuracy of the names (naming) “naming” of sequence is made from the results of “contigation”. This evaluation makes it possible to give each of the clone plates, as well as each of the subsets of plates, a weight which is inversely proportional to probable error rate existing in the “naming” of the sequences obtained from this plate or from a subset of this plate. In spite of a low error rate, errors may occur throughout the steps of production of the clones and of the sequences. These steps are numerous, repetitive and although most of them are automated, others, like the deposition in the sequencers, are manual; it is then possible for the operator to make mistakes such as the inversion of two sequences. This type of error has a repercussion on the subsequent processing of the data, by resulting in relationships (between the contigs) which do not exist in reality, then in attempts at directed sequencing between the contigs which will end in failure. It is because of this that the evaluation of the naming errors is of particular importance since it allows the establishment of a probabilistic assembly map from which it becomes possible to determine all the clones which will serve as template to obtain sequences separating two adjacent contigs. Table 2 of parent U.S. application serial No. 60/107078 filed Nov. 4, 1998 and French application 97-14673 filed Nov. 21, 1997, each of which is incorporated by reference herein in its entirety, gives the clones and the sequences of the primers initially used during the initial operations.




To avoid the step which consists in ordering and then preparing the clones by conventional microbiological means, outer and inner primers oriented towards the regions not yet sequenced are defined by the software. The primers thus determined make it possible to prepare, by PCR, a template covering the nonsequenced region. It is the so-called outer primers (the ones most distant from the region to be sequenced) which are used to prepare this template. The template is then purified and a sequence is obtained on each of the two strands during 2 sequencing reactions which each use one of the 2 inner primers. In order to facilitate the use of this approach, the two outer primers and the two inner primers are prepared and then stored on the same position of 4 different 96-well plates. The two plates containing the outer primers are used to perform the PCRs which will serve to prepare the templates. These templates will be purified on purification columns preserving the topography of the plates. Each of the sequences will be obtained using primers situated on one and then on the other of the plates containing the inner primers. This distribution allows a very extensive automation of the process and results in a method which is simple to use for finishing the regions not yet sequenced. Table 3 of parent U.S. application serial No. 60/107078 filed Nov. 4, 1998 and French application 97-14673 filed Nov. 21, 1997, each of which is incorporated by reference herein in its entirety, gives the names and the sequences of the primers used for finishing


Chlamydia pneumoniae.






Finally, a number of contigs exist in a configuration where one of their ends is not linked to any other contig end (

FIG. 3



b


) by a connecting clone relationship (a connecting clone is defined as a clone having one sequence end on a contig and the other end of its sequence on another contig; furthermore, this clone must be derived from a plate or a subset of plates with adequate naming quality). For the


Chlamydia pneumoniae


project, this particular case occurred 24 times. Two adjacent PCR primers orienting the synthesis of the DNA towards the end of the consensus sequence are defined for each of the orphan ends of the consensus sequence. The primer which is closest to the end of the sequence is called the inner primer whereas the primer which is more distant from the end of the sequence is called the outer primer. The outer primers are used to explore the mutual relationship between the orphan ends of the different contigs. The presence of a single PCR product and the possibility of amplifying this product unambiguously using the inner primers evokes the probable relationship between the contigs on which the primers which allowed the amplification are situated. This relationship will be confirmed by sequencing and will allow the connection between the orphan ends of the consensus sequences. This strategy has made it possible to obtain a complete map of the


Chlamydia pneumoniae


chromosome and then to finish the project.




Quality control




All the bases not determined with certainty in the chromosomal sequence were noted and the density of uncertainties was measured on the entire chromosome. The regions with a high density of uncertainties were noted and the PCR primers spanning these regions were drawn and are represented in Table 4 of parent U.S. application serial No. 60/107078 filed Nov. 4, 1998 and French application 97-14673 filed Nov. 21, 1997 each of which is incorporated by reference herein in its entirety.




The sequence of each of the PCR products was obtained with two operational primers different from the amplification primers. The sequences were obtained in both directions for all the PCRs (100% success).




Data banks




Local reorganizations of major public banks were used. The protein bank used consists of the nonredundant fusion of the Genpept bank (automated translation of GenBank, NCBI; Benson et al., 1996).




The entire BLAST software (public domain, Altschul et al., 1990) for searching for homologies between a sequence and protein or nucleic data banks was used. The significance levels used depend on the length and the complexity of the region tested as well as the size of the reference bank. They were adjusted and adapted to each analysis.




The results of the search for homologies between a sequence according to the invention and protein or nucleic data banks are presented and summarized in Table 1 below.




Table 1: List of Coding Chromosome Regions and Homologies Between These Regions and the Sequence Banks




Legend to Table 1: Open reading frames are identified with the GenMark software version 2.3A (GenePro), the template used is


Chlamydia pneumoniae


of order 4 on a length of 196 nucleotides with a window of 12 nucleotides and a minimum signal of 0.5. The reading frames ORF2 to ORF 1137 are numbered in order of appearance on the chromosome, starting with ORF2 (ORF column). The positions of the beginning and of the end are then given in column 2 (position). When the position of the beginning is greater than the position of the end, this means that the region is encoded by the strand complementary to the sequence which was given in the sequence SEQ ID No. 1.




All the putative products were subjected to a search for homology on GENPEPT (release 102 for SEQ ID No. 2 to SEQ ID No. 1137, and release 108 for SEQ ID No. 1138 to SEQ ID No. 1291 and SEQ ID No. 6844 to SEQ ID No. 6849) with the BLASTP software (Altschul et al. 1990). With, as parameters, the default parameters with the exception of the expected value E set at 10


−5


(for SEQ ID No. 2 to SEQ ID No. 1137) and P value set at e


−10


(for SEQ ID No. 1138 to SEQ ID No. 1291 and SEQ ID No. 6844 to SEQ ID No. 6849). Subsequently, only the identities greater than 30% (I% column) were taken into account. The description of the most homologous sequence is given in the Homology column; the identifier for the latter sequence is given in the ID column and the animal species to which this sequence belongs is given in the Species column. The Homology score is evaluated by the sum of the blast scores for each region of homology and reported in the Score column.




Materials and Methods for transmembrane domains:




The DAS software was used as recommended by the authors (Cserzo et al., 1997).




This method uses, to predict the transmembrane domains, templates derived from a sampling of selected proteins. All the regions for which a “Cutoff” greater than 1.5 was found by the program were taken into account.




Additional ORF Finder Programs




For this analysis, two additional ORF finder programs were used to predict potential open reading frames of a minimum length of 74 amino acids; Glimmer (Salzberg, S. L., Delcher, A., Kasif, S., and W. White. 1998. Microbial gene identification using interpolated Markov models. Nucleic Acids Res. 26:544-548.), and an in-house written program. The in-house program used a very simple search algorithm. The analysis required the that the genomic DNA sequence text be in the 5′ to 3′ direction, the genome is circular, and that TAA, TAG, and TGA are stop codons. The search parameters were as follows:




(1) A search for an ORF that started with a GTG codon was performed. If no GTG codons were found, then a search for an ATG codon was performed. However, if a GTG codon was found, then a search downstream for a ATG codon was performed. All start and stop nucleotide positions were recorded.




(2) A search for an ORF that started with a TTG codon was performed. If no TTG codons were found, then a search for a ATG codon was performed. However, if a TTG codon was found, then a search downstream for a ATG codon was performed. All start and stop nucleotide positions were recorded.




(3) The analysis described in steps 1 and 2 were repeated for the opposite strand of DNA sequence.




(4) A search for ORFs that determined all ORF lengths using start and stop positions in the same reading frames was performed.




(5) All ORFs whose DNA length was less than 225 nucleotides were eliminated from the search.




Surface Exposed Protein Search Criteria




Potential cell surface vaccine targets are outer membrane proteins such as porins, lipoproteins, adhesions and other non-integral proteins. In


Chlamydia psittaci,


the major immunogens is a group of putative outer membrane proteins (POMPs) and no homologs have been found in


Chlamydia pneumoniae


and


Chlamydia trachomatis


by traditional analysis (Longbottom, D., Russell, M., Dunbar, S. M., Jones, G. E., and A. J. Herring. 1998. Molecular Cloning and Characterization of the Genes Coding for the Highly Immunogenic Cluster of 90-Kilodalton Envelope Proteins from


Chlamydia psittaci


Subtype That Causes Abortion in Sheep. Infect Immun 66:1317-1324.) Several putative outer membrane proteins have been identified in


Chlamydia pneumoniae,


all of which may represent vaccine candidates. The major outer membrane protein (MOMP) gene (omp1) has been found in various isolates of


Chlamydia pneumoniae


(Jantos, Calif., Heck, S., Roggendorf, R., Sen-Gupta, M., and Hegemann, J H. 1997. Antigenic and molecular analyses of different chlamydia pneumoniae strains. J. Clin Microbiology 35(3):620-623.) Various criteria, as listed below, were used to identify putative surface exposed ORFs from the genomic DNA sequence of


Chlamydia pneumoniae


(French application 97-14673 filed Nov. 21, 1997). Any ORF which met any one or more of the individual criteria were listed in this category.




Protein homology searches were done using the Blastp 2.0 tool (Altschul, S. F., Madden, T. L., Schaffer, A. A., Zhang, J., Zhang, Z., Miller, W., and D. J. Lipman. 1997. Gapped BLAST and PSI-BLAST: a new generation of protein database search programs. Nucleic Acids Res. 25:3389-3402.)




An ORF product was labeled surface exposed if there was homology to a known, or hypothetical, or putative surface exposed protein with a P score better than e


−10


.




Most, if not all, proteins that are localized to the membrane of bacteria, via a secretory pathway, contain a signal peptide. A software program, SignalP, analyzes the amino acid sequence of an ORF for such a signal peptide (Nielsen, H., Engelbrecht. J., Brunak, S., and G. von Heijne. 1997. Identification of prokaryotic and eukaryotic signal peptides and prediction of their cleavage sites. Protein Engineering 10:1-6.) The first 60 N-terminal amino acids of each ORF were analyzed by SignalP using the Gram-Negative software database. The output generates four separate values, maximum C, maximum Y, maximum S, and mean S. The S-score, or signal region, is the probability of the position belonging to the signal peptide. The C-score, or cleavage site, is the probability of the position being the first in the mature protein. The Y-score is the geometric average of the C-score and a smoothed derivative of the S-score. A conclusion of either a Yes or No is given next to each score. If all four conclusions are Yes and the C-terminal amino acid is either a phenylalanine (F) or a tyrosine (Y), the ORF product was labelled outer membrane (Struyve, M., Moons, M., and J. Tommassen. 1991. Carboxy-terminal Phenylalanine is Essential for the Correct Assembly of a Bacterial Outer Membrane Protein. J. Mol. Biol. 218:141-148.)




The program called Psort, determines the localization of a protein based on its signal sequence, recognition of transmembrane segments, and analysis of its amino acid composition (Nakai, K., and M. Kanehisa. 1991. Expert system for predicting protein localization sites in gram-negative bacteria. Proteins 11:95-110.) An ORF product is considered to be an outer membrane protein if the output data predicts the protein as outer membrane with a certainty value of 0.5 or better and whose value is at least twice as large as the next predicted localized certainty value.




Finally, ORF products that were not predicted to be outer membrane or surface exposed, based on the above criteria, were further analyzed. The blastp output data for these ORFs were searched using various general and specific keywords, suggestive of known cell surface exposed proteins. An ORF was labeled surface exposed if the keywords matched had a Blastp hit, had a P score better than e


−10


, and that there was no better data indicating otherwise. The following is a list of the searched keywords:






















Invasion







Adhesion




Adhesin




Invasion




Outer







Omp




Outer Surface




Porin




Membrane




Extensin






Cell Surface




Cell Wall




Pilus




Pilin




Flagellar sheath




























BtuB











Cir




ChuA




CopB




ExeD




FadL




FecA






FepA




FhuA




FmdC




FomA




FrpB




GspD






HemR




HgbA




Hgp




HmbR




HmuR




HMW






HrcC




Hrp




InvG




LamB




LbpA




LcrQ






Lmpl




MxiD




MOMP




PilE




HpaA




NolW






NspA




OpcP




OpnP




Opr




OspA




PhoE






PldA




Por




PscC




Pu1D




PupA




QuiX






RafY




ScrY




SepC




ShuA




SomA




SpiA






Tbpl




Yop




YscC




mip




Tol














Those ORFs that did not meet the minimum requirement for being an outer membrane protein based on the above search criteria but which were homologous to identified outer membrane ORFs in


Chlamydia trachomatis


were included. The


Chlamydia trachomatis


genome (French patent applications FR97-15041, filed Nov. 28, 1997 and FR97-16034 filed Dec. 17, 1997) was analyzed using the above search criteria and a number of outer membrane ORFs were identified. These


Chlamydia trachomatis


ORFs were then tested against the


Chlamydia pneumoniae


genome using Blastp. Any


Chlamydia pneumoniae


ORF with a Blastp P value better than e


−10


against a


Chlamydia trachomatis


outer membrane was included in this section, if there was no better data indicating otherwise. A list of ORFs in the


Chlamydia pneumoniae


genome encoding putative surface exposed proteins is set forth above in the specification.




Identification of Putative Lipoproteins in the Genome of


Chlamydia pneumoniae






Lipoproteins are the most abundant post-translationally modified bacterial secretory proteins (Pugsley, A. P. 1993. The complete general secretory pathway in Gram-negative bacteria. Microbiol. Rev. 57:50-108). The characteristic features of lipoproteins are a thiol-linked diacylglyceride and an amine-linked monoacyl group on the cysteine that becomes the amino-terminal residue after signal peptide cleavage by Signal Peptidase II. (Pugsley, A. P. 1993. The complete general secretory pathway in Gram-negative bacteria. Microbiol. Rev. 57:50-108). The identification of putative lipoproteins from the genomic sequencing of


Chlamydia pneumoniae


was done by examining the deduced amino acid sequence of identified ORFs for the presence of a signal peptide with a Signal Peptidase II cleavage site analogous to the consensus sequence for prolipoprotein modification and processing reactions (Hayashi, S., and H. C. Wu. 1992. Identification and characterization of lipid-modified proteins in bacteria, p. 261-285. In N. M. Hooper and A. J. Turner (ed.) Lipid modification of proteins: A practical approach. Oxford University Press, New York; Sutcliffe, I. C. and R. R. B. Russell. 1995. Lipoproteins of Gram-positive bacteria. J. Bacteriol. 177:1123-1128.).






Chlamydia pneumoniae


ORFs were initially screened for the most basic of lipoprotein characteristics, a cysteine in the first 30 amino acids of the deduced protein. ORFs with a standard start codon (ATG, GTG, or TTG) and having one or more of the following characteristics were selected for direct analysis of their first 30 amino acids:




(a) Significant Signal P value (at least two out of the four values are Yes)




(b) PSORT value indicating membrane passage (IM-inner membrane, Peri-periplasm, or OM-outer membrane)




(c) Identification of the word lipoprotein among the ORF blastp data set.




(d) A Blastp value of <e


−10


with a putative lipoprotein from


Chlamydia trachomatis


(French applications 97-15041 filed Nov. 28, 1997 and FR-97-16034 filed Dec. 17, 1997).




The first 30 amino acids of each ORF in this set were analyzed for the characteristics commonly found in lipoprotein signal peptides (Pugsley, A. P. 1993. The complete general secretory pathway in Gram-negative bacteria. Microbiol. Rev. 57:50-108; Hayashi, S., and H. C. Wu. 1992. Identification and characterization of lipid-modified proteins in bacteria, p. 261-285. In N. M. Hooper and A. J. Turner (ed.) Lipid modification of proteins: A practical approach. Oxford University Press, New York; Sutcliffe, I. C. and R. R. B. Russell. 1995. Lipoproteins of Gram-positive bacteria. J. Bacteriol. 177:1123-1128.) Putative lipoprotein signal peptides were required to have a cysteine between amino acid 10 and 30 and reach a minimum score of three based on the following criteria for lipoprotein signal peptides:




(a) Identification of specific amino acids in specific positions around the cysteine which are part of the consensus Signal Peptidase II cleavage site (Hayashi, S., and H. C. Wu. 1992. Identification and characterization of lipid-modified proteins in bacteria, p. 261-285. In N. M. Hooper and A. J. Turner (ed.) Lipid modification of proteins: A practical approach. Oxford University Press, New York); Sutcliffe, I. C. and R. R. B. Russell. 1995. Lipoproteins of Gram-positive bacteria. J. Bacteriol. 177:1123-1128). Since the identification of the cleavage site is the most important factor in identifying putative lipoproteins, each correctly positioned amino acid contributed toward reaching the minimum score of three.




(b) A hydrophobic region rich in alanine and leucine prior to the cleavage site (Pugsley, A. P. 1993. The complete general secretory pathway in Gram-negative bacteria. Microbiol. Rev. 57:50-108) contributed toward reaching the minimum score of three.




(c) A short stretch of hydrophilic amino acids greater than or equal to 1 usually lysine or arginine following the N-terminal methionine (Pugsley, A. P. 1993. The complete general secretory pathway in Gram-negative bacteria. Microbiol. Rev. 57:50-108) contributed toward reaching the minimum score of three.




A list of ORFs in the


Chlamydia pneumoniae


genome encoding putative lipoproteins is set forth above in the specification.




LPS-Related ORFs of


Chlamydia pneumoniae






Lipopolysaccharide (LPS) is an important major surface antigen of Chlamydia cells. Monoclonal antibodies (Mab) directed against LPS of


Chlamydia pneumoniae


have been identified that can neutralize the infectivity of


Chlamydia pneumoniae


both in vitro and in vivo (Peterson, E. M., de la Maza, L. M., Brade, L., Brade, H. 1998. Characterization of a Neutralizing Monoclonal Antibody Directed at the Lipopolysaccharide of


Chlamydia pneumonia.


Infect. Immun. August 66(8):3848-3855.) Chlamydial LPS is composed of lipid A and a core oligosaccharide portion and is phenotypically of the rough type (R-LPS) (Lukacova, M., Baumann, M., Brade, L., Mamat, U., Brade, H. 1994. Lipopolysaccharide Smooth-Rough Phase Variation in Bacteria of the Genus Chlamydia. Infect. Immun. June 62(6):2270-2276.) The lipid A component is composed of fatty acids which serve to anchor LPS in the outer membrane. The core component contains sugars and sugar derivatives such as a trisaccharide of 3-deoxy-D-manno-octulosonic acid (KDO) (Reeves, P. R., Hobbs, M., Valvano, M. A., Skurnik, M., Whitfield, C., Coplin, D., Kido, N., Klena, J., Maskell, D., Raetz, C. R. H., Rick, P. D. 1996.


Bacterial Polysaccharide Synthesis and Gene Nomenclature


pp. 10071-10078, Elsevier Science Ltd.). The KDO gene product is a multifunctional glycosyltransferase and represents a shared epitope among the Chlamydia. For a review of LPS biosynthesis see, e.g., Schnaitman, C. A., Klena, J. D. 1993. Genetics of Lipopolysaccharide Biosynthesis in Enteric Bacteria. Microbiol. Rev. 57:655-682.




A text search of the ORF blastp results identified several genes that are involved in Chlamydial LPS production with a P score better than e


−10


. The following key-terms were used in the text search: KDO, CPS (Capsular Polysaccharide Biosynthesis), capsule, LPS, rfa, rfb, rfc, rfe, rha, rhl, core, epimerase, isomerase, transferase, pyrophosphorylase, phosphatase, aldolase, heptose, manno, glucose, lpxB, fibronectin, fibrinogen, fucosyltransferase , lic, lgt, pgm, tolC, rol, ChoP, phosphorylcholine, waaF, PGL-Tb1. A list of ORFs in the


Chlamydia pneumoniae


genome encoding putative polypeptides involved in LPS biosynthesis is set forth above in the specification.




Type III And Other Secreted Products




Type III secretion enables gram-negative bacteria to secrete and inject pathogenicity proteins into the cytosol of eukaryotic host cells (Hueck, C. J., 1998. Type III Protein Secretion Systems in Bacterial Pathogens of Animals and Plants. In Microbiology and Molecular Biology Reviews. 62:379-433.) These secreted factors often resemble eukaryotic signal transduction factors, thus enabling the bacterium to redirect host cell functions (Lee, C. A., 1997. Type III secretion systems: machines to deliver bacterial proteins into eukaryotic cells? Trends Microbiol. 5:148-156.) In an attempt to corrupt normal cellular functions, Chlamydial pathogenicity factors injected into the host cytosol will nonetheless, as cytoplasmic constituents be processed and presented in the context of the Major Histocompatibility Complex (MHC class I). As such, these pathogenicity proteins represent MHC class I antigens and will play an important role in cellular immunity. Also included in this set are secreted non-type III products that may play a role as vaccine components.




A text search of the ORF blastp results identified genes that are involved in


Chlamydia pneumoniae


protein secretion with a P score better than e


−10


. The following key-terms were used in the text search in an effort to identify surface localized or secreted products: Yop, Lcr, Ypk, Exo, Pcr, Pop, Ipa, Vir, Ssp, Spt, Esp, Tir, Hrp, Mxi, hemolysin, toxin, IgA protease, cytolysin, tox, hap, secreted and Mip.






Chlamydia pneumoniae


ORFs that did not meet the above keyword search criteria, but have homologs in


Chlamydia trachomatis


that do meet the search criteria are included herein. The


Chlamydia trachomatis


genome (French patent applications FR97-15041, filed Nov. 28, 1997 and 97-16034 filed Dec. 17, 1997) was analyzed using the above search criteria and a number of ORFs were identified. These


Chlamydia trachomatis


ORFs were tested against the


Chlamydia pneumoniae


genome using Blastp. Any


Chlamydia pneumoniae


ORF with a Blastp P value <e


−10


against a


Chlamydia trachomatis


homolog, identified using the above search criteria, was included. A list of ORFs in the


Chlamydia pneumoniae


genome encoding putative secreted proteins is in the specification.






Chlamydia pneumoniae:


RGD Recognition Sequence




Proteins that contain Arg-Gly-Asp (RGD) attachment site, together with integrins that serve as their receptor constitute a major recognition system for cell adhesion. The RGD sequence is the cell attachment site of a large number of adhesive extracellular matrix, blood, and cell surface proteins and nearly half of the known integrins recognize this sequence in their adhesion protein ligands. There are many RGD containing microbial proteins such as the penton protein of adenovirus, the coxsackie virus, the foot and mouth virus and pertactin, a 69 kDa (kilodalton) surface protein of


Bordetella pertussis,


that serve as ligands through which these microbes bind to integrins on the cell surfaces and gain entry into the cell. The following provides evidence supporting the importance of RGD in microbial adhesion:




a) The adenovirus penton base protein has a cell rounding activity and when penton base was expressed in


E. coli,


it caused cell rounding and cells adhered to polystyrene wells coated with the protein. Mutant analysis showed that both these properties required an RGD sequence. Virus mutants with amino acid substitutions in the RGD sequence, showed much less adherence to HeLa S3 cells, and also were delayed in virus reproduction (Bai, M., Harfe, B., and Freimuth, P. 1993. Mutations That Alter an RGD Sequence in the Adenovirus Type 2 Penton Base Protein Abolish Its Cell-Rounding Activity and Delay Virus Reproduction in Flat Cells. J. Virol. 67:5198-5205).




b) It has been shown that attachment and entry of coxsackie virus A9 to GMK cells were dependent on an RGD motif in the capsid protein VP1. VP1 has also been shown to bind a


v


b


3


integrin, which is a vitronectin receptor (Roivainen, M., Piirainen, L., Hovi, T., Virtanen, I., Riikonen, T., Heino, J., and Hyypia, T. 1994. Entry of Coxsackievirus A9 into Host Cells: Specific Interactions with a


v


b


3


Integrin, the Vitronectin Receptor Virology, 203:357-65).




c) During the course of whooping cough,


Bordetella pertussis


interacts with alveolar macrophages and other leukocytes on the respiratory epithelium. Whole bacteria adheres by means of two proteins, filamentous hemagglutinin (FHA) and pertussis toxin. FHA interacts with two classes of molecules on macrophages, galactose containing glycoconjugates and the integrin CR3. The interaction between CR3 and FHA involves recognition of RGD sequence at the positions 1097-1099 in FHA (Relman, D., Tuomanen, E., Falkow, S., Golenbock, D. T., Saukkonen, K., and Wright, S. D. “Recognitition of a Bacterial Adhesin by an Integrin: Macrophage CR3 Binds Filamentous Hemagglutinin of Bordetella Pertussis.” Cell, 61:1375-1382 (1990)).




d) Pertactin, a 69 kDa outer membrane protein of


Bordetella pertussis,


has been shown to promote attachment of Chinese hamster ovary cells (CHO). This attachment is mediated by recognition of RGD sequence in pertactin by integrins on CHO cells and can be inhibited by synthetic RGD containing peptide homologous to the one present in pertactin (Leininger, E., Roberts, M., Kenimer, J. G., Charles, I. G., Fairweather, N., Novotny, P., and Brennan, M. J. 1991. Pertactin, an Arg-Gly-Asp containing


Bordetella pertussis


surface protein that promotes adherence of mammalian cells Proc. Natl. Acad. Sci. USA, 88:345-349).




e) The RGD sequence is highly conserved in the VP1 protein of foot and mouth disease virus (FMDV). Attachment of FMDV to baby hamster kidney cells (BHK) has been shown to be mediated by VP1 protein via the RGD sequence. Antibodies against the RGD sequence of VP1 blocked attachment of virus to BHK cells (Fox, G., Parry, N. R., Barnett, P. V., McGinn, B., Rowland, D. J., and Brown, F. 1989. The Cell Attachment Site on Foot-and-Mouth Disease Virus Includes the Amino Acid Sequence RGD (Arginine-Glycine-Aspartic Acid) J. Gen. Virol., 70:625-637).




It has been demonstrated that bacterial adherence can be based on interaction of a bacterial adhesin RGD sequence with an integrin and that bacterial adhesins can have multiple binding site characteristic of eukaryotic extracellular matrix proteins. RGD recognition is one of the important mechanisms used by microbes to gain entry into eukaryotic cells.




The complete deduced protein sequence of the


Chlamydia pneumoniae


genome was searched for the presence of RGD sequence. There were a total of 54 ORFs that had one or more RGD sequences. Not all RGD containing proteins mediate cell attachment. It has been shown that RGD containing peptides that have proline immediately following the RGD sequence are inactive in cell attachment assays (Pierschbacher & Ruoslahti. 1987. Influence of stereochemistry of the sequence Arg-Gly-Asp-Xaa on binding specificity in cell adhesion. J. Biol. Chem. 262:17294-98). ORFs that had RGD, with proline as the amino acid following the RGD sequence were excluded from the list. Also, RGD sequence may not be available at the surface of the protein or may be present in a context that is not compatible with integrin binding. Since not all RGD-containing proteins are involved in cell attachment, several other criteria were used to refine the list of RGD-containing proteins. A list of ORFs in the


Chlamydia pneumoniae


genome encoding polypeptides with RGD recognition sequence(s) is in the specification.




Non-


Chlamydia trachomatis


ORFs






Chlamydia pneumoniae


ORFs were compared to the ORFs in the


Chlamydia trachomatis


genome (French patent applications FR97-15041, filed Nov. 28, 1997 and 97-16034 filed Dec. 17, 1997) using Blastp. Any


Chlamydia pneumoniae


ORF with a Blastp P value worse than e


−10


(i.e. >e


−10


) against


Chlamydia trachomatis


ORFs are included in this section. A list of ORFs in the


Chlamydia pneumoniae


genome which are not found in


Chlamydia trachomatis


is set forth above in the specification.




Cell Wall Anchor Surface ORFs




Many surface proteins are anchored to the cell wall of Gram-positive bacteria via the conserved LPXTG motif (Schneewind, O., Fowler, A., and Faull, K. F. 1995. Structure of the Cell Wall Anchor of Surface Proteins in


Staphylococcus aureus.


Science 268:103-106). A search of the


Chlamydia pneumoniae


ORFs was done using the motif LPXTG. A list of ORFs in the


Chlamydia pneumoniae


genome encoding polypeptides anchored to the cell wall is in the specification.




ATCC Deposits




Samples of


Chlamydia pneumoniae


were deposited with the American Type Culture Collection (ATCC), Rockville, Md., on Nov. 19, 1998, and assigned the accession number VR-2634. Cells can be grown, harvested and purified, and DNA can be prepared as discussed above. In order to enable recovery of specific fragments of the chromosome, one can run targeted PCR reactions, whose amplification products can then be sequenced and/or cloned into any suitable vector, according to standard procedures known to those skilled in the art.




In addition, a sample of three pools of clones covering chromosomal regions of interest were deposited with the American Type Culture Collection (ATCC), Rockville, Md., on Nov. 19, 1998, and assigned the indicated accession numbers: 207000, 207001, and 207002. Each pool of clones contains a series of clones. When taken together, the three pools in the sample cover a portion of the chromosome, with a redundancy of slightly more than two. The total number of clones in the sample is 196.




The clones cover the following three regions of interest:




(i) position 30,000 to 40,000 of SEQ ID No. 1, referred to as region A;




(ii) position 501,500 to 557,000 of SEQ ID No. 1, referred to as region B; and




(iii) position 815,000 to 830,000 of SEQ ID No. 1, referred to as region C.




Table 4 lists groups of oligonucleotides to be used to amplify each of ORFs 2-1291 according to standard procedures known to those skilled in the art. Such oligonucleotides are listed as SEQ ID Nos. 1292 to 6451. For each ORF, the following is listed: one forward primer positioned 2,000 bp upstream of the beginning of the ORF; one forward primer positioned 200 bp upstream of the beginning of the ORF; one reverse primer positioned 2,000 bp downstream at the end of ORF, which is 2,000 bp upstream of the end site of the ORF on the complementary strand; and one reverse primer 200 bp downstream at the end of ORF, which is 200 bp upstream of the end site of the ORF on the complementary strand. The corresponding SEQ ID Nos. for the primers are listed in Table 4, where Fp is the proximal forward primer; Fd is the distal forward primer; Bp is the proximal reverse primer; and Bd is the distal reverse primer. The positions of the 5′ ends of each of these primers on the nucleotide sequence of SEQ ID No. 1 are shown in Table 5 (F refers to forward primers; R refers to reverse primers).




Table 6 lists oligonucleotides (SEQ ID Nos. 6452-6843) to be used to amplify the inserts of each of the 196 clones present in the pooled sample according to standard procedures well known to those of skill in the art. These primers can also be utilized to amplify the chromosomal region corresponding to the region A, B or C within which the particular insert lies. Their positions are indicated in Table 7 (F refers to forward primers; R refers to reverse primary).




The present invention is not to be limited in scope by the specific embodiments described herein, which are intended as single illustrations of individual aspects of the invention, and functionally equivalent methods and components are within the scope of the invention. Indeed, various modifications of the invention, in addition to those shown and described herein will become apparent to those skilled in the art from the foregoing description and accompanying drawings. Such modifications are intended to fall within the scope of the appended claims.




All publications and patent applications mentioned in this specification are herein incorporated by reference to the same extent as if each individual publication or patent application was specifically and individually indicated to be incorporated by reference.



















TABLE 1









ORF




Begin




End




Homology




ID




Species




Score




I %






























ORF2




42




794




triosephosphate isomerase




L27492






Thermotoga maritima






567




54






ORF3




1258




1614




putative






ORF4




1807




2418




polypeptide deformylase




D90906




Synechocystis sp.




316




40






ORF5




3393




2491




hypothetical protein




Z75208






Bacillus subtilis






338




42






ORF6




3639




4067




unknown




U87792






Bacillus subtilis






117




38






ORF7




5649




4270




putative






ORF8




7463




6012




putative






ORF9




8051




8962




putative






ORF10




9129




9959




putative






ORF11




10687




10361




putative






ORF12




10927




11232




putative






ORF13




11246




12727




amidase




U49269






Moraxella catarrhalis






1108




42






ORF14




12691




14190




PET112




D90913




Synechocystis sp.




1044




46






ORF15




14484




17249




POMP91A




U65942






Chlamydia psittaci






1074




43






ORF16




16039




15770




putative






ORF17




17845




20853




putative






ORF18




21137




22042




putative






ORF19




22046




23476




putative






ORF20




23681




26110




putative






ORF21




26109




25861




putative






ORF22




26241




26978




putative






ORF23




26960




27754




putative






ORF24




27747




28577




putative






ORF25




28887




29492




POMP91A




U65942






Chlamydia psittaci






180




39






ORF26




29432




30028




POMP91A




U65942






Chlamydia psittaci






361




51






ORF27




30024




31472




POMP91A




U65942






Chlamydia psittaci






879




54






ORF28




31758




32288




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






144




43









protein






ORF29




32201




33991




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






1126




48









protein






ORF30




33852




34541




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






589




62









protein






ORF31




34783




36063




POMP91B precursor




U65943






Chlamydia psittaci






469




46






ORF32




36009




37529




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






1338




51









protein






ORF33




37881




39362




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






671




40









protein






ORF34




39418




39161




putative






ORF35




39366




40715




POMP90A precursor




U65942






Chlamydia psittaci






904




47






ORF36




43076




41094




putative






ORF37




43800




43066




putative






ORF38




44828




43785




putative






ORF39




45340




44753




homologous to unidentified


E. coli






M96343






Bacillus subtilis






136




44









protein






ORF40




45752




45372




o530; This 530 aa orf is 33 pct




AE000184






Escherichia coli






269




43









identical (14 gaps) to 525 residues of









an approx. 640 aa protein









YHES_HAEIN SW: P44808






ORF41




46996




45701




ABC transporter, ATP-binding




AE000596






Helicobacter pylori






878




39









protein (yheS)






ORF42




47961




47569




putative






ORF43




48960




48040




hypothetical protein




D64001




Synechocystis sp.




404




37






ORF44




51452




50133




Lon protease-like protein




X74215






Homo sapiens






1232




54






ORF45




52606




51335




unknown




Z54285






Schizosaccharomyces pombe






781




47






ORF46




53684




53319




putative






ORF47




54195




53746




putative






ORF48




55278




56453




heat-shock protein




U15010






Legionella pneumophila






975




45






ORF49




56493




57266




branched chain alpha-keto acid




M97391






Bacillus subtilis






329




36









dehydrogenase E1-alpha






ORF50




57297




58526




branched chain alpha-keto acid




M97391






Bacillus subtilis






707




50









dehydrogenase E1-beta






ORF51




59851




58565




putative






ORF52




61495




59924




ComE




D90903




Synechocystis sp.




134




55






ORF53




61324




62151




putative






ORF54




62132




62470




Hpr protein




X12832






Bacillus subtilis






136




36






ORF55




62474




63733




enzyme I (ptsI)




U32844






Haemophilus influenzae






381




35






ORF56




63881




64186




f831; This 831 aa orf is 46 pct




AE000326






Escherichia coli






123




34









identical (11 gaps) to 709 residues of









an approx. 712 aa protein









PT1A_ECOLI SW: P32670






ORF57




64611




64318




ORF107




X17014






Bacillus subtilis






128




33






ORF58




65485




64673




putative






ORF59




65999




65301




dnaZX-like ORF put. DNA




X06803






Bacillus subtilis






596




52









polymerase III






ORF60




66244




67281




putative






ORF61




67265




67699




putative






ORF62




67703




68539




putative






ORF63




68805




70736




putative






ORF64




69172




68831




putative






ORF65




70642




71142




putative






ORF66




71325




72029




putative






ORF67




72060




73637




putative






ORF68




74061




76175




YqfF




D84432






Bacillus subtilis






542




44






ORF69




78351




77680




porphobilinogen deaminase




D28503






Clostridium josui






262




42






ORF70




79356




78355




sms protein




D90914




Synechocystis sp.




736




52






ORF71




79983




79693




ribonuclease III (rnc)




AE000579






Helicobacter pylori






98




33






ORF72




80441




79938




ORF3




D64116






Bacillus subtilis






268




44






ORF73




80475




80969




putative






ORF74




81296




83080




hypothetical protein




Y14079






Bacillus subtilis






893




38






ORF75




83291




83932




manganese superoxide dismutase




X77021






Caenorhabditis elegans






622




58






ORF76




84005




84769




acetyl-CoA carboxylase beta subunit




AE000604






Helicobacter pylori






602




50









(accD)






ORF77




84975




85244




deoxyuridinetriphosphatase (dut)




U32776






Haemophilus influenzae






110




41






ORF78




85123




85425




deoxyuridine 5′-triphosphate




AE000596






Helicobacter pylori






265




68









nucleotidohydrolase (dut)






ORF79




85397




85903




ORF2




L26916






Pseudomonas aeruginosa






173




34






ORF80




85909




86583




enzyme IIANtr




U18997






Escherichia coli






170




42






ORF81




86626




88065




putative






ORF82




89257




91026




putative






ORF83




91291




93030




putative






ORF84




93295




94086




putative






ORF85




95285




94707




putative






ORF86




95667




96557




putative






ORF87




96317




97456




putative






ORF88




98435




97968




putative






ORF89




99460




98426




putative






ORF90




100144




101325




elongation factor Tu




L22216






Chlamydia trachomatis






1917




95






ORF91




101457




101720




putative






ORF92




101704




102273




transcription factor




L10348






Thermus aquaticus






376




49













thermophilus








ORF93




102356




102805




ribosomal protein L11




D13303






Bacillus subtilis






458




63






ORF94




102835




103530




ribosomal protein L1




Z11839






Thermotoga maritima






642




51






ORF95




103549




104058




ribosomal protein L10




M89911






Streptomyces antibioticus






82




31






ORF96




104096




104491




rp112 (AA 1-128)




X53178




Synechocystis PCC6803




325




47






ORF97




104601




108386




DNA-directed RNA polymerase beta




X64172






Staphylococcus aureus






2740




52









chain






ORF98




108401




112054




rpoC




V00339






Escherichia coli






2947




54






ORF99




112033




112590




acetylornithine deacetylase (EC




M22622






Leptospira biflexa






514




62









5.1.1.16)






ORF100




112672




113682




transaldolase




L19437






Homo sapiens






755




49






ORF101




113726




114121




putative






ORF102




114711




114136




putative






ORF103




115267




115755




putative






ORF104




115911




116543




putative






ORF105




116736




118055




ATPase alpha-subunit




X63855






Thermus aquaticus






934




50













thermophilus








ORF106




117968




118522




adenosine triphosphatase A subunit




D50528






Acetabularia acetabulum






147




32






ORF107




118530




119843




V-ATPase B subunit




U96487




Desulfurococcus sp. SY




751




48






ORF108




119816




120457




putative






ORF109




120451




122430




v-type Na-ATPase




X76913






Enterococcus hirae






264




35






ORF110




122504




122950




ATP synthase, subunit K




U67478






Methanococcus jannaschii






184




31






ORF111




123528




126347




valyl-tRNA synthetase




X05891






Escherichia coli






1679




49






ORF112




126332




129166




protein kinase-like protein




U19250






Streptomyces coelicolor






427




37






ORF113




134690




129213




UvrA




D49911






Thermus thermophilus






3107




41






ORF114




134925




136382




pyruvate kinase




U83196






Chlamydia trachomatis






1748




71






ORF115




137870




136482




HtrB protein




X61000






Escherichia coli






147




38






ORF116




137899




138240




putative






ORF117




138239




137928




putative






ORF118




139558




138257




putative






ORF119




140352




139516




YbbP




AB002150






Bacillus subtilis






231




46






ORF120




140498




141841




cyanide insensitive terminal oxidase




Y10528






Pseudomonas aeruginosa






538




50






ORF121




141855




142658




cyanide insensitive terminal oxidase




Y10528






Pseudomonas aeruginosa






310




40






ORF122




144258




143050




putative






ORF123




145258




144494




putative






ORF124




145454




146749




product similar to


E. coli


PhoH




Z97025






Bacillus subtilis






836




47









protein






ORF125




147318




146767




putative






ORF126




148261




147677




putative






ORF127




149029




152157




isoleucyl-tRNA synthetase




U04953






Homo sapiens






2361




52






ORF128




154108




152201




leader peptidase I




D90904




Synechocystis sp.




225




47






ORF129




155135




154308




putative






ORF130




155141




155467




YtiA




AF008220






Bacillus subtilis






201




43






ORF131




155703




156779




orf 361; ranslated orf similarity to




X78969






Coxiella burnetii






863




59









SW: RF1_SALTY peptide chain









release factor 1 of


Salmonella













typhimurium








ORF132




156748




157635




product similar to


E. coli


PRFA2




Z49782






Bacillus subtilis






144




37









protein






ORF133




157653




158996




Ffh




U82109






Thermus aquaticus






797




45






ORF134




159363




159986




tRNA




U32705






Haemophilus influenzae






545




49









(guanine-N1)-methyltransferase









(trmD)






ORF135




159880




160446




putative






ORF136




160477




160839




ribosomal protein L19




X72627




Synechocystis sp.




319




50






ORF137




160898




161539




putative protein highly homologous




D32253




Magnetospirillum sp.




427




49









to


E. coli


RNase HII.






ORF138




161527




162153




5′ guanylate kinase (gmk)




U32848






Haemophilus influenzae






385




43






ORF139




162144




162443




putative






ORF140




162437




164098




methionyl-tRNA synthetase




AB004537






Schizosaccharomyces pombe






861




54






ORF141




165451




164228




exodeoxyribonuclease V (recD)




U32811






Haemophilus influenzae






432




32






ORF142




166349




165411




putative






ORF143




166949




168442




putative






ORF144




169416




171029




putative






ORF145




170857




171459




putative






ORF146




172652




173428




putative biotin-protein ligase




Z97992






Schizosaccharomyces pombe






292




44






ORF147




174626




173439




putative






ORF148




174816




175613




putative






ORF149




175598




175954




putative






ORF150




175958




176935




putative






ORF151




177708




176938




orf 3′ of chaperonin homolog hypB




S40172






Chlamydia psittaci






376




74









[


Chlamydia psittaci


, pigeon strain









P-1041, Peptide Partial, 98 aa]






ORF152




177128




177376




putative






ORF153




179472




177841




putative




M69217






Chlamydia pneumoniae






2678




100






ORF154




179822




179517




putative




M69217






Chlamydia pneumoniae






498




99






ORF155




181793




179943




Pz-peptidase




D88209






Bacillus licheniformis






1088




38






ORF156




182628




181876




o247; This 247 aa orf is 51 pct




AE000174






Escherichia coli






401




42









identical (0 gaps) to 117 residues of









an approx. 160 aa protein









YPH7_CHRVI SW: P45371






ORF157




184420




183074




glutamate-1-semialdehyde




X53696






Escherichia coli






823




41









2,1-aminomutase






ORF158




184988




184467




ORF_o211




U28377






Escherichia coli






87




54






ORF159




185483




185112




hypothetical protein




D90906




Synechocystis sp.




91




33






ORF160




185902




185483




ribose 5-phosphate isomerase




U28377






Escherichia coli






111




41






ORF161




186174




185839




ribose 5-phosphate isomerase A




U32729






Haemophilus influenzae






190




46









(SP: P27252)






ORF162




187720




186587




hypothetical




D83026






Bacillus subtilis






536




42






ORF163




188318




190933




ATP-dependent protease binding




M29364






Escherichia coli






2010




53









subunit






ORF164




191090




191635




putative






ORF165




191547




192743




putative






ORF166




192969




193469




putative






ORF167




194044




193610




putative






ORF168




194196




195809




unknown




Z84395






Mycobacterium tuberculosis






242




52






ORF169




196088




198073




DNA ligase (EC 6.5.1.2)




M24278






Escherichia coli






1317




46






ORF170




198132




199454




putative






ORF171




199351




202818




putative






ORF172




204552




202999




PcpB




U60175






Sphingomonas






80




41











chlorophenolica






ORF173




205648




204692




putative






ORF174




205807




207327




leucine tRNA synthetase




AF008220






Bacillus subtilis






1595




57






ORF175




207182




207775




leucyl-tRNA synthetase




X06331






Escherichia coli






363




51






ORF176




207779




208267




transfer RNA-Leu synthetase




M88581






Bacillus subtilis






285




43






ORF177




208267




209577




KDO-transferase




Z31593






Chlamydia pneumoniae






2262




100






ORF178




211807




211271




KDO-transferase




X80061






Chlamydia psittaci






105




38






ORF179




212188




211844




putative






ORF180




214079




212448




pyrophosphate-dependent




Z32850






Ricinus communis






1003




45









phosphofructokinase beta subunit






ORF181




214907




214083




CinI




U44893






Butyrivibrio fibrisolvens






111




41






ORF182




216154




215429




putative






ORF183




216115




216678




putative






ORF184




216728




217282




putative






ORF185




217267




217866




putative






ORF186




218593




218261




putative






ORF187




219821




218994




putative






ORF188




221382




220309




putative






ORF189




222719




221433




GMP synthetase




M10101






Escherichia coli






1151




48






ORF190




223521




222724




IMP dehydrogenase




X66859






Acinetobacter calcoaceticus






778




58






ORF191




224499




225008




putative






ORF192




225140




225559




putative






ORF193




225555




226802




putative






ORF194




227800




226892




putative






ORF195




228335




228072




putative






ORF196




229251




228643




putative






ORF197




230983




229622




YqhX




D84432






Bacillus subtilis






1386




56






ORF198




231483




230983




acetyl-CoA carboxylase biotin




U38804






Porphyra purpurea






199




52









carboxyl carrier protein






ORF199




232063




231509




elongation factor P




D64001




Synechocystis sp.




282




32






ORF200




232739




232053




pentose-5-phosphate-3-epimerase




D90911




Synechocystis sp.




463




43






ORF201




233166




234356




putative






ORF202




233518




233165




putative






ORF203




234536




235186




ORF2




L35036






Chlamydia psittaci






570




60






ORF204




235379




236689




putative






ORF205




236680




237618




putative






ORF206




237521




238345




putative






ORF207




238281




238973




putative






ORF208




238871




240115




putative






ORF209




240191




241564




putative






ORF210




242281




241604




YqiZ




D84432






Bacillus subtilis






379




39






ORF211




242933




242274




f222; This 222 aa orf is 48 pct




AE000284






Escherichia coli






382




45









identical (0 gaps) to 208 residues of









an approx. 232 aa protein









YCKA_BACSU SW: P42399






ORF212




243416




242976




arginine repressor protein (argR)




U32800






Haemophilus influenzae






229




46






ORF213




243500




244531




sialoglycoprotease




U15958






Pasteurella haemolytica






565




53






ORF214




244480




246021




oligopeptide permease homolog AII




AF000366






Borrelia burgdorferi






457




34






ORF215




246330




247811




OppAIV




AF000948






Borrelia burgdorferi






453




35






ORF216




247831




249174




OppA gene product




X56347






Bacillus subtilis






255




37






ORF217




249437




251038




dciAE




X56678






Bacillus subtilis






469




37






ORF218




251325




252212




OppB gene product




X56347






Bacillus subtilis






652




42






ORF219




253156




254007




oligopeptidepermease




X89237






Streptococcus pyogenes






574




48






ORF220




253974




254852




ATP binding protein




L18760






Lactococcus lactis






433




40






ORF221




255258




256094




KDO-transferase




X80061






Chlamydia psiitaci






106




46






ORF222




256640




257455




putative






ORF223




257502




258239




2-OXOGLUTARAT




A47930






Spinacia oleracea






636




52






ORF224




257869




257501




putative






ORF225




259248




260897




pyrophosphate-fructose 6-phosphate




M55191






Solanum tuberosum






1055




44









1-phosphotransferase beta-subunit






ORF226




262753




261788




putative






ORF227




263059




262757




putative






ORF228




264375




263182




putative






ORF229




265985




264747




putative






ORF230




266637




266059




putative






ORF231




267338




266538




putative






ORF232




267922




267473




putative






ORF233




269647




270771




tRNA guanine transglycosylase




L33777






Zymomonas mobilis






628




44






ORF234




272777




273145




ORF4




D00624




Bacteriophage chp1




100




41






ORF235




273253




273636




putative






ORF236




273705




273977




putative






ORF237




276016




275717




putative






ORF238




276439




276020




putative






ORF239




276792




277253




putative






ORF240




277318




277599




putative






ORF241




278578




277877




putative






ORF242




279258




278554




FbpC




U33937






Neisseria gonorrhoeae






312




39






ORF243




280435




279533




putative






ORF244




281547




280849




putative






ORF245




281696




282325




CMP-2-keto-3-deoxyoctulosonic




U15192






Chlamydia trachomatis






637




63









acid synthetase






ORF246




282459




284069




CTP synthetase




U15192






Chlamydia trachomatis






2000




68






ORF247




284056




284517




ORF3




U15192






Chlamydia trachomatis






453




65






ORF248




284606




285775




glucose 6-phosphate dehydrogenase




U83195






Chlamydia trachomatis






1263




77






ORF249




285592




285987




glucose 6-phosphate dehydrogenase




U83195






Chlamydia trachomatis






519




79






ORF250




286179




286976




glucose-6-phosphate dehydrogenase




D88189






Actinobacillus






216




40









isozyme





actinomycetemcomitans






ORF251




287583




287002




putative






ORF252




287951




287451




putative






ORF253




288499




288816




putative






ORF254




289674




288505




putative






ORF255




288839




289213




putative






ORF256




289970




290254




putative






ORF257




291931




292803




gamma-D-glutamyl-L-diamino acid




X64809






Bacillus sphaericus






95




39









endopeptidase II






ORF258




293258




292755




ScoS9




U43429






Streptomyces coelicolor






233




45






ORF259




293718




293272




ribosomal protein L13 (rpLl3)




U32823






Haemophilus influenzae






364




47






ORF260




294630




293953




glutamine transport ATP-binding




U67524




Methanococcus jannaschii




387




46









protein Q






ORF261




296153




294636




putative






ORF262




294817




295068




putative






ORF263




296354




297862




conserved hypothetical protein




AE000586






Helicobacter pylori






641




46






ORF264




298415




297879




putative






ORF265




298777




298253




putative






ORF266




299572




298781




putative






ORF267




300487




299633




putative






ORF268




301586




300702




putative






ORF269




302440




301571




putative






ORF270




302838




302437




putative






ORF271




303335




302745




putative






ORF272




304394




303852




putative






ORF273




304606




305223




f311; This 311 aa orf is 22 pct




AE000232






Escherichia coli






250




38









identical (13 gaps) to 186 residues of









an approx. 488 aa protein









YACA_BACSU SW: P37563; pyul









of D21139






ORF274




305394




306236




survival protein surE




U81296






Sinorhizobium meliloti






156




42






ORF275




306501




307439




YqfU




D84432






Bacillus subtilis






547




42






ORF276




308033




307458




3-octaprenyl-4-hydroxybenzoate




U61168






Bacillus firmus






403




42









carboxy-lyase






ORF277




308924




308037




4-hydroxybenzoate




U61168






Bacillus firmus






152




40









octaprenyltransferase






ORF278




309485




310180




putative






ORF279




310426




311214




putative






ORF280




311597




311253




putative






ORF281




312772




311780




putative






ORF282




313425




312772




putative






ORF283




313646




313377




putative






ORF284




313937




314665




lysophospholipase homolog




AF006678






Schistosoma mansoni






141




44






ORF285




315576




314755




dnaZX




X17014






Bacillus subtilis






154




39






ORF286




316157




315531




unknown




D26185






Bacillus subtilis






284




31






ORF287




318657




316156




DNA gyrase




L47978






Aeromonas salmonicida






1785




48






ORF288




321042




318676




DNA gyrase subunit B




U35453






Clostridium acetobutylicum






1838




59






ORF289




321445




321098




putative






ORF290




322309




321710




putative






ORF291




323190




322366




outer membrane protein




AE000654






Helicobacter pylori






376




43






ORF292




323843




323181




hypothetical




U70214






Escherichia coli






356




37






ORF293




324878




323856




ATP-binding protein (abc)




U32744






Haemophilus influenzae






545




44






ORF294




325340




326410




f374; This 374 aa orf is 30 pct




AE000299






Escherichia coli






1194




62









identical (9 gaps) to 102 residues of









an approx. 512 aa protein









FLIC_SALMU SW: P06177






ORF295




326433




327836




Xas A




AE000246






Escherichia coli






479




33






ORF296




328465




327839




putative






ORF297




329360




328857




putative






ORF298




330907




329357




putative






ORF299




332455




330956




MgtE




U18744






Bacillus firmus






203




36






ORF300




334536




332395




putative






ORF301




336091




334877




putative






ORF302




336103




337302




putative






ORF303




338129




338830




putative






ORF304




338965




339501




putative






ORF305




339508




340143




putative






ORF306




340247




342967




putative






ORF307




343385




343810




cAMP-dependent protein kinase type




U75932






Rattus norvegicus






102




37









I regulatory subunit






ORF308




344171




343935




acyl carrier protein (acpP)




AE000570






Helicobacter pylori






198




55






ORF309




345082




344330




3-ketoacyl-ACP reductase




U39441






Vibrio harveyi






598




48






ORF310




346005




345082




malonyl-CoA: Acyl carrier protein




U59433






Bacillus subtilis






538




45









transacylase






ORF311




346784




346437




beta-ketoacyl-acyl carrier protein




AE000540






Helicobacter pylori






273




50









synthase III (fabH)






ORF312




347029




346715




beta-ketoacyl-acyl carrier protein




M77744






Escherichia coli






265




63









synthase III






ORF313




347034




347723




recombination protein




D90916




Synechocystis sp.




363




42






ORF314




348075




350459




putative






ORF315




350598




351071




putative






ORF316




351075




352175




rifampicin resistance protein




L22690






Rickettsia rickettsii






495




46






ORF317




353291




352230




putative






ORF318




353442




354467




pyruvate dehydrogenase E1




D90915




Synechocystis sp.




571




44









component, alpha subunit






ORF319




354451




354933




pyruvate dehydrogenase E1 beta




U09137






Arabidopsis thaliana






495




59









subunit






ORF320




355000




355449




pyruvate dehydrogenase E1




U38804






Porphyra purpurea






336




47









component, beta subunit






ORF321




355448




356743




F23B12.5




Z77659






Caenorhabditis elegans






759




46






ORF322




355953




355642




putative






ORF323




359310




356827




glycogen phosphorylase B




U47025






Homo sapiens






2193




57






ORF324




359120




359377




putative






ORF325




359525




359908




putative






ORF326




361290




359947




DnaA




D89066






Staphylococcus aureus






375




46






ORF327




363785




361362




hypothetical




U32781






Haemophilus influenzae






394




44






ORF328




364496




363888




putative






ORF329




364832




365290




putative






ORF330




365304




365669




dpj




M76470






Escherichia coli






160




45






ORF331




366599




365667




NADPH thioredoxin reductase




AC002329






Arabidopsis thaliana






975




60






ORF332




367291




369030




ribosomal protein S1 (rpS1)




U32801






Haemophilus influenzae






1209




41






ORF333




369134




369808




NusA




U74759






Chlamydia trachomatis






995




87






ORF334




369917




370438




NusA




U74759






Chlamydia trachomatis






760




87






ORF335




370365




372647





U74759






Chlamydia trachomatis






2173




61






ORF336




372557




373066




initiation factor IF2-beta (infB; gtg




X00513






Escherichia coli






333




39









start codon)






ORF337




373020




373442




ORF6 gene product




Z18631






Bacillus subtilis






192




34






ORF338




373467




374195




tRNA pseudouridine 55 synthase




D90917




Synechocystis sp.




358




47






ORF339




374176




375099




hypothetical 34.6 kD protein in




AE000113






Escherichia coli






395




39









rpsT-ileS intergenic region






ORF340




375676




375083




hypothetical GTP-binding protein in




AE000219






Escherichia coli






507




53









pth 3′ region






ORF341




376173




375634




hypothetical




U32723






Haemophilus influenzae






480




59






ORF342




376564




377643




YscU




U08019






Yersinia enterocolitica






538




37






ORF343




377956




379773




IcrD gene product




X67771






Yersinia enterocolitica






1302




47






ORF344




379781




380425




putative






ORF345




380281




381000




putative






ORF346




381008




381460




putative






ORF347




381460




383037




4-alpha-glucanotransferase




L37874






Clostridium butyricum






302




38






ORF348




383257




383523




ribosomal protein L28 (rpL28)




U32776






Haemophilus influenzae






175




55






ORF349




383553




385304




hypothetical protein




D90901




Synechocystis sp.




565




38






ORF350




385397




386458




comE ORF1




D64002




Synechocystis sp.




187




10






ORF351




387242




386514




putative






ORF352




388764




387013




putative






ORF353




390120




390932




methylenetetrahydrofolate




D64000




Synechocystis sp.




588




53









dehydrogenase






ORF354




390919




391818




f351; Residues 1-121 are 100 pct




AE000310






Escherichia coli






186




39









identical to YOJL_ECOLI SW:









P33944 (122 aa) and aa 152-351 are









100 pct identical to YOJK_ECOLI









SW: P33943






ORF355




392379




391885




small protein




D90914




Synechocystis sp.




387




46






ORF356




392582




392986




putative






ORF357




392776




393684




putative






ORF358




394151




394804




RecF protein




D90907




Synechocystis sp.




232




34






ORF359




394928




395308




putative






ORF360




395259




395990




putative






ORF361




397815




395953




hypothetical




U32773






Haemophilus influenzae






391




36






ORF362




398850




397831






H. influenzae


predicted coding




U32763






Haemophilus influenzae






580




39









region H10807






ORF363




400085




399099




putative






ORF364




401245




400073




YtgC




AF008220






Bacillus subtilis






244




30






ORF365




401474




401136




putative






ORF366




402199




401423




unknown




U52850






Erysipelothrix rhusiopathiae






534




46






ORF367




403193




402186




putative






ORF368




403650




404165




putative






ORF369




404343




405914




adenine nucleotide translocase




Z49227






Arabidopsis thaliana






1280




55






ORF370




405984




407327




putative






ORF371




407712




408806




putative






ORF372




410439




409075




putative






ORF373




411826




410954




putative






ORF374




412482




414302




lepA gene product




X91655






Bacillus subtilis






1827




59






ORF375




415402




414407




6-phosphogluconate dehydrogenase,




U32737






Haemophilus influenzae






687




51









decarboxylating (gnd)






ORF376




415848




415237




6-phosphogluconate dehydrogenase,




S67873






Ceratitis capitata






695




64









6PGD [


Ceratitis capitata


= medflies,









Peptide, 481 aa]






ORF377




417131




415866




tyrosyl-tRNA synthetase (tyrS)




J01719






Escherichia coli






821




45






ORF378




417258




417566




putative






ORF379




418326




417454




whiG-Stv gene product




X68709






Streptoverticillium






464




41











griseocarneum






ORF380




420057




418426




FLHA gene product




X63698






Bacillus subtilis






455




49






ORF381




420448




420720




ferredoxin IV




M59855






Rhodobacter capsulatus






174




63






ORF382




420980




421552




putative






ORF383




421556




422029




putative






ORF384




422461




422925




putative






ORF385




423562




424320




putative






ORF386




424250




424591




putative






ORF387




424830




426047




putative






ORF388




426240




427397




putative






ORF389




428841




430703




GcpE




D90908




Synechocystis sp.




877




47






ORF390




430694




431446




YfiH




U50134






Escherichia coli






136




35






ORF391




431597




432100




putative






ORF392




432165




432779




putative






ORF393




433272




432832




dihydrolipoamide




U32839






Haemophilus influenzae






475




64









succinyltransferase (sucB)






ORF394




433925




433227




dihydrolipoamide




U32839






Haemophilus influenzae






332




45









succinyltransferase (sucB)






ORF395




436678




433934




alpha-ketoglutarate dehydrogenase




U41762






Rhodobacter capsulatus






1530




44






ORF396




437176




438357




oxygen-independent




AE000628






Helicobacter pylori






442




42









coproporphyrinogen III oxidase









(hemN)






ORF397




440317




438518




putative






ORF398




440001




440345




putative






ORF399




441233




440517




ORF_f286




U18997






Escherichia coli






168




45






ORF400




440719




441012




putative






ORF401




442192




441230




putative






ORF402




442888




442343




putative






ORF403




442371




442961




putative






ORF404




443578




443003




[karp] gene products




M86605






Chlamydia trachomatis






505




78






ORF405




444500




443526




aminopeptidase




D17450






Mycoplasma salivarium






273




39






ORF406




444842




444528




putative






ORF407




445009




444743




putative




L39923






Mycobacterium leprae






133




33






ORF408




445718




445182




putative






ORF409




445807




447804




Su1p




U18908






Zea mays






1307




52






ORF410




448738




447803




putative






ORF411




449628




448618




RuvB protein




U38840






Thermotoga maritima






845




53






ORF412




450298




450867




deoxycytidine triphosphate




AE000554






Helicobacter pylori






573




58









deaminase (dcd)






ORF413




450713




451207




putative






ORF414




451211




452452




hemolysin




D90914




Synechocystis sp.




227




39






ORF415




452448




453659




similar to [SwissProt Accession




D90888






Escherichia coli






96




33









Number P37908]






ORF416




454843




453725




NifS gene product




L34879






Anabaena azollae






533




38






ORF417




455608




454865




hypothetical protein




D90908




Synechocysus sp.




371




36






ORF418




456243




457007




putative






ORF419




457016




457708




putative






ORF420




458368




457979




unknown




D26185






Bacillus subtilis






152




36






ORF421




459496




458372




mutY homolog




U63329






Homo sapiens






466




46






ORF422




459493




460194




hypothetical protein




D90914




Synechocystis sp.




98




38






ORF423




461446




460355




putative






ORF424




462298




461450




putative






ORF425




462444




463349




enoyl-ACP reductase




Y13861






Nicotiana tabacum






1008




69






ORF426




464241




463342




putative






ORF427




464574




465065




putative






ORF428




465129




465611




putative






ORF429




465571




466317




putative






ORF430




466317




467093






H. pylori


predicted coding region




AE000536






Helicobacter pylori






246




36









HP0152






ORF431




466999




467502




putative






ORF432




469691




467715




unidentified transporter-ATP binding




Z82044






Bacillus subtilis






496




45






ORF433




470691




469660




acetyl-CoA carboxylase subunit




AF008220






Bacillus subtilis






781




52






ORF434




472010




470709




putative






ORF435




471545




471799




putative






ORF436




472359




472045




putative






ORF437




473523




472732




orf1




X75413






Escherichia coli






313




42






ORF438




474889




473441




murE gene product




Z15056






Bacillus subtilis






679




37






ORF439




477323




475365




penicillin-binding protein 2




X59630






Neisseria meningitidis






451




42






ORF440




478496




477597




hypothetical protein




D90906




Synechocystis sp.




534




52






ORF441




478722




479273




putative






ORF442




479277




479705




putative






ORF443




480050




481450




chromosomal replication initiator




D90909




Synechocystis sp.




793




40









protein DnaA






ORF444




481469




482053




OrfH




U35673






Borrelia burgdorferi






157




37






ORF445




482600




482025




putative






ORF446




482654




484204




NADH: ubiquinone oxidoreductase




Z37111






Vibrio alginolyticus






801




49









subunit B






ORF447




484211




485170




NADH: ubiquinone oxidoreductase




U32702






Haemophilus influenzae






258




48









(GP: Z37111_4)






ORF448




485170




485838




NADH: uniquinone oxidoreductase




Z37111






Vibrio alginolyticus






543




55






ORF449




485813




486580




unidentified protein of




D49364






Vibrio alginolyticus






488




48









Na+-translocating NADH-quinone









reductase






ORF450




486976




486638




putative






ORF451




489071




487764




putative






ORF452




489341




489090




putative






ORF453




489958




489152




putative






ORF454




490549




489962




putative






ORF455




491163




490522




putative






ORF456




491396




491112




putative






ORF457




492121




491390




putative






ORF458




492304




494838




ClpC adenosine triphosphatase




U02604






Bacillus subtilis






2370




46






ORF459




495943




494822




hypothetical protein in purB 5′




AE000213






Escherichia coli






927




53









region






ORF460




496011




496565




putative






ORF461




496569




497228




putative






ORF462




497358




497834




putative






ORF463




497770




498327




putative






ORF464




499209




499589




putative






ORF465




499520




499792




putative






ORF466




500774




504169




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






1215




45









protein






ORF467




504139




504600




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






319




47









protein






ORF468




504865




506877




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






992




42









protein






ORF469




506790




507671




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






739




46









protein






ORF470




507718




510507




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






1813




42









protein






ORF471




508325




507912




putative






ORF472




510660




513440




POMP90A precursor




U65942






Chlamydia psittaci






1830




46






ORF473




514965




513787




hypothetical




D83026






Bacillus subtilis






482




48






ORF474




517347




515419




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






1554




51









protein






ORF475




517058




517363




putative






ORF476




517798




517277




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






222




41









protein






ORF477




518200




517847




POMP91B precursor




U65943






Chlamydia psittaci






162




42






ORF478




518300




521146




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






1900




45









protein






ORF479




521392




522948




POMP91A




U65942






Chlamydia psittaci






490




39






ORF480




523244




524809




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






507




35









protein






ORF481




524379




524125




putative






ORF482




524649




526238




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






969




41









protein






ORF483




526265




527104




putative






ORF484




526947




526702




putative






ORF485




526975




528450




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






197




48









protein






ORF486




528408




529199




putative outer membrane protein




U72499






Chlamydia psittaci






154




37






ORF487




530612




529542




putative






ORF488




531656




530616




putative






ORF489




533974




532067




putative






ORF490




536432




534324




putative






ORF491




537150




536707




putative






ORF492




537928




537080




putative






ORF493




538438




537932




putative






ORF494




538737




538333




putative






ORF495




539594




539127




putative






ORF496




541215




539590




putative






ORF497




542571




541282




putative






ORF498




543014




542457




putative






ORF499




543369




542962




putative






ORF500




543809




546628




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






506




89









protein






ORF501




546619




549525




POMP91A




U65942






Chlamydia psittaci






128




50






ORF502




547293




546994




putative






ORF503




549699




550523




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






96




32









protein






ORF504




550490




551551




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






223




33









protein






ORF505




551448




552623




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






139




46









protein






ORF506




552652




555117




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






487




48









protein






ORF507




555029




555493




putative






ORF508




558006




555673




putative






ORF509




559694




558162




putative






ORF510




558208




558573




putative






ORF511




561692




559899




putative






ORF512




561412




561708




putative






ORF513




563942




561777




1,4-alpha-glucan branching enzyme




X73903






Streptomyces coelicolor






1743




45






ORF514




564969




563950




putative






ORF515




566204




564936




YqeV




D84432






Bacillus subtilis






639




38






ORF516




567717




566302




putative GTPase required for high




U00005






Escherichia coli






686




41









frequency lysogenization by









bacteriophage lambda






ORF517




568526




567708




putative






ORF518




569467




568742




putative






ORF519




571065




569431




putative






ORF520




571828




571118




arginine-binding periplasmic protein




AE000188






Escherichia coli






197




45









1 precursor






ORF521




572202




573308




putative






ORF522




573146




575056




putative






ORF523




575023




575916




carboxysome formation protein




D90901




Synechocystis sp.




557




59






ORF524




577891




576497




putative






ORF525




578914




578204




putative






ORF526




579924




578857




putative






ORF527




580187




579858




protein kinase C inhibitor




D90906




Synechocystis sp.




260




49






ORF528




580017




580406




putative






ORF529




581086




580187




Yer156cp




U18917






Saccharomyces cerevisiae






176




34






ORF530




581367




581828




putative






ORF531




581678




582367




putative






ORF532




582361




583428




putative






ORF533




584690




583431




putative






ORF534




585237




584950




putative






ORF535




585626




586888




hypothetical protein




D64004




Synechocystis sp.




805




45






ORF536




586846




587907




putative






ORF537




589049




588180




putative






ORF538




590500




589301




putative






ORF539




590755




592458




aminoacyl-tRNA synthetase




L25105






Chlamydia trachomatis






2125




71






ORF540




592526




592903




has homology to putative heat shock




L25105






Chlamydia trachomatis






324




59









proteins of


Bacillus subtilis


and











Clostridium acetobutylicum


; ORFA;









putative






ORF541




592836




593747




Possible negative regulator of




U52216






Chlamydia trachomatis






960




65









CIRCE element; Homologs in


B.













subtilis


and Clostridia spp. referred









to as hrcA or orfA






ORF542




593747




594298




grpE




M62819






Chlamydia trachomatis






661




71






ORF543




594331




595947




DnaK protein homolog; 71,550 Da;




M69227






Chlamydia pneumoniae






2619




100









putative






ORF544




595905




596309




DnaK protein homolog; 71,550 Da;




M69227






Chlamydia pneumoniae






674




100









putative






ORF545




596514




597215




putative






ORF546




597184




597957




vacB gene product




U14003






Escherichia coli






306




48






ORF547




597755




598612




ORF-2




D11024






Shigella flexneri






168




46






ORF548




598602




599204




homologous to DNA glycosylases;




D83026






Bacillus subtilis






374




47









hypothetical






ORF549




599373




599939




putative






ORF550




600903




602072




hemolysin




X73141






Serpulina hyodysenteriae






362




36






ORF551




602240




602587




hypothetical protein




D90908




Synechocystis sp.




182




35






ORF552




602637




603272




putative






ORF553




603142




604512




putative






ORF554




604627




605853




conserved hypothetical protein




AE000579






Helicobacter pylori






423




40






ORF555




605790




606620




putative






ORF556




606571




607281




putative




L14679






Lactococcus lactis






384




45






ORF557




609004




607355




putative






ORF558




610906




609932




putative






ORF559




611786




611004




diaminopimelate epimerase




D90917




Synechocystis sp.




207




55






ORF560




612333




611746




ATP-dependent Clp protease




D90915




Synechocystis sp.




389




44









proteolytic subunit






ORF561




613897




612341




serine hydroxymethyltransferase




D90903




Synechocystis sp.




909




52






ORF562




615179




616279




putative






ORF563




616610




617383




putative






ORF564




618796




617810




ORF_o328




U18997






Esherichia coli






413




45






ORF565




620004




618826




branched chain alpha-keto acid




M97391






Bacillus subtilis






688




41









dehydrogenase E2






ORF566




619649




619918




putative






ORF567




621265




620021




Hypothetical protein




Y14083






Bacillus subtilis






727




37






ORF568




622359




621265




hypothetical




U32691






Haemophilus influenzae






294




52






ORF569




623420




622560




rRNA methylase




D90913




Synechocyslis sp.




244




38






ORF570




624297




623335




hypothetical protein (SP: P39587)




U67605






Methanococcus jannaschii






147




35






ORF571




624773




624174




riboflavin synthase alpha chain




AE000261






Escherichia coli






424




50






ORF572




625029




625484




ORF168




D28752




Synechococcus sp.




323




43






ORF573




625488




625883




YteA




AF008220






Bacillus subtilis






172




35






ORF574




625892




626395




signalpeptidase II




X78084






Staphylococcus carnosus






204




38






ORF575




626444




627790




D-alanine permease (dagA)




U32770






Haemophilus influenzae






566




33






ORF576




627912




628607




putative






ORF577




628774




629697




putative






ORF578




629660




631639




POMP91A




U65942






Chlamydia psittaci






579




44






ORF579




631725




633551




putative






ORF580




633520




636957




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






266




45









protein






ORF581




637232




638098




adhesion protein




D90903




Synechocystis sp.




267




38






ORF582




640648




639593




GTP-binding protein




D90901




Synechocystis sp.




759




45






ORF583




640979




640728




50S ribosomal protein L27




U38804






Porphyra purpurea






265




65






ORF584




641327




641007




50S ribosomal subunit protein L21




U18997






Escherichia coli






210




41






ORF585




641687




642283




hypothetical protein




D90906




Synechocystis sp.




76




39






ORF586




643023




642286




assimilatory sulfite reductase




L26503






Saccharomyces cerevisiae






284




42






ORF587




643330




643076




putative






ORF588




643704




643351




ribosomal protein S10 (rpS10)




U32761






Haemophilus influenzae






349




69






ORF589




645628




643676




translation elongation factor EF-G




AF000625






Helicobacter pylori






1991




58









(fusA)






ORF590




645783




645538




elongation factor G (AA 1-691)




X16278






Thermus aquaticus






170




80













thermophilus








ORF591




646269




645793




ribosomal protein S7




Z11567






Chlamydia trachomatis






730




88






ORF592




646751




646314




ribosomal protein S12 (AA 1-123)




X52912






Cryptomonas phi






485




67






ORF593




647848




647045




putative






ORF594




648393




650336




ORF of prc gene (alt.)




D00674






Escherichia coli






554




42






ORF595




651016




650420




hypothetical sulfur-rich protein




U41759






Chlamydia psittaci






301




50






ORF596




652956




651289




60 kDa CrP




X53511






Chlamydia pneumoniae






2951




100






ORF597




653395




653126




9 kDa CrP




X53511






Chlamydia pneumoniae






502




99






ORF598




655740




654193




glutamyl-tRNA synthetase homolog




U41759






Chlamydia psittaci






2259




82






ORF599




656508




655966




early stage-specific transcription




L13598






Chlamydia psittaci






666




62









experimentally demonstrated; early









upstream open reading frame (EUO)






ORF600




658140




657022




unknown




U41759






Chlamydia psittaci






950




44






ORF601




660216




658525




RecJ recombination protein




U41759






Chlamydia psittaci






807




73






ORF602




663238




660248




protein-export membrane protein




D64000




Synechocystis sp.




413




41









SecD






ORF603




664461




663157




putative






ORF604




665735




664635




putative






ORF605




666212




666994




hypothetical protein




D64006




Synechocystis sp.




538




58






ORF606




666998




667921




o298; This 298 aa orf is 33 pct




AE000238






Escherichia coli






253




45









identical (24 gaps) to 248 residues of









an approx. 256 aa protein









CDSA_ECOLI SW: P06466






ORF607




667909




668568




cytidylate kinase




AE000193






Escherichia coli






400




48






ORF608




668502




669203




hypothetical protein




D90915




Synechocyslis sp.




225




33






ORF609




669154




670893




arginyl-tRNA-synthetase




D64006




Synechocystis sp.




1365




49






ORF610




672226




670853




UDP-N-acetylglucosamine




U32788






Haemophilus influenzae






642




40









enolpyruvyl transferase (murZ)






ORF611




671137




671424




putative






ORF612




672453




673001




putative






ORF613




673072




674721




putative






ORF614




674549




674262




putative






ORF615




675518




674796




ORF246 gene product




X59551






Escherichia coli






520




43






ORF616




676083




675499




putative






ORF617




676630




676067




putative






ORF618




677016




676600




ORF3




D10279






Bacillus subtilis






361




63






ORF619




677647




677015




peptide release factor 2




X99401






Bacillus firmus






427




43






ORF620




677990




678259




unknown




Z49939






Saccharomyces cerevisiae






175




48






ORF621




679444




680097




unknown




D26185






Bacillus subtilis






263




38






ORF622




680097




680897




unknown




D64126






Bacillus subtilis






506




45






ORF623




681637




680849




putative






ORF624




681409




682281




putative






ORF625




682453




682821




putative






ORF626




682763




683902




sensor protein




L39904






Myxococcus xanthus






190




48






ORF627




684616




683969




putative






ORF628




685169




684534




putative






ORF629




685986




685117




putative






ORF630




686278




687288




NtrC/NifA-like protein regulator




U17902






Escherichia coli






820




45






ORF631




687483




688151




putative






ORF632




688740




689501




putative






ORF633




690242




689622




putative






ORF634




690470




691126




unknown




Z48008






Saccharomyces cerevisiae






380




46






ORF635




692600




691497




putative






ORF636




692674




695064




phenylalanyl-tRNA synthetase




U32810






Haemophilus influenzae






593




45









beta-subunit (pheT)






ORF637




695049




696032




putative






ORF638




697964




696585




OppC-like protein




D85103




Synechococcus sp.




371




37






ORF639




699803




698274




OppB gene product




X56347






Bacillus subtilis






197




40






ORF640




701926




699788




AppA




U20909






Bacillus subtilis






324




43






ORF641




703196




702567




putative






ORF642




704221




703208




putative






ORF643




704240




705289




ferrochelatase




X73417






Arabidopsis thaliana






266




42






ORF644




706070




705300




histidine periplasmic binding protein




U58045






Campylobacter jejuni






128




31









P29






ORF645




706841




706254




conserved hypothetical protein




AE000592






Helicobacter pylori






155




37






ORF646




707596




706811




putative






ORF647




708666




707677




ADP-glucose pyrophosphorylase




X55650






Solanum tuberosum






595




43






ORF648




709793




709119




pyrE-F gene product




X71842






Arabidopsis thaliana






400




44






ORF649




711523




710132




transcription termination factor




J01673






Escherichia coli






1251




60






ORF650




712236




711523




putative






ORF651




714734




712125




DNA polymerase I




J04479






Streptococcus pneumoniae






1334




43






ORF652




715759




714761




protease IV




U67512






Methanococcus jannaschii






101




55






ORF653




717538




715886




adenine nucleotide translocase




Z49227






Arabidopsis thaliana






832




39






ORF654




719113




720243




replicative DNA helicase




D26185






Bacillus subtilis






776




44






ORF655




720590




722422




homologous to


E. coli


gidA




X62540






Pseudomonas putida






1575




52






ORF656




722406




723056




putative






ORF657




723551




723120




nucleoside 5′-diphosphate




J05207






Myxococcus xanthus






451




62









phosphotransferase (EC 2.7.4.6)






ORF658




724246




723626




Holliday junction DNA helicase




U32716






Haemophilus influenzae






293




43









(ruvA)






ORF659




724754




724251




crossover junction




U32717






Haemophilus influenzae






296




53









endodeoxyribonuclease (ruvC)






ORF660




725868




724900




putative






ORF661




727115




726270




putative






ORF662




728126




727119




glyceraldehyde-3-phosphate




U83198






Chlamydia trachomatis






1340




75









dehydrogenase






ORF663




728594




728208




ribosomal protein L17




L33834






Chlamydia trachomatis






439




82






ORF664




729614




728604




RNA polymerase alpha-subunit




L33834






Chlamydia trachomatis






1356




89






ORF665




729778




729533




RNA polymerase alpha-subunit




L33834






Chlamydia trachomatis






273




82






ORF666




730149




729751




ribosomal protein S11




L33834






Chlamydia trachomatis






562




90






ORF667




730539




730174




ribosomal protein S13




L33834






Chlamydia trachomatis






544




89






ORF668




731983




730598




homolog




L25077






Chlamydia trachomatis






1956




83






ORF669




732427




731996




ribosomal protein CtrL15e




M80325






Chlamydia trachomatis






563




77






ORF670




732917




732423




ribosomal protein CtrS5e




M80325






Chlamydia trachomatis






702




84






ORF671




733598




733320




ribosomal protein L6




M60652






Chlamydia trachomatis






316




87






ORF672




733869




733492




ribosomal protein L6




M60652






Chlamydia trachomatis






469




77






ORF673




734298




733900




ribosomal protein CtrS8e




M80325






Chlamydia trachomatis






572




82






ORF674




734858




734319




ribosomal protein CtrL5e




M80325






Chlamydia trachomatis






730




90






ORF675




735195




734863




ribosomal protein CtrL24e




M80325






Chlamydia trachomatis






420




70






ORF676




735578




735342




ribosomal protein CtrL14e




M80325






Chlamydia trachomatis






270




95






ORF677




735861




735604




ribosomal protein S17e




M80325






Chlamydia trachomatis






322




77






ORF678




736492




736079




50S ribosomal protein L16




D90905




Synechocystis sp.




439




60






ORF679




737192




736524




ribosomal protein S3




D64071






Actinobacillus






612




58













actinomycetemcomitans








ORF680




737555




737211




ribosomal protein L22




Z21677






Thermotoga maritima






228




48






ORF681




738688




737837




50S ribosomal subunit protein L2




U18997






Escherichia coli






769




62






ORF682




739048




738713




putative






ORF683




739736




739065




ribosomal protein L4




X67014






Bacillus stearothermophilus






308




46






ORF684




740477




739773




ribosomal protein L3




Z46265






Thermus aquaticus






463




50













thermophilus








ORF685




740659




740958




putative






ORF686




741722




740721




putative






ORF687




742789




741827




methionyl-tRNA formyltransferase




D64001




Synechocystis sp.




511




48






ORF688




743618




742782




UDP-N-acetylglucosamine




L22690






Rickettsia rickettsii






542




43









acyltransferase






ORF689




744092




743634




(3R)-hydroxymyristol acyl carrier




D90910




Synechocystis sp.




339




55









protein dehydrase






ORF690




744604




744107




UDP-3-0-acyl N-acetylglcosamine




D90902




Synechocystis sp.




287




45









deacetylase






ORF691




744953




744498




UDP-3-O-acyl-GlcNAc deacetylase




U67855






Pseudomonas aeruginosa






262




51






ORF692




746608




744986




apolipoprotein N-acyltransferase




U32716






Haemophilus influenzae






194




50









(cute)






ORF693




747085




746621




low homology to P14 protein of




D78189






Bacillus subtilis






235




37











Heamophilus influenzar


and 14.2









kDa protein of


Escherichia coli








ORF694




747974




747219




polymerase III




M22996






Bacillus subtilis






180




34






ORF695




748594




748169




hypothetical protein




D90914




Synechocystis sp.




160




43






ORF696




749145




748573




putative






ORF697




749652




749957




trxA




L39892






Chlamydia psittaci






393




72






ORF698




750446




749979




spoU




L39892






Chlamydia psittaci






559




72






ORF699




751219




750446




mip




L39892






Chlamydia psittaci






948




60






ORF700




753042




751291




aspartyl-tRNA synthetase




D90910




Synechocystis sp.




1347




47






ORF701




754309




753020




histidine-tRNA ligase




Z17214






Streptococcus equisimilis






757




44






ORF702




755120




756175




hexosephosphate transport protein




M89480






Salmonella typhimurium






870




49






ORF703




756120




756485




hexosephosphate transport protein




M89479






Escherichia coli






321




45






ORF704




756499




760227




DNA polymerase III alpha-subunit




AE000646






Helicobacter pylori






1977




42









(dnaE)






ORF705




761217




760297




putative






ORF706




761297




761809




putative






ORF707




761782




762282




putative






ORF708




762260




762895




putative






ORF709




762867




763316




hypothetical protein




D90908




Synechocystis sp.




177




43






ORF710




763780




763325




putative






ORF711




763861




765168




DD-carboxypeptidase




M85047






Bacillus subtilis






292




37






ORF712




766809




765697




fmu and fmv protein




D90902




Synechocystis sp.




130




36






ORF713




768051




766888




putative






ORF714




768566




768321




putative






ORF715




769342




768551




putative






ORF716




770532




769378




putative






ORF717




771451




770804




putative






ORF718




773058




771847




3-phosphoglycerate kinase




U83197






Chlamydia trachomatis






1540




72






ORF719




773094




773456




putative






ORF720




774376




773093




putative phosphate permease




U84890






Mesembryanthemum






870




45













crystallinum








ORF721




775123




774380




putative






ORF722




775398




774916




putative






ORF723




775046




776077




sporulation protein




M57689






Bacillus subtilis






698




43






ORF724




776070




777041




was dppE




U00039






Escherichia coli






565




56






ORF725




777964




777536




orf288; translated orf similarity to




Y10436






Coxiella burnetii






256




46









SWISS-PROT: YGI2_PSEPU









hypothetical 32.4 kDa protein of











Pseudomomas putida








ORF726




778176




777904






B. subtilis


genes rpmH, rnpA, 50 kd,




X62539






Bacillus subtilis






112




37









gidA and gidB






ORF727




778621




779334




putative






ORF728




781173




780307




f406; This 406 aa orf is 28 pct




AE000263






Escherichia coli






603




40









identical (12 gaps) to 264 residues of









an approx. 440 aa protein









YAOA_SCHPO SW: Q10089






ORF729




781526




781116




f406; This 406 aa orf is 28 pct




AE000263






Escherichia coli






258




45









identical (12 gaps) to 264 residues of









an approx. 440 aa protein









YAOA_SCHPO SW: Q10089






ORF730




782784




781555




f423; This 423 aa orf is 29 pct




AE000263






Escherichia coli






197




44









identical (1 gaps) to 172 residues of









an approx. 488 aa protein









YC24_CYAPA SW: P48260






ORF731




783572




782805




hypothetical chloroplast ORF16




U38804






Porphyra purpurea






597




52






ORF732




785032




783581




ABC transporter subunit




D64004




Synechocystis sp.




1720




62






ORF733




786412




785360




putative






ORF734




788429




786450




pbp




Y14206






Streptomyces coelicolor






148




55






ORF735




788944




788528




penicillin-binding protein 3




X84053






Pseudomonas aeruginosa






148




38






ORF736




789758




788901




putative






ORF737




790332




791504




major outer membrane protein




M64064






Chlamydia pneumoniae






2028




99






ORF738




791846




792721




ribosomal protein S2




U60196






Chlamydia trachomatis






904




70






ORF739




792724




793569




elongation factor Ts




U60196






Chlamydia trachomatis






1023




71






ORF740




793580




794323




UMP kinase




U60196






Chlamydia trachomatis






891




72






ORF741




794304




794843




ribosome-releasing factor




U60196






Chlamydia trachomatis






673




73






ORF742




795217




795732




unknown




D26185






Bacillus subtilis






105




42






ORF743




795722




796795




unknown




D26185






Bacillus subtilis






208




33






ORF744




798735




797053




putative




L33796






Vibrio cholerae






386




34






ORF745




799823




798681




putative






ORF746




799297




799578




putative






ORF747




801313




799808




Pkn5




U40656






Myxococcus xanthus






345




33






ORF748




802453




801332




putative






ORF749




803299




802457




putative






ORF750




803811




803290




putative






ORF751




805151




803826




YscN




U02499






Yersinia enterocolitica






1185




53






ORF752




805860




805156




putative






ORF753




806604




806332




putative






ORF754




806913




806608




putative






ORF755




808222




806903




putative






ORF756




808751




808146




putative






ORF757




809437




808673




putative






ORF758




809939




809454




putative






ORF759




811235




810213




delta-aminolevulinate synthase (EC




M30785






Escherichia coli






172




40









2.3.1.37)






ORF760




811779




813056




DNA gyrase subunit B




U35453






Clostridium acetobutylicum






584




38






ORF761




812890




812516




putative






ORF762




812954




813583




DNA gyrase subunit B




Z19108






Spiroplasma citri






371




39






ORF763




813587




815023




gyrA




X92503






Mycobacterium smegmatis






414




55






ORF764




815420




815746




putative






ORF765




816036




817010




orf-X; hypothetical protein; Method:




U48870






Bacillus subtilis






569




47









conceptual translation supplied by









author






ORF766




817111




817356




unknown




Z74024






Mycobacterium tuberculosis






114




34






ORF767




817791




818609




3-deoxy-d-manno-octulosonic acid




Z50747






Chlamydia psittaci






1112




78









8-phosphate synthetase






ORF768




818609




819094




protein of unknown function




Z50747






Chlamydia psittaci






545




65






ORF769




819104




819823




ATP binding protein




U72493






Chlamydia trachomatis






1099




88






ORF770




820722




819826




putative






ORF771




822313




821000




putative






ORF772




823503




822238




putative






ORF773




823678




825612




putative






ORF774




825461




826312




putative






ORF775




827280




826645




putative






ORF776




828604




827171




76 kDa protein




L23921






Chlamydia pneumoniae






2179




100






ORF777




830026




828713




76 kDa protein




L23921






Chlamydia pneumoniae






1162




100






ORF778




831047




830085




mviB homolog




U50732






Chlamydia trachomatis






982




58






ORF779




831725




831051




mviB homolog




U50732






Chlamydia trachomatis






740




65






ORF780




832220




833098




T05H10.2




Z47812






Caenorhabditis elegans






407




34






ORF781




833851




833396




ribosomal protein S4 (rps4)




AE000633






Helicobacter pylori






372




53






ORF782




834068




835039




This ORF is homologous to a 40.0 kd




L22217




Mycoplasma-like organism




377




49









hypothetical protein in the htrB 3′









region from


E. coli


, Accession









Number X61000






ORF783




835792




835127




uridine kinase




L31783






Mus musculus






436




43






ORF784




837624




836116




ORF_f397




U29581






Escherichia coli






92




38






ORF785




838951




840882




putative






ORF786




840869




842185




exodeoxyribonuclease V (recB)




U32811






Haemophilus influenzae






409




40






ORF787




841989




843455




DNA helicase II




U39703






Mycoplasma genitalium






110




46






ORF788




843242




844021




exodeoxyribonuclease V (recB)




U32811






Haemophilus influenzae






196




40






ORF789




845018




843987




MreC protein




M31792






Escherichia coli






76




53






ORF790




846174




844990




aspartate aminotransferase (aspC)




X03629






Escherichia coli






754




40






ORF791




848509




846311




GreA




U02878






Rickettsia prowazekii






190




35






ORF792




848568




849014




putative






ORF793




849082




850488




NADH: ubiquinone oxidoreducatase




U32702






Haemophilus influenzae






445




37









subunit A (GP: Z37111_2)






ORF794




851512




850574




porphobilinogen synthase




U38348






Chlorobium vibrioforme






769




45






ORF795




852064




852447




putative






ORF796




852398




853690




putative






ORF797




855118




854243




geranylgeranyl pyrophosphate




D85029






Arabidopsis thaliana






408




41









synthase






ORF798




855751




855128




f147; This 147 aa orf is 26 pct




AE000143






Escherichia coli






187




36









identical (1 gaps) to 99 residues of an









approx. 728 aa protein









E2BE_RABIT SW: P47823






ORF799




856551




855829




membrane associated regulatory




M28368






Salmonella typhimurium






172




36









protein






ORF800




856730




858556




unknown function




Z32530






Chlamydia trachomatis






842




35






ORF801




858717




859601




exodeoxyribonuclease V (recD)




U32811






Haemophilus influenzae






182




51






ORF802




859591




860205




exonuclease V alpha subunit (AA




X04582






Escherichia coli






235




45









1-608)






ORF803




861132




860284




putative






ORF804




861426




861163




30S ribosomal protein S20




Z67753






Odontella sinensis






153




41






ORF805




861701




862921




putative






ORF806




863026




864798




major sigma factor




U04442






Chlamydia psiitaci






2661




94






ORF807




864831




865256




putative






ORF808




865226




866581




dihydropterin pyrophosphokinase/




Y08611






Pisum sativum






455




48









dihydropteroate synthase






ORF809




866562




867119




dehydrofolate reductase, type I




U32772






Haemophilus influenzae






213




49









(folA)






ORF810




867025




867816






M. jannaschii


predicted coding




U67522






Methanococcus jannaschii






207




36









region MJ0768






ORF811




867820




868497




putative






ORF812




869743




868661




RecA




U16739






Chlamydia trachomatis






1512




87






ORF813




870633




870094




unknown function




Z32530






Chlamydia trachomatis






308




45






ORF814




871929




870646




unknown function




Z32530






Chlamydia trachomatis






1410




63






ORF815




872538




872086




putative






ORF816




873908




872517




putative






ORF817




874281




874670




nifR3-like gene product




Z37984






Azospirillum brasilense






181




32






ORF818




874582




875286




ORF1 gene product




X62399






Escherichia coli






307




42






ORF819




877857




875377




DNA topoisomerase I




L27797






Bacillis subtilis






1488




50






ORF820




878446




879255




putative






ORF821




880635




879268




sigma factor (ntrA) (AA 1-502)




X05888






Azotobacter vinelandii






257




47






ORF822




882524




880593




DNA helicase II




D90906




Synechocystis sp.




1140




50






ORF823




882612




883319




ipa-57d gene product




X73124






Bacillus subtilis






601




51






ORF824




884155




883538




hypothetical protein




D90915




Synechocystis sp.




344




39






ORF825




884340




885611




19/20 residue stretch (32-51)




L19954






Bacillus subtilis






456




37









identical to N-terminal putative









signal sequence of unknown, partly









cloned


B. subtilis


gene.; putative






ORF826




885722




887302




heat shock protein




L12004






Chlamydia trachomatis






915




39






ORF827




887587




888153




bas1 protein




Z34917






Hordeum vulgare






474




50






ORF828




888627




888220




putative






ORF829




889330




888716




hypothetical protein




Y14079






Bacillus subtilis






223




55






ORF830




889898




889323




peptidoglycan-associated lipoprotein




X65796






Escherichia coli






222




50






ORF831




891190




889898




TolB




U32470






Haemophilus influenzae






280




35






ORF832




891828




891247




putative






ORF833




892421




892017




exbD peptide




M28819






Escherichia coli






77




48






ORF834




893116




892421




inner membrane protein (tolQ)




U32722






Haemophilus influenzae






157




54






ORF835




892521




892925




putative






ORF836




893392




895419




inner membrane copper tolerance




Z36905






Escherichia coli






120




35









protein






ORF837




895745




896527




unknown




D26185






Bacillus subtilis






381




41






ORF838




896668




897558




succinate dehydrogenase subunit C




Y08563






Paenibacillus macerans






253




40






ORF839




897565




899442




succinate dehydrogenase subunit A




Y08563






Paenibacillus macerans






1667




57






ORF840




899420




900229




succinate dehydrogenase subunit B




Y08563






Paenibacillus macerans






656




54






ORF841




903230




900237




putative






ORF842




905081




903234




putative






ORF843




906931




905045




sigma factor SibG regulation protein




D90905




Synechocystis sp.




117




35









RsbU






ORF844




907248




907832




putative






ORF845




907784




908128




putative






ORF846




908132




908677




putative






ORF847




908589




909320




putative






ORF848




909405




911465




putative






ORF849




911677




912360




putative






ORF850




912303




912821




putative






ORF851




912937




913983




putative






ORF852




915128




914067




putative






ORF853




916658




915303




enolase




L29475






Bacillus subtilis






1036




60






ORF854




915627




915376




enolase




U43738






Mycoplasma pneumoniae






226




65






ORF855




917707




916853




excinuclease ABC subunit B (uvrB)




U32804






Haemophilus influenzae






724




46






ORF856




918837




917722




excinuclease ABC subunit B (uvrB)




U32804






Haemophilus influenzae






1029




54






ORF857




919868




918837




tryptophanyl-tRNA synthetase (trpS)




U32746






Haemophilus influenzae






376




40






ORF858




920434




919880




putative






ORF859




921187




920438




ORF8




X82078




Chlamydia sp.




164




50






ORF860




921959




921195




hypothetical protein




X62475






Chlamydia psittaci






511




44






ORF861




923773




921995




Threonyl tRNA Synthetase




Z80360






Bacillus subtilis






1476




44






ORF862




922146




922415




putative






ORF863




923943




923674




putative






ORF864




924077




925006




putative






ORF865




925436




925083




putative






ORF866




926524




925349




putative






ORF867




927920




926433




putative






ORF868




928319




927951




putative






ORF869




928963




928334




putative






ORF870




929248




930987




DNA mismatch repair protein




U32692






Haemophilus influenzae






585




40









(mutL)






ORF871




930995




932059




YqhT




D84432






Bacillus subtilis






445




39






ORF872




932121




933515




putative






ORF873




932881




932513




putative






ORF874




933485




935746




pulD (ttg start codon)




M32613






Klebsiella pneumoniae






210




33






ORF875




935724




937082




epsE




M96172






Vibrio cholerae






890




55






ORF876




937229




938410




PilG




U32588






Neisseria gonorrhoeae






280




38






ORF877




938281




938805




putative






ORF878




938809




939255




putative






ORF879




939165




939782




putative






ORF880




939760




940791




putative






ORF881




940822




941106




putative






ORF882




940977




941351




putative






ORF883




942537




941623




yscT




L25667






Yersinia pseudotuberculosis






169




44






ORF884




942784




942500




yscS




L25667






Yersinia pseudotuberculosis






173




42






ORF885




943149




942799




HrcR




AE000107




Rhizobium sp. NGR234




265




52






ORF886




943799




943029




pathogenicity protein




M64094






Xanthomonas campestris






252




41






ORF887




944055




943732




putative




M74011






Yersinia enterocolitica






112




33






ORF888




944413




943994




putative






ORF889




945395




944556




putative






ORF890




945853




945389




putative






ORF891




946392




945751




HrcJ




U56662






Erwinia amylovora






229




44






ORF892




947410




948081




putative






ORF893




949871




948915




ORF YOR196c




Z75104






Saccharomyces cerevisiae






702




44






ORF894




951058




949868




dihydrolipoamide dehydrogenase E3




M57435






Bacillus subtilis






745




39









subunit






ORF895




951249




950959




dihydrolipoamide acetyltransferase




M73535






Staphylococcus aureus






166




49









E3 subunit






ORF896




951664




952134




putative






ORF897




952674




952165




SNF




X98455






Bacillus aereus






229




47






ORF898




953491




952589




helicase




U39680






Mycoplasma genitalium






307




42






ORF899




955324




953495




F01G4.1




Z68341






Caenorhabditis elegans






133




57






ORF900




955823




955281




putative






ORF901




957082




955847




branched-chain amino acid carrier




Z48676




Lactobacillus delbrueckii




297




40






ORF902




957902




957270




endonuclease III




U11289






Bacillus subtilis






317




37






ORF903




959231




957906




homologous to


E. coli


50K




X62539






Bacillus subtilis






805




45






ORF904




959376




960284




phosphatidylserine decarboxylase




U72715






Chlamydia trachomatis






776




51






ORF905




960266




961669




putative






ORF906




961856




964765




secretory component




U06928






Caulobacter crescentus






1812




55






ORF907




966855




965395




28.2% of identity to the


Escherichia






L47648






Bacillus subtilis






778




41











coli


GTP-binding protein Era;









putative






ORF908




968204




966975




poly(A) polymerase




L47709






Bacillus subtilis






383




41






ORF909




968791




968237




ClpX-like protein




U18229






Bacillus subtilis






340




39






ORF910




969498




968731




ATP-dependent protease ATPase




D64006




Synechocystis sp.




846




66









subunit






ORF911




969858




969511




ClpP




U16135




Synechococcus sp.




257




54






ORF912




970118




969762




ATP-dependent clp protease




AE000591






Helicobacter pylori






362




63









proteolytic component (clpP)






ORF913




970593




970300




putative






ORF914




971261




970542




putative






ORF915




971680




971123




putative






ORF916




971876




975100




SNF




X98455






Bacillus cereus






778




49






ORF917




975419




976516




MreB protein




M96343






Bacillus subtilis






960




55






ORF918




976584




978320




phospho enol pyruvate




S56812






Chlorobium limicola






1667




64









carboxykinase






ORF919




977680




977231




putative






ORF920




978399




980738




putative






ORF921




980756




981928




putative






ORF922




982974




981931




precursor protein (AA-22 to 371)




X52557






Chlamydia trachomatis






97




50






ORF923




984120




983119




NAD+ dependent




L47648






Bacillus subtilis






618




43









glycerol-3-phosphate dehydrogenase






ORF924




985502




984120




AgX-1 antigen [human, infertile




S73498






Homo sapiens






254




34









patient, testis, Peptide, 505 aa]






ORF925




987180




985882




ORF4




M72718






Bacillus subtilis






697




38






ORF926




987172




987444




putative






ORF927




989846




989049




nifU-like protein




AE000542






Helicobacter pylori






302




31






ORF928




991048




989846




putative






ORF929




991638




990955




phosphoglyceromutase




L09651






Zymomonas mobilis






471




53






ORF930




991794




992498




ORFX13




L09228






Bacillus subtilis






403




39






ORF931




993619




993041




biotin [acetyl-COA-carboxylase]




L47709






Bacillus subtilis






136




38









ligase






ORF932




993530




994792




rod-shape-determining protein




M22857






Escherichia coli






312




44






ORF933




995970




994795




cadmium-transporting ATPase




D64005




Synechocystis sp.




358




47






ORF934




996857




995739




ATPase




L28104




Transposon Tn5422




449




39






ORF935




997603




996782




putative






ORF936




998969




997572




seryl-trna synthetase




Y09924






Staphylococcus aureus






851




42






ORF937




998896




1000023




orf2, homologue to


B. subtilis


ribG




X64395






Escherichia coli






596




40






ORF938




1000087




1001340




GTP cyclohydrolase II




D90912




Synechocystis sp.




1078




52






ORF939




1001357




1001818




riboflavin synthase beta subunit




U27202






Actinobacillus






278




36













pleuropneumoniae








ORF940




1003288




1001873




putative






ORF941




1003487




1004146




putative






ORF942




1004485




1005639




D-alanine glycine permease (dagA)




AE000603






Helicobacter pylori






394




33






ORF943




1005643




1005972




hypothetical protein MTCY180.08




Z97193






Mycobacterium tuberculosis






274




58






ORF944




1006784




1006116




similar to trithorax protein in final




U13875






Caenorhabditis elegans






155




46









three exons






ORF945




1007563




1006769




yycJ




D78193






Bacillus subtilis






406




38






ORF946




1009226




1007568




YtpT




AF008220






Bacillus subtilis






992




47






ORF947




1009989




1009336




putative






ORF948




1015852




1016337




putative






ORF949




1016561




1016181




putative






ORF950




1016297




1017532




putative






ORF951




1016802




1016452




putative






ORF952




1018993




1017701




phenolhydroxylase component




U32702






Haemophilus influenzae






909




47






ORF953




1019454




1019137




ORF




M63939






Escherichia coli






96




45






ORF954




1020764




1019562




pCTHom1 gene product




M94254






Chlamydia trachomatis






1185




65






ORF955




1021405




1021037




histone H1-like protein




M80324






Chlamydia psittaci






319




62






ORF956




1021821




1024286




phosphoprotein




L25078






Chlamydia trachomatis






739




41






ORF957




1024697




1024248




putative






ORF958




1025569




1024508




protoporphyrinogen oxidase




U25114






Mus musculus






86




38






ORF959




1026969




1025590




oxygen independent




D90912




Synechocystis sp.




880




42









coprophorphyrinogen III oxidase






ORF960




1027789




1026947




uroporphyrinogen decarboxylase




M97208






Bacillus subtilis






372




38






ORF961




1031199




1027945




transcription-repair coupling factor




U32805






Haemophilus influenzae






1584




42









(trcF) (mfd)






ORF962




1031717




1031172




alanyl-tRNA synthetase




X95571






Thiobacillus ferrooxidans






76




31






ORF963




1033057




1031612




alanyl-tRNA synthetase




AE000353






Escherichia coli






889




40






ORF964




1033425




1033039




alanyl-tRNA synthetase (alaS)




AE000629






Helicobacter pylori






327




51






ORF965




1033784




1033200




alanyl-tRNA synthetase




X59956






Rhizobium leguminosarum






416




47






ORF966




1033963




1036038




transketolase




Z73234






Bacillus subtilis






1398




44






ORF967




1036945




1036010




AMP nucleosidase




AE000290






Escherichia coli






265




42






ORF968




1037110




1037679




elongation factor P




U140003






Escherichia coli






458




51






ORF969




1037696




1037944




putative






ORF970




1038916




1037975




putative






ORF971




1040582




1039026




HSP60 chaperonin




X62914






Clostridium perfringens






284




31






ORF972




1040997




1042337




PROBABLE




AB001488






Bacillus subtilis






446




39









UDP-N-ACETYLMURAMOYLAL









ANYL-D-GLUTAMYL-2,









6-DIAMINOLIGASE (EC 6.3.2.15).






ORF973




1042357




1043403




ORF-Y (AA 1-360)




X51584






Escherichia coli






582




45






ORF974




1043367




1044623




UDP-N-acetylmuramoylalanine-D-gl




U32793






Haemophilus influenzae






348




42









utamate ligase (murD)






ORF975




1044607




1045362




hypothetical protein




Y14079






Bacillus subtilis






115




38






ORF976




1045384




1046538




spoVE gene product (AA 1-366)




X51419






Bacillus subtilis






479




35






ORF977




1046447




1047517




mur




Y13922






Enterococcus hirae






256




45






ORF978




1047521




1049956




UDP-N-acetylmuramate-alanine




U32794






Haemophilus influenzae






756




38









ligase (murC)






ORF979




1050611




1050036




unknown




Z74024






Mycobacterium tuberculosis






78




44






ORF980




1050925




1050566




cycY gene product




U14003






Escherichia coli






179




34






ORF981




1051728




1051090




putative






ORF982




1051743




1052063




hypothetical protein




D90908




Synechocystis sp.




135




33






ORF983




1052101




1053126




trna




Z98209






Mycobacterium tuberculosis






441




37









delta(2)-isopentenylpyrophosphate









transferase






ORF984




1054201




1053107




conserved hypothetical protein




AE000579






Helicobacter pylori






826




44






ORF985




1054242




1055555




putative






ORF986




1055483




1055908




putative






ORF987




1056609




1056965




YqeL




D84432






Bacillus subtilis






202




38






ORF988




1056961




1058232




beta-ketoacyl-ACP synthase




L13242






Ricinus communis






1266




55






ORF989




1058238




1058687




diadenosine tetraphosphatase




U30313






Homo sapiens






122




42






ORF990




1059371




1058727




inorganic pyrophosphatase (ppa)




AE000576






Helicobacter pylori






209




39






ORF991




1059526




1060578




leucine dehydrogenase LeuDH




U51099






Bacillus cereus






680




45






ORF992




1061553




1060579




3′(2′),5′-bisphosphate nucleotidase




U40433






Arabidopsis thaliana






335




43






ORF993




1061674




1062411




putative






ORF994




1062377




1064077




2-acylglycerophosphoethanolamine




U29581






Escherichia coli






383




44









acyl transferase/acyl carrier protein









synthetase






ORF995




1064116




1065243




7-keto-8-aminopelargonic acid




M29291






Bacillus sphaericus






200




35









synthetase (bioF)






ORF996




1067451




1065178




priA




Y10304






Bacillus subtilis






1009




43






ORF997




1068065




1067376




putative






ORF998




1068209




1068706




putative






ORF999




1069958




1068819




unknown




U41759






Chlamydia psittaci






777




41






ORF1000




1071163




1070033




unknown




U41759






Chlamydia psittaci






381




36






ORF1001




1072438




1071332




unknown




U41759






Chlamydia psittaci






254




37






ORF1002




1072997




1073476




putative






ORF1003




1074239




1075864




lysyl-tRNA synthetase




D90906




Synechocystis sp.




1007




48






ORF1004




1076790




1075867




cysteinyl-tRNA synthetase




L14580






Bacillus subtilis






395




52






ORF1005




1077268




1076573




cys-tRNA synthetase (cysS)




U32693






Haemophilus influenzae






431




56






ORF1006




1077999




1078724




putative






ORF1007




1079088




1078672




ribonuclease P protein component




M11056






Escherichia coli






78




46









(gtg start codon)






ORF1008




1079642




1079944




30S ribosomal subunit protein S14




U18997






Escherichia coli






260




50






ORF1009




1080501




1079995




F18C12.2




Z75536






Caenorhabditis elegans






118




38






ORF1010




1080775




1081341




putative






ORF1011




1083158




1081350




deoxyribodipyrimidine photolyase




J03294






Bacillus subtilis






687




44






ORF1012




1084677




1083235




DNA mismatch repair protein




U71154






Aquifex pyrophilus






735




48






ORF1013




1085648




1084632




DNA mismatch repair protein




D90909




Synechocystis sp.




565




39






ORF1014




1086117




1086737




DNA primase (dnaG)




U32735






Haemophilus influenzae






303




40






ORF1015




1086692




1087897




DnaG




Z83860






Mycobacterium tuberculosis






222




37






ORF1016




1088646




1089005




putative






ORF1017




1089146




1089805




putative






ORF1018




1092931




1089890




glycyl-tRNA synthetase




U20547






Chlamydia trachomatis






2569




48






ORF1019




1093179




1092889




putative






ORF1020




1093584




1094204




phosphatidylglycerophosphate




U87792






Bacillus subtilis






163




55









synthase






ORF1021




1095619




1094192




glycogen (starch) synthase




D90899




Synechocystis sp.




574




40






ORF1022




1096074




1096628




partial ctc gene product (AA 1-186)




X16518






Bacillus subtilis






86




37






ORF1023




1096633




1097082




peptidyl-tRNA hydrolase




U31570






Chlamydia trachomatis






378




53






ORF1024




1097266




1097601




ribosomal protein S6 (rps6)




AE000630






Helicobacter pylori






179




39






ORF1025




1097622




1097867




ribosomal protein S18 homolog;




M62820






Chlamydia trachomatis






324




86









putative






ORF1026




1097886




1098392




putative heat shock protein ORF;




M62820






Chlamydia trachomatis






190




79









putative






ORF1027




1699521




1099279




putative






ORF1028




1099689




1101053




putative






ORF1029




1102192




1101107




putative






ORF1030




1104950




1102116




glycerol-3-phosphate acyltransferase




M80571






Cucumis sativus






574




43






ORF1031




1106508




1104946




ORF_f495; orfF of ECMRED, uses




U18997






Escherichia coli






855




38









2nd start






ORF1032




1106722




1107249




putative






ORF1033




1107463




1108101




PlsX




U59433






Bacillus subtilis






282




45






ORF1034




1108041




1108421




fatty acid/phospholipid synthesis




AE000540






Helicobacter pylori






205




35









protein (plsX)






ORF1035




1108520




1113370




putative 98 kDa outer membrane




U72499






Chlamydia psittaci






352




44









protein






ORF1036




1114958




1113447




putative






ORF1037




1116915




1115071




lipid A disaccharide synthetase




U32786






Haemophilus influenzae






477




42









(lpxB)






ORF1038




1118183




1116894




poly(A) polymerase




AE000123






Escherichia coli






555




46






ORF1039




1118846




1120030




putative




L12968






Escherichia coli






880




50






ORF1040




1120040




1120522




glucosamine fructose-6-phosphate




AE000651






Helicobacter pylori






396




52









aminotransferase (isomerizing)









(glmS)






ORF1041




1120510




1121430




glutamine amidotransferase;




AE000450






Escherichia coli






494




44









glucosamine-fructose-6-phosphate









aminotransferase






ORF1042




1121321




1121866




L-glutamine: D-fructose-6-P




U17352






Thermus aquaticus






374




50









amidotransferase precursor







thermophilus








ORF1043




1122123




1122899




tyrosine-specific transport protein




AE000284






Escherichia coli






281




41






ORF1044




1124842




1125564




putative






ORF1045




1126526




1125579




cell division protein (ftsY)




U32760






Haemophilus influenzae






497




41






ORF1046




1126519




1127676




succinyl-CoA synthetase




J01619






Escherichia coli






784




43









beta-subunit






ORF1047




1127672




1128571




succinyl coenzyme A synthetase




U23408






Dictyostelium discoideum






978




63









alpha subunit






ORF1048




1130230




1131336




putative






ORF1049




1131480




1132553




putative






ORF1050




1132830




1133843




putative






ORF1051




1134121




1134855




serine protease HtrA




D90905




Synechocystis sp.




307




51






ORF1052




1134642




1135592




GsrA protein




D78376






Yersinia enterocolitica






497




41






ORF1053




1135964




1135653




putative






ORF1054




1137132




1135954




R11H6.1




Z93386






Caenorhabditis elegans






445




37






ORF1055




1137169




1140102




Ydr430cp; CAI: 0.15




U33007






Saccharomyces cerevisiae






559




40






ORF1056




1141365




1140112




hypothetical 54.7 kD protein in udp




AE000459






Escherichia coli






222




34









3′ region precursor (o475)






ORF1057




1142150




1141356




phosphatidylserine synthase (pssA)




AE000614






Helicobacter pylori






307




41






ORF1058




1142520




1145660




ribonucleotide reductase subunit M1




K02927






Mus musculus






1433




45






ORF1059




1145627




1146721




ribonucleoside diphosphate




AE000553






Helicobacter pylori






443




32









reductase, beta subunit (nrdB)






ORF1060




1146862




1147545




unknown




Z95398






Mycobacterium leprae






191




35






ORF1061




1147666




1148190




YtqB




AF008220






Bacillus subtilis






262




44






ORF1062




1148514




1148224




ORF2




U01958






Bacillus licheniformis






135




54






ORF1063




1149136




1148348




ORF2




M31827






Bacillus subtilis






268




40






ORF1064




1149702




1149166




putative






ORF1065




1150031




1150591




unknown




Z85982






Mycobacterium tuberculosis






445




49






ORF1066




1150785




1151147




ribosomal protein L20 (AA 1-119)




X16188






Bacillus stearothermophilus






273




44






ORF1067




1151165




1152181




phenylalany-tRNA synthetase beta




Z75208






Bacillus subtilis






777




40









subunit






ORF1068




1152522




1154591




putative






ORF1069




1155666




1154566




putative






ORF1070




1156743




1155670




putative






ORF1071




1156859




1157815




hypothetical




U32723






Haemophilus influenzae






252




42






ORF1072




1157982




1160735




ATP-binding protein




U01376






Escherichia coli






1314




56






ORF1073




1162620




1160917




polynucleotide phosphorylase




AF010578






Pisum sativum






1416




52






ORF1074




1162970




1162590




polyribonucleotide phophorylase




U52048






Spinacia oleracea






312




53






ORF1075




1163532




1164020




orf150 gene product




X95938






Porphyromonas gingivalis






335




43






ORF1076




1163995




1164294




putative






ORF1077




1165569




1165030




putative






ORF1078




1166108




1165566




putative






ORF1079




1166644




1166141




putative






ORF1080




1167055




1168374




putative






ORF1081




1169218




1168337




methionine aminopeptidase




D64003




Synechocystis sp.




488




54






ORF1082




1169823




1169218




ORF_o197




U18997






Escherichia coli






281




30






ORF1083




1171324




1170572




putative






ORF1084




1172085




1171177




hypothetical




U32720






Haemophilus influenzae






162




44






ORF1085




1172394




1173773




fumarase




D64000




Synechocystis sp.




1292




57






ORF1086




1175209




1173881




prs-associated putative membrane




U02424






Escherichia coli






570




39









protein






ORF1087




1175555




1175127




hypothetical protein in pth-prs




AE000219






Escherichia coli






278




46









intergenic region






ORF1088




1175778




1177043




hypothetical protein




Z96072






Mycobacterium tuberculosis






109




43






ORF1089




1177177




1179048




putative






ORF1090




1179156




1180085




penicillin tolerance protein (lytB)




U32781






Haemophilus influenzae






731




54






ORF1091




1180045




1180779




putative






ORF1092




1181942




1180788




putative






ORF1093




1182296




1181961




putative






ORF1094




1183844




1182300




putative






ORF1095




1184420




1183848




putative






ORF1096




1185382




1184366




putative






ORF1097




1185858




1185226




putative






ORF1098




1186164




1186481




putative






ORF1099




1187386




1186484




site-specific recombinase




U92524






Salmonella typhimurium






401




48






ORF1100




1187370




1189028




phophoglucoisomerase-like protein




L40822






Chlamydia trachomatis






1154




63






ORF1101




1189321




1190889




putative






ORF1102




1191142




1192146




NADP-malate dehydrogenase




L40958






Flaveria bidentis






775




46






ORF1103




1191974




1191729




putative






ORF1104




1193815




1192991




putative






ORF1105




1195702




1194248




o460; This 460 aa orf is 46 pct




AE000256






Escherichia coli






1022




44









identical (26 gaps) to 458 residues of









an approx. 488 aa protein









ARCD_PSEAE SW: P18275






ORF1106




1196303




1195716




putative






ORF1107




1196831




1196337




putative






ORF1108




1197807




1196746




putative






ORF1109




1198740




1197883




putative






ORF1110




1200232




1198721




shikimate 5-dehydrogenase




U67551






Methanococcus jannaschii






245




37






ORF1111




1201286




1200135




3-dehydroquinate synthase (aroB)




U32705






Haemophilus influenzae






478




45






ORF1112




1202386




1201259




2,3-dihydroxybenzoic acid




L29562






Vibrio anguillarum






780




50






ORF1113




1202901




1202350




putative






ORF1114




1204162




1202816




5-enolpyruvylshikimate 3-phosphate




U67500






Methanococcus jannaschii






520




40









synthase






ORF1115




1203177




1203464




putative






ORF1116




1205028




1204180




putative






ORF1117




1206392




1204878




bioA gene product




A02587




unidentified




834




48






ORF1118




1206742




1206086




dethiobiotin synthase (bioD)




U32830






Haemophilus influenzae






243




37






ORF1119




1207872




1206724




L-alanine-pimelyl CoA ligase




U51868






Bacillus subtilis






601




41






ORF1120




1208852




1207851




biotin sythase




U24147






Arabidopsis thaliana






892




52






ORF1121




1210518




1209742




tryptophan hydroxylase




U26428






Gallus gallus






237




34






ORF1122




1210703




1211494




dihydrodipicolinate reductase




U47017






Pseudomonas syringae pv.






345




37













tabaci








ORF1123




1211870




1212754




aspartate-semialdehyde




U67476






Methanococcus jannaschii






444




43









dehydrogenase






ORF1124




1212742




1214064




aspartokinase III




U00006






Escherichia coli






473




47






ORF1125




1214046




1214858




dihydrodipicolinate synthase




D64006




Synechocystis sp.




238




40






ORF1126




1215551




1216318




putative






ORF1127




1216493




1216849




putative






ORF1128




1217183




1219612




putative






ORF1129




1220068




1219673




putative






ORF1130




1219710




1220669




putative






ORF1131




1220630




1221376




putative






ORF1132




1221645




1223681




unknown




D26185






Bacillus subtilis






621




43






ORF1133




1223894




1224988




putative






ORF1134




1225000




1225830




high level kasgamycin resistance




D26185






Bacillus subtilis






422




41






ORF1135




1227810




1225879




hypothetical protein




D90903




Synechocystis sp.




1129




43






ORF1136




1226528




1226908




putative






ORF1137




1229972




1228311




exonuclease VII, large subunit




U32723






Haemophilus influenzae






666




46









(xseA)






ORF1138




47569




47018




Integrase/recombinase




AE001308






Chlamydia trachomatis






716




72






ORF1139




49980




49117




putative






ORF1140




53356




52898




putative






ORF1141




54477




54884




O-Sialoglycoprotein Endopeptidase




AE001307






Chlamydia trachomatis






311




51






ORF1142




63753




63998




PTS PEP Phosphotransferase




AE001306






Chlamydia trachomatis






198




61






ORF1143




77164




77487




putative






ORF1144




79724




79302




Sms Protein




AE001302






Chlamydia trachomatis






458




57






ORF1145




88721




88951




putative






ORF1146




94067




94429




putative






ORF1147




122832




123341




hypothetical protein




AE001303






Chlamydia trachomatis






398




61






ORF1148




147536




147234




putative






ORF1149




158990




159346




S16 Ribosomal Protein




AE001277






Chlamydia trachomatis






467




78






ORF1150




168470




168979




putative






ORF1151




169183




169452




putative






ORF1152




171785




171504




Cationic Amino Acid Transporter




AE001278






Chlamydia trachomatis






262




68






ORF1153




172518




171775




Cationic Amino Acid Transporter




AE001278






Chlamydia trachomatis






533




48






ORF1154




193599




194045




putative






ORF1155




195704




196075




S/T Protein Kinase




AE001288






Chlamydia trachomatis






536




82






ORF1156




210687




210145




KDO-transferase




X80061






Chlamydia pneumoniae






856




96






ORF1157




211100




210708




putative






ORF1158




215420




215088




putative






ORF1159




217914




218246




putative






ORF1160




218925




218701




putative






ORF1161




223785




223525




IMP dehydrogenase




U13372






Borrelia burgdorferi






270




63






ORF1162




224271




223999




putative






ORF1163




228691




228407




putative






ORF1164




235050




235334




(Methylase)




AE001287






Chlamydia trachomatis






331




66






ORF1165




252308




253021




Oligopeptide Permease




AE001293






Chlamydia trachomatis






838




72






ORF1166




258280




258912




Dicarboxylate Translocator




AE001294






Chlamydia trachomatis






909




80






ORF1167




261325




261567




putative






ORF1168




268195




268878




hypothetical protein




AE001287






Chlamydia trachomatis






556




52






ORF1169




269447




268881




putative






ORF1170




271263




271538




putative






ORF1171




271957




272346




putative






ORF1172




274176




274550




putative






ORF1173




275736




275314




Disulfide bond Oxidoreductase




AE001291






Chlamydia trachomatis






519




73






ORF1174




276490




276927




hypothetical protein




AE001291






Chlamydia trachomatis






249




53






ORF1175




277577




277861




hypothetical protein




AE001291






Chlamydia trachomatis






256




52






ORF1176




288163




287909




putative






ORF1177




290130




289789




putative






ORF1178




290989




291225




putative






ORF1179




291372




291860




adenylate cyclase




AE001286






Chlamydia trachomatis






388




48






ORF1180




311239




311622




putative






ORF1181




328665




328384




putative






ORF1182




337348




338289




sodium-dependent transporter




AF017105






Chlamydia psittaci






1112




72






ORF1183




364764




364369




Prolipoprotein Diacylglycerol




AE001298






Chlamydia trachomatis






300




54









Transferase






ORF1184




389623




390135




hypothetical protein




AE001282






Chlamydia trachomatis






75




33






ORF1185




393729




394343




ABC superfamily ATPase




AE001282






Chlamydia trachomatis






473




52






ORF1186




407379




407621




putative






ORF1187




410944




410708




putative






ORF1188




427632




427988




putative






ORF1189




428172




428486




putative






ORF1190




436761




437246




hypothetical protein




AE001279






Chlamydia trachomatis






661




81






ORF1191




460911




461159




putative






ORF1192




477597




477313




hypothetical protein




AE001300






Chlamydia trachomatis






309




62






ORF1193




487303




487001




putative






ORF1194




487764




487534




Glycine Cleavage System H Protein




AE001300






Chlamydia trachomatis






221




67






ORF1195




498502




499017




hypothetical protein




AE001275






Chlamydia trachomatis






206




32






ORF1196




499795




500466




putative






ORF1197




571928




572344




putative






ORF1198




572367




572131




putative






ORF1199




588184




587915




hypothetical protein




AE001312






Chlamydia trachomatis






256




62






ORF1200




600587




600907




(Metalloenzyme)




AE001316






Chlamydia trachomatis






314




61






ORF1201




609731




608895




putative






ORF1202




614039




614755




hypothetical protein




AE001317






Chlamydia trachomatis






475




46






ORF1203




614823




615152




putative






ORF1204




638244




638831




ABC Transporter ATPase




AE001315






Chlamydia trachomatis






614




61






ORF1205




638819




639094




(Metal Transport Protein)




AE001315






Chlamydia trachomatis






265




63






ORF1206




639073




639636




(Metal Transport Protein)




AE001315






Chlamydia trachomatis






687




69






ORF1207




647901




648236




hypothetical protein




AE001317






Chlamydia trachomatis






139




38






ORF1208




678510




679469




phosphohydrolase




AE001320






Chlamydia trachomatis






995




63






ORF1209




688178




688732




hypothetical protein




AE001320






Chlamydia trachomatis






366




43






ORF1210




696045




696563




methyltransferase




AE001321






Chlamydia trachomatis






369




49






ORF1211




708998




708588




Glucose-1-P Adenyltransferase




AE001322






Chlamydia trachomatis






507




83






ORF1212




709808




710089




putative






ORF1213




718240




717737




Glycerol-3-P Phosphatidyltransferase




AE001323






Chlamydia trachomatis






573




66






ORF1214




737828




737565




S19 Ribosomal Protein




AE001323






Chlamydia trachomatis






439




94






ORF1215




779502




780257




hypothetical protein




AE001322






Chlamydia trachomatis






476




48






ORF1216




806310




805864




hypothetical protein




AE001337






Chlamydia trachomatis






512




67






ORF1217




820931




820707




putative






ORF1218




837696




839096




Exodeoxyribonuclease V, Gamma




AE001334






Chlamydia trachomatis






967




49






ORF1219




883307




883549




putative






ORF1220




892010




891726




putative






ORF1221




893277




893564




putative






ORF1222




936998




937225




Gen. Secretion Protein E




AE001327






Chlamydia trachomatis






256




67






ORF1223




946865




947419




putative






ORF1224




975187




975411




SWF/SNF family helicase




AE001341






Chlamydia trachomatis






363




96






ORF1225




985882




985517




hypothetical protein




AE001342






Chlamydia trachomatis






166




33






ORF1226




987713




987180




hypothetical protein




AE001342






Chlamydia trachomatis






447




59






ORF1227




988215




987733




Flagellar M-Ring Protein




AE001342






Chlamydia trachomatis






304




44






ORF1228




988754




988530




Flagellar M-Ring Protein




AE001342






Chlamydia trachomatis






92




36






ORF1229




992542




992841




hypothetical protein




AE001343






Chlamydia trachomatis






112




39






ORF1230




992759




993067




hypothetical protein




AE001343






Chlamydia trachomatis






100




32






ORF1231




1004247




1004528




D-Ala/Gly Permease




AE001344






Chlamydia trachomalis






283




64






ORF1232




1015013




1014294




235aa long hypothetical protein




AB009472






Pyrococcus horikoshii






104




54






ORF1233




1056147




1056545




putative






ORF1234




1077682




1078035




predicted disulfide bond isomerase




AE001351






Chlamydia trachomatis






233




46






ORF1235




1088121




1088381




putative






ORF1236




1098430




1098852




Predicted Kinase




AE001352






Chlamydia trachomatis






384




59






ORF1237




1098798




1099319




Predicted Kinase




AE001352






Chlamydia trachomatis






322




45






ORF1238




1123198




1123515




Transport Permease




AE001354






Chlamydia trachomatis






313




72






ORF1239




1123606




1124256




Tyrosine Transport




AE001354






Chlamydia trachomatis






577




58






ORF1240




1124453




1124797




Tyrosine Transport




AE001354






Chlamydia trachomalis






323




50






ORF1241




1129253




1129567




putative






ORF1242




1164947




1164474




hypothetical protein




AE001357






Chlamydia trachomatis






412




56






ORF1243




1170457




1170053




hypothetical protein




AE001358






Chlamydia trachomatis






283




59






ORF1244




1172342




1171863




ABC transporter permease




AE001358






Chlamydia trachomatis






457




55






ORF1245




1192155




1192835




putative






ORF1246




1192759




1192992




putative






ORF1247




1193861




1194142




putative






ORF1248




1194036




1193779




(D-Amino Acid Dehydrogenase)




AE001311






Chlamydia trachomatis






269




79






ORF1249




1209748




1209053




conserved hypothetical protein




AE000958






Archaeoglobus fulgidus






121




38






ORF1250




1215111




1215419




putative






ORF1251




1216302




1216538




putative






ORF1252




1228072




1227818




hypothetical protein




AE001306






Chlamydia trachomatis






134




39






ORF1253




1228304




1228080




xseB




AL021897






Mycobacterium tuberculosis






89




33






ORF1254




26599




26222




putative






ORF1255




27609




27367




putative






ORF1256




67206




66967




putative






ORF1257




70612




70352




putative






ORF1258




132703




132945




putative






ORF1259




178073




178393




putative






ORF1260




208576




208349




putative






ORF1261




209156




208929




putative






ORF1262




209263




209024




putative






ORF1263




210304




210639




putative






ORF1264




299009




299452




putative






ORF1265




352106




351717




putative






ORF1266




420182




419949




Flagellar Secretion Protein




AE001280






Chlamydia trachomatis






115




43






ORF1267




553602




553381




putative






ORF1268




556538




556807




putative






ORF1269




594348




593797




putative






ORF1270




595169




594876




putative






ORF1271




662148




662381




putative






ORF1272




706528




706893




putative






ORF1273




803315




803650




putative






ORF1274




849551




849306




putative






ORF1275




913676




913275




putative






ORF1276




927087




926836




putative






ORF1277




930587




930360




putative






ORF1278




986531




986764




ORF12




M72718






Bacillus subtilis






106




48






ORF1279




996229




996486




putative






ORF1280




1000373




1000002




putative






ORF1281




1010291




1010037




putative






ORF1282




1011128




1010793




106 aa long hypothetical protein




AB009472






Pyrococcus horikoshii






159




50






ORF1283




1012924




1012694




putative






ORF1284




1028659




1028913




putative






ORF1285




1086481




1086762




putative






ORF1286




1118658




1118879




Phosphoglucomutase




AE001354






Chlamydia trachomatis






291




84






ORF1287




1170098




1169835




hypothetical protein




AE001358






Chlamydia trachomatis






187




53






ORF1288




1180828




1181184




putative






ORF1289




1182658




1183035




putative






ORF1290




1195076




1194795




putative






ORF1291




1195890




1196183




putative



























TABLE 2











ORF Nos




begin




end




potential start





























2




42




794




42







3




1258




1614




1261







4




1807




2418




1807







5




3393




2491




3393







6




3639




4067




3639







7




5649




4270




5649







8




7463




6012




7463







9




8051




8962




8051







10




9129




9959




9138







11




10687




10361




10639







12




10927




11232




10927







13




11246




12727




11246







14




12691




14190




12691







15




14484




17249




14484







16




16039




15770




16036







17




17845




20853




17845







18




21137




22042




21137







19




22046




23476




22046







20




23681




26110




23681







21




26109




25861




26109







22




26241




26978




26241







23




26960




27754




26960







24




27747




28577




27747







25




28887




29492




28950







26




29432




30028




29432







27




30024




31472




30024







28




31758




32288




31758







29




32201




33991




32201







30




33852




34541




33852







31




34783




36063




34783







32




36009




37529




36009







33




37881




39362




37881







34




39418




39161




39418







35




39366




40715




39366







36




43076




41094




43076







37




43800




43066




43800







38




44828




43785




44768







39




45340




44753




45340







40




45752




45372




45752







41




46996




45701




46996







42




47961




47569




47961







43




48960




48040




48960







44




51452




50133




51452







45




52606




51335




52606







46




53684




53319




53684







47




54195




53746




54195







48




55278




56453




55278







49




56493




57266




56493







50




57297




58526




57297







51




59851




58565




59851







52




61495




59924




61495







53




61324




62151




61324







54




62132




62470




62132







55




62474




63733




62474







56




63881




64186




63881







57




64611




64318




64611







58




65485




64673




65485







59




65999




65301




65999







60




66244




67281




66244







61




67265




67699




67265







62




67703




68539




67760







63




68805




70736




68805







64




69172




68831




69172







65




70642




71142




70642







66




71325




72029




71325







67




72060




73637




72060







68




74061




76175




74061







69




78351




77680




78351







70




79356




78355




79356







71




79983




79693




79983







72




80441




79938




80441







73




80475




80969




80475







74




81296




83080




81332







75




83291




83932




83291







76




84005




84769




84005







77




84975




85244




84975







78




85123




85425




85123







79




85397




85903




85397







80




85909




86583




85909







81




86626




88065




86626







82




89257




91026




89257







83




91291




93030




91291







84




93295




94086




93295







85




95285




94707




95279







86




95667




96557




95667







87




96317




97456




96317







88




98435




97968




98435







89




99460




98426




99460







90




100144




101325




100144







91




101457




101720




101457







92




101704




102273




101704







93




102356




102805




i02356







94




102835




103530




102835







95




103549




104058




103549







96




104096




104491




104096







97




104601




108386




104601







98




108401




112054




108401







99




112033




112590




112033







100




112672




113682




112672







101




113726




114121




113726







102




114711




114136




114711







103




115267




115755




115267







104




115911




116543




115911







105




116736




118055




116778







106




117968




118522




117968







107




118530




119843




118530







108




119816




120457




119816







109




120451




122430




120451







110




122504




122950




122504







111




123528




126347




123528







112




126332




129166




126332







113




134690




129213




134690







114




134925




136382




134931







115




137870




136482




137867







116




137899




138240




137899







117




138239




137928




138239







118




139558




138257




139558







119




140352




139516




140352







120




140498




141841




140498







121




141855




142658




141855







122




144258




143050




144258







123




145258




144494




145258







124




145454




146749




145454







125




147318




146767




147318







126




148261




147677




148261







127




149029




152157




149029







128




154108




152201




154108







129




155135




154308




155135







130




155141




155467




155141







131




155703




156779




155703







132




156748




157635




156748







133




157653




158996




157653







134




159363




159986




159363







135




159880




160446




159880







136




160477




160839




160477







137




160898




161539




160898







138




161527




162153




161527







139




162144




162443




162144







140




162437




164098




162437







141




165451




164228




165451







142




166349




165411




166349







143




166949




168442




166949







144




169416




171029




169416







145




170857




171459




170857







146




172652




173428




172652







147




174626




173439




174626







148




174816




175613




174816







149




175598




175954




175598







150




175958




176935




175958







151




177708




176938




177708







152




177128




177376




177128







153




179472




177841




179472







154




179822




179517




179822







155




181793




179943




181793







156




182628




181876




182628







157




184420




183074




184420







158




184988




184467




184988







159




185483




185112




185483







160




185902




185483




185902







161




186174




185839




186174







162




187720




186587




187720







163




188318




190933




188318







164




191090




191635




191090







165




191547




192743




191547







166




192969




193469




192969







167




194044




193610




194044







168




194196




195809




194196







169




196088




198073




196088







170




198132




199454




198132







171




199351




202818




199351







172




204552




202999




204552







173




205648




204692




205639







174




205807




207327




205807







175




207182




207775




207182







176




207779




208267




207779







177




208267




209577




208267







178




211807




211271




211807







179




212188




211844




212188







180




214079




212448




214079







181




214907




214083




214907







182




216154




215429




216154







183




216115




216678




216115







184




216728




217282




216728







185




217267




217866




217267







186




218593




218261




218590







187




219821




218994




219821







188




221382




220309




221382







189




222719




221433




222719







190




223521




222724




223521







191




224499




225008




224499







192




225140




225559




225140







193




225555




226802




225555







194




227800




226892




227743







195




228335




228072




228335







196




229251




228643




229251







197




230983




229622




230983







198




231483




230983




231483







199




232063




231509




232063







200




232739




232053




232739







201




233166




234356




233166







202




233518




233165




233518







203




234536




235186




234536







204




235379




236689




235379







205




236680




237618




236689







206




237521




238345




237521







207




238281




238973




238281







208




238871




240115




238871







209




240191




241564




240191







210




242281




241604




242281







211




242933




242274




242933







212




243416




242976




243416







213




243500




244531




243500







214




244480




246021




244480







215




246330




247811




246330







216




247831




249174




247870







217




249437




251038




249455







218




251325




252212




251325







219




253156




254007




253156







220




253974




254852




253974







221




255258




256094




255258







222




256640




257455




256640







223




257502




258239




257502







224




257869




257501




257869







225




259248




260897




259248







226




262753




261788




262753







227




263059




262757




263059







228




264375




263182




264375







229




265985




264747




265985







230




266637




266059




266637







231




267338




266538




267338







232




267922




267473




267922







233




269647




270771




269647







234




272777




273145




272777







235




273253




273636




273253







236




273705




273977




273705







237




276016




275717




276016







238




276439




276020




276418







239




276792




277253




276792







240




277318




277599




277318







241




278578




277877




278578







242




279258




278554




279258







243




280435




279533




280435







244




281547




280849




281547







245




281696




282325




281717







246




282459




284069




282459







247




284056




284517




284056







248




284606




285775




284606







249




285592




285987




285592







250




286179




286976




286179







251




287583




287002




287583







252




287951




287451




287951







253




288499




288816




288499







254




289674




288505




289674







255




288839




289213




288839







256




289970




290254




289970







257




291931




292803




291931







258




293258




292755




293258







259




293718




293272




293718







260




294630




293953




294630







261




296153




294636




296153







262




294817




295068




294817







263




296354




297862




296354







264




298415




297879




298415







265




298777




298253




298777







266




299572




298781




299572







267




300487




299633




300487







268




301586




300702




301568







269




302440




301571




302440







270




302838




302437




302838







271




303335




302745




303335







272




304394




303852




304394







273




304606




305223




304606







274




305394




306236




305394







275




306501




307439




306501







276




308033




307458




308033







277




308924




308037




308924







278




309485




310180




309485







279




310426




311214




310426







280




311597




311253




311504







281




312772




311780




312772







282




313425




312772




313425







283




313646




313377




313646







284




313937




314665




313937







285




315576




314755




315576







286




316157




315531




316157







287




318657




316156




318657







288




321042




318676




321042







289




321445




321098




321445







290




322309




321710




322309







291




323190




322366




323181







292




323843




323181




323843







293




324878




323856




324878







294




325340




326410




325340







295




326433




327836




326433







296




328465




327839




328465







297




329360




328857




329360







298




330907




329357




330907







299




332455




330956




332455







300




334536




332395




334536







301




336091




334877




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1098852




1098430







1237




1098798




1099319




1098798







1238




1123198




1123515




1123198







1239




1123606




1124256




1123606







1240




1124453




1124797




1124453







1241




1129253




1129567




1129253







1242




1164947




1164474




1164947







1243




1170457




1170053




1170457







1244




1172342




1171863




1172342







1245




1192155




1192835




1192155







1246




1192759




1192992




1192759







1247




1193861




1194142




1193861







1248




1194036




1193779




1194036







1249




1209748




1209053




1209748







1250




1215111




1215419




1215111







1251




1216302




1216538




1216302







1252




1228072




1227818




1228072







1253




1228304




1228080




1228304







1254




26599




26222




26599







1255




27609




27367




27609







1256




67206




66967




67197







1257




70612




70352




70588







1258




132703




132945




132703







1259




178073




178393




178073







1260




208576




208349




208576







1261




209156




208929




209156







1262




209263




209024




209263







1263




210304




210639




210304







1264




299009




299452




299030







1265




352106




351717




352061







1266




420182




419949




420170







1267




553602




553381




553602







1268




556538




556807




556538







1269




594348




593797




594342







1270




595169




594876




595160







1271




662148




662381




662160







1272




706528




706893




706528







1273




803315




803650




803339







1274




849551




849306




849551







1275




913676




913275




913676







1276




927087




926836




927087







1277




930587




930360




930587







1278




986531




986764




986531







1279




996229




996486




996229







1280




1000373




1000002




1000334







1281




1010291




1010037




1010273







1282




1011128




1010793




1011128







1283




1012924




1012694




1012924







1284




1028659




1028913




1028659







1285




1086481




1086762




1086481







1286




1118658




1118879




1118658







1287




1170098




1169835




1170098







1288




1180828




1181184




1180828







1289




1182658




1183035




1182658







1290




1195076




1194795




1195055







1291




1195890




1196183




1195890







1292




189042




188809




189030







1293




691250




691567




691250







1294




914544




914780




914556







1295




928525




928833




928579







1296




1040685




1040948




1040712







1297




377646




378068




377646



























TABLE 4









SEQ ID NO (ORF)




Fp




Fd




Bp




Bd



























2




1292




1293




3796




3797






3




1294




1295




3798




3799






4




1296




1297




3800




3801






5




1298




1299




3802




3803






6




1300




1301




3804




3805






7




1302




1303




3806




3807






8




1304




1305




3808




3809






9




1306




1307




3810




3811






10




1308




1309




3812




3813






11




1310




1311




3814




3815






12




1312




1313




3816




3817






13




1314




1315




3818




3819






14




1316




1317




3820




3821






15




1318




1319




3822




3823






16




1320




1321




3824




3825






17




1322




1323




3826




3827






18




1324




1325




3828




3829






19




1326




1327




3830




3831






20




1328




1329




3832




3833






21




1330




1331




3834




3835






22




1332




1333




3836




3837






23




1334




1335




3838




3839






24




1336




1337




3840




3841






25




1338




1339




3842




3843






26




1340




1341




3844




3845






27




1342




1343




3846




3847






28




1344




1345




3848




3849






29




1346




1347




3850




3851






30




1348




1349




3852




3853






31




1350




1351




3854




3855






32




1352




1353




3856




3857






33




1354




1355




3858




3859






34




1358




1359




3862




3863






35




1356




1357




3860




3861






36




1360




1361




3864




3865






37




1362




1363




3866




3867






38




1364




1365




3868




3869






39




1366




1367




3870




3871






40




1368




1369




3872




3873






41




1370




1371




3874




3875






42




1374




1375




3878




3879






43




1376




1377




3880




3881






44




1380




1381




3884




3885






45




1382




1383




3886




3887






46




1386




1387




3890




3891






47




1388




1389




3892




3893






48




1392




1393




3896




3897






49




1394




1395




3898




3899






50




1396




1397




3900




3901






51




1398




1399




3902




3903






52




1402




1403




3906




3907






53




1400




1401




3904




3905






54




1404




1405




3908




3909






55




1406




1407




3910




3911






56




1410




1411




3914




3915






57




1412




1413




3916




3917






58




1414




1415




3918




3919






59




1416




1417




3920




3921






60




1418




1419




3922




3923






61




1420




1421




3924




3925






62




1422




1423




3926




3927






63




1424




1425




3928




3929






64




1426




1427




3930




3931






65




1428




1429




3932




3933






66




1430




1431




3934




3935






67




1432




1433




3936




3937






68




1434




1435




3938




3939






69




1438




1439




3942




3943






70




1440




1441




3944




3945






71




1444




1445




3948




3949






72




1446




1447




3950




3951






73




1448




1449




3952




3953






74




1450




1451




3954




3955






75




1452




1453




3956




3957






76




1454




1455




3958




3959






77




1456




1457




3960




3961






78




1458




1459




3962




3963






79




1460




1461




3964




3965






80




1462




1463




3966




3967






81




1464




1465




3968




3969






82




1468




1469




3972




3973






83




1470




1471




3974




3975






84




1472




1473




3976




3977






85




1476




1477




3980




3981






86




1478




1479




3982




3983






87




1480




1481




3984




3985






88




1482




1483




3986




3987






89




1484




1485




3988




3989






90




1486




1487




3990




3991






91




1488




1489




3992




3993






92




1490




1491




3994




3995






93




1492




1493




3996




3997






94




1494




1495




3998




3999






95




1496




1497




4000




4001






96




1498




1499




4002




4003






97




1500




1501




4004




4005






98




1502




1503




4006




4007






99




1504




1505




4008




4009






100




1506




1507




4010




4011






101




1508




1509




4012




4013






102




1510




1511




4014




4015






103




1512




1513




4016




4017






104




1514




1515




4018




4019






105




1516




1517




4020




4021






106




1518




1519




4022




4023






107




1520




1521




4024




4025






108




1522




1523




4026




4027






109




1524




1525




4028




4029






110




1526




1527




4030




4031






111




1530




1531




4034




4035






112




1532




1533




4036




4037






113




1534




1535




4038




4039






114




1536




1537




4040




4041






115




1538




1539




4042




4043






116




1540




1541




4044




4045






117




1542




1543




4046




4047






118




1544




1545




4048




4049






119




1546




1547




4050




4051






120




1548




1549




4052




4053






121




1550




1551




4054




4055






122




1552




1553




4056




4057






123




1554




1555




4058




4059






124




1556




1557




4060




4061






125




1558




1559




4062




4063






126




1562




1563




4066




4067






127




1564




1565




4068




4069






128




1566




1567




4070




4071






129




1568




1569




4072




4073






130




1570




1571




4074




4075






131




1572




1573




4076




4077






132




1574




1575




4078




4079






133




1576




1577




4080




4081






134




1580




1581




4084




4085






135




1582




1583




4086




4087






136




1584




1585




4088




4089






137




1586




1587




4090




4091






138




1588




1589




4092




4093






139




1590




1591




4094




4095






140




1592




1593




4096




4097






141




1594




1595




4098




4099






142




1596




1597




4100




4101






143




1598




1599




4102




4103






144




1604




1605




4108




4109






145




1606




1607




4110




4111






146




1612




1613




4116




4117






147




1614




1615




4118




4119






148




1616




1617




4120




4121






149




1618




1619




4122




4123






150




1620




1621




4124




4125






151




1624




1625




4128




4129






152




1622




1623




4126




4127






153




1626




1627




4130




4131






154




1628




1629




4132




4133






155




1630




1631




4134




4135






156




1632




1633




4136




4137






157




1634




1635




4138




4139






158




1636




1637




4140




4141






159




1638




1639




4142




4143






160




1640




1641




4144




4145






161




1642




1643




4146




4147






162




1644




1645




4148




4149






163




1646




1647




4150




4151






164




1648




1649




4152




4153






165




1650




1651




4154




4155






166




1652




1653




4156




4157






167




1656




1657




4160




4161






168




1658




1659




4162




4163






169




1662




1663




4166




4167






170




1664




1665




4168




4169






171




1666




1667




4170




4171






172




1668




1669




4172




4173






173




1670




1671




4174




4175






174




1672




1673




4176




4177






175




1674




1675




4178




4179






176




1676




1677




4180




4181






177




1678




1679




4182




4183






178




1684




1685




4188




4189






179




1686




1687




4190




4191






180




1688




1689




4192




4193






181




1690




1691




4194




4195






182




1694




1695




4198




4199






183




1696




1697




4200




4201






184




1698




1699




4202




4203






185




1700




1701




4204




4205






186




1704




1705




4208




4209






187




1708




1709




4212




4213






188




1710




1711




4214




4215






189




1712




1713




4216




4217






190




1714




1715




4218




4219






191




1720




1721




4224




4225






192




1722




1723




4226




4227






193




1724




1725




4228




4229






194




1726




1727




4230




4231






195




1728




1729




4232




4233






196




1732




1733




4236




4237






197




1734




1735




4238




4239






198




1736




1737




4240




4241






199




1738




1739




4242




4243






200




1740




1741




4244




4245






201




1742




1743




4246




4247






202




1744




1745




4248




4249






203




1746




1747




4250




4251






204




1750




1751




4254




4255






205




1752




1753




4256




4257






206




1754




1755




4258




4259






207




1756




1757




4260




4261






208




1758




1759




4262




4263






209




1760




1761




4264




4265






210




1762




1763




4266




4267






211




1764




1765




4268




4269






212




1766




1767




4270




4271






213




1768




1769




4272




4273






214




1770




1771




4274




4275






215




1772




1773




4276




4277






216




1774




1775




4278




4279






217




1776




1777




4280




4281






218




1778




1779




4282




4283






219




1782




1783




4286




4287






220




1784




1785




4288




4289






221




1786




1787




4290




4291






222




1788




1789




4292




4293






223




1790




1791




4294




4295






224




1792




1793




4296




4297






225




1796




1797




4300




4301






226




1800




1801




4304




4305






227




1802




1803




4306




4307






228




1804




1805




4308




4309






229




1806




1807




4310




4311






230




1808




1809




4312




4313






231




1810




1811




4314




4315






232




1812




1813




4316




4317






233




1818




1819




4322




4323






234




1824




1825




4328




4329






235




1826




1827




4330




4331






236




1828




1829




4332




4333






237




1834




1835




4338




4339






238




1836




1837




4340




4341






239




1840




1841




4344




4345






240




1842




1843




4346




4347






241




1846




1847




4350




4351






242




1848




1849




4352




4353






243




1850




1851




4354




4355






244




1852




1853




4356




4357






245




1854




1855




4358




4359






246




1856




1857




4360




4361






247




1858




1859




4362




4363






248




1860




1861




4364




4365






249




1862




1863




4366




4367






250




1864




1865




4368




4369






251




1866




1867




4370




4371






252




1868




1869




4372




4373






253




1872




1873




4376




4377






254




1876




1877




4380




4381






255




1874




1875




4378




4379






256




1878




1879




4382




4383






257




1886




1887




4390




4391






258




1888




1889




4392




4393






259




1890




1891




4394




4395






260




1892




1893




4396




4397






261




1896




1897




4400




4401






262




1894




1895




4398




4399






263




1898




1899




4402




4403






264




1900




1901




4404




4405






265




1902




1903




4406




4407






266




1904




1905




4408




4409






267




1906




1907




4410




4411






268




1908




1909




4412




4413






269




1910




1911




4414




4415






270




1912




1913




4416




4417






271




1914




1915




4418




4419






272




1916




1917




4420




4421






273




1918




1919




4422




4423






274




1920




1921




4424




4425






275




1922




1923




4426




4427






276




1924




1925




4428




4429






277




1926




1927




4430




4431






278




1928




1929




4432




4433






279




1930




1931




4434




4435






280




1934




1935




4438




4439






281




1936




1937




4440




4441






282




1938




1939




4442




4443






283




1940




1941




4444




4445






284




1942




1943




4446




4447






285




1944




1945




4448




4449






286




1946




1947




4450




4451






287




1948




1949




4452




4453






288




1950




1951




4454




4455






289




1952




1953




4456




4457






290




1954




1955




4458




4459






291




1956




1957




4460




4461






292




1958




1959




4462




4463






293




1960




1961




4464




4465






294




1962




1963




4466




4467






295




1964




1965




4468




4469






296




1966




1967




4470




4471






297




1970




1971




4474




4475






298




1972




1973




4476




4477






299




1974




1975




4478




4479






300




1976




1977




4480




4481






301




1978




1979




4482




4483






302




1980




1981




4484




4485






303




1984




1985




4488




4489






304




1986




1987




4490




4491






305




1988




1989




4492




4493






306




1990




1991




4494




4495






307




1992




1993




4496




4497






308




1994




1995




4498




4499






309




1996




1997




4500




4501






310




1998




1999




4502




4503






311




2000




2001




4504




4505






312




2002




2003




4506




4507






313




2004




2005




4508




4509






314




2006




2007




4510




4511






315




2008




2009




4512




4513






316




2010




2011




4514




4515






317




2012




2013




4516




4517






318




2014




2015




4518




4519






319




2016




2017




4520




4521






320




2018




2019




4522




4523






321




2020




2021




4524




4525






322




2022




2023




4526




4527






323




2026




2027




4530




4531






324




2024




2025




4528




4529






325




2028




2029




4532




4533






326




2030




2031




4534




4535






327




2032




2033




4536




4537






328




2034




2035




4538




4539






329




2038




2039




4542




4543






330




2040




2041




4544




4545






331




2042




2043




4546




4547






332




2044




2045




4548




4549






333




2046




2047




4550




4551






334




2048




2049




4552




4553






335




2050




2051




4554




4555






336




2052




2053




4556




4557






337




2054




2055




4558




4559






338




2056




2057




4560




4561






339




2058




2059




4562




4563






340




2060




2061




4564




4565






341




2062




2063




4566




4567






342




2064




2065




4568




4569






343




2066




2067




4570




4571






344




2068




2069




4572




4573






345




2070




2071




4574




4575






346




2072




2073




4576




4577






347




2074




2075




4578




4579






348




2076




2077




4580




4581






349




2078




2079




4582




4583






350




2080




2081




4584




4585






351




2082




2083




4586




4587






352




2084




2085




4588




4589






353




2088




2089




4592




4593






354




2090




2091




4594




4595






355




2092




2093




4596




4597






356




2094




2095




4598




4599






357




2096




2097




4600




4601






358




2100




2101




4604




4605






359




2102




2103




4606




4607






360




2104




2105




4608




4609






361




2106




2107




4610




4611






362




2108




2109




4612




4613






363




2110




2111




4614




4615






364




2112




2113




4616




4617






365




2114




2115




4618




4619






366




2116




2117




4620




4621






367




2118




2119




4622




4623






368




2120




2121




4624




4625






369




2122




2123




4626




4627






370




2124




2125




4628




4629






371




2128




2129




4632




4633






372




2130




2131




4634




4635






373




2134




2135




4638




4639






374




2136




2137




4640




4641






375




2138




2139




4642




4643






376




2140




2141




4644




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570




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571




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2642




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2644




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5148




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609




2646




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5150




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610




2650




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5154




5155






611




2648




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5152




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612




2652




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5156




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613




2654




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5158




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614




2656




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5160




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615




2658




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616




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617




2662




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618




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5168




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619




2666




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5170




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620




2668




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621




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622




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623




2678




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5182




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624




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5180




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625




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626




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627




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628




2686




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5190




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629




2688




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5192




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630




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631




2692




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632




2696




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5200




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633




2698




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634




2700




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635




2702




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636




2704




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637




2706




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638




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639




2712




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640




2714




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641




2716




2117




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642




2718




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643




2720




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644




2722




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645




2724




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2736




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651




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652




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653




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654




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655




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656




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657




2754




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658




2756




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659




2758




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660




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661




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662




2764




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5268




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663




2766




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5270




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664




2768




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5272




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665




2770




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666




2772




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5276




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667




2774




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5278




5279






668




2776




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5280




5281






669




2778




2779




5282




5283






670




2780




2781




5284




5285






671




2782




2783




5286




5287






672




2784




2785




5288




5289






673




2786




2787




5290




5291






674




2788




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5292




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675




2790




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676




2792




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677




2794




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5299






678




2796




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5300




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679




2798




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5302




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680




2800




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681




2804




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682




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683




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684




2810




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685




2812




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686




2814




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687




2816




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5321






688




2818




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689




2820




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690




2822




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5326




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691




2824




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5328




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692




2826




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5330




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693




2828




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5333






694




2830




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695




2832




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696




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697




2836




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698




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699




2840




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700




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701




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702




2846




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703




2848




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704




2850




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705




2852




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5356




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706




2854




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5358




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707




2856




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5360




5361






708




2858




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5362




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709




2860




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5364




5365






710




2862




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5366




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711




2864




2865




5368




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712




2866




2867




5370




5371






713




2868




2869




5372




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714




2870




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5374




5375






715




2872




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5376




5377






716




2874




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5378




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717




2876




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5380




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718




2878




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5382




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719




2880




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5384




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720




2882




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5386




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721




2886




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5390




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722




2888




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5392




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723




2884




2885




5388




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724




2890




2891




5394




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725




2892




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5396




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726




2894




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5398




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727




2896




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5400




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728




2900




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5404




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729




2902




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5406




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730




2904




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731




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5410




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732




2908




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5412




5413






733




2910




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734




2912




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5416




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735




2914




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5418




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736




2916




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5420




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737




2918




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5422




5423






738




2920




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739




2922




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5426




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740




2924




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741




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742




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743




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744




2932




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745




2934




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746




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747




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748




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749




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750




2944




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751




2946




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752




2948




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753




2952




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754




2954




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755




2956




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5460




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756




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757




2960




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758




2962




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759




2964




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760




2966




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5471






761




2968




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5472




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762




2970




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763




2972




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5476




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764




2974




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5478




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765




2976




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766




2978




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767




2980




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768




2982




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5486




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769




2984




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770




2986




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5490




5491






771




2990




2991




5494




5495






772




2992




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5496




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773




2994




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5498




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774




2996




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5500




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775




2998




2999




5502




5503






776




3000




3001




5504




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777




3002




3003




5506




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778




3004




3005




5508




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779




3006




3007




5510




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780




3008




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5512




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781




3010




3011




5514




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782




3012




3013




5516




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783




3014




3015




5518




5519






784




3016




3017




5520




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785




3020




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5524




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786




3022




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5526




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787




3024




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5528




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788




3026




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789




3028




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5532




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790




3030




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5534




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791




3032




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5536




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792




3034




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5538




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793




3036




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3038




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795




3040




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3044




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3046




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799




3048




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800




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5555






801




3052




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5556




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802




3054




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5558




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803




3056




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5560




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804




3058




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5562




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805




3060




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806




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807




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808




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809




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810




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811




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813




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814




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816




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818




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820




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3100




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825




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827




3106




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828




3108




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829




3110




3111




5614




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830




3112




3113




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831




3114




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832




3116




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5620




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833




3120




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834




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835




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836




3128




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837




3130




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5634




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838




3132




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839




3134




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5638




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840




3136




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841




3138




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842




3140




3141




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843




3142




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844




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845




3146




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5650




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846




3148




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847




3150




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848




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849




3154




3155




5658




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850




3156




3157




5660




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851




3158




3159




5662




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852




3160




3161




5664




5665






853




3164




3165




5668




5669






854




3162




3163




5666




5667






855




3166




3167




5670




5671






856




3168




3169




5672




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857




3170




3171




5674




5675






858




3172




3173




5676




5677






859




3174




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5678




5679






860




3176




3177




5680




5681






861




3180




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5684




5685






862




3178




3179




5682




5683






863




3182




3183




5686




5687






864




3184




3185




5688




5689






865




3186




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5690




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866




3188




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5692




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867




3190




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868




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869




3194




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5698




5699






870




3196




3197




5700




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871




3198




3199




5702




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872




3200




3201




5704




5705






873




3202




3203




5706




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874




3204




3205




5708




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875




3206




3207




5710




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876




3210




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877




3212




3213




5716




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878




3214




3215




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879




3216




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5720




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880




3218




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881




3220




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882




3222




3223




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883




3224




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5728




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884




3226




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885




3228




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886




3230




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887




3232




3233




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888




3234




3235




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889




3236




3237




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890




3238




3239




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891




3240




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892




3244




3245




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893




3246




3247




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5751






894




3248




3249




5752




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895




3250




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896




3252




3253




5756




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897




3254




3255




5758




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898




3256




3257




5760




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899




3258




3259




5762




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900




3260




3261




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901




3262




3263




5766




5767






902




3264




3265




5768




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903




3266




3267




5770




5771






904




3268




3269




5772




5773






905




3270




3271




5774




5775






906




3272




3273




5776




5777






907




3274




3275




5778




5779






908




3276




3277




5780




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909




3278




3279




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910




3280




3281




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5785






911




3282




3283




5786




5787






912




3284




3285




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5789






913




3286




3287




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5791






914




3288




3289




5792




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915




3290




3291




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916




3292




3293




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5797






917




3296




3297




5800




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918




3298




3299




5802




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919




3300




3301




5804




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920




3302




3303




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921




3304




3305




5808




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922




3306




3307




5810




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3308




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5812




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924




3310




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925




3316




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926




3314




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927




3324




3325




5828




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928




3326




3327




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929




3328




3329




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930




3330




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931




3338




3339




5842




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932




3336




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933




3340




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934




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5846




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935




3344




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936




3346




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5851






937




3348




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5852




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938




3350




3351




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939




3352




3353




5856




5857






940




3354




3355




5858




5859






941




3356




3357




5860




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942




3360




3361




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943




3362




3363




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944




3364




3365




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945




3366




3367




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5871






946




3368




3369




5872




5873






947




3370




3371




5874




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948




3374




3375




5878




5879






949




3378




3379




5882




5883






950




3376




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951




3380




3381




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5885






952




3382




3383




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953




3384




3385




5888




5889






954




3386




3387




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5891






955




3388




3389




5892




5893






956




3390




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957




3392




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5897






958




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959




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960




3398




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5902




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961




3400




3401




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962




3402




3403




5906




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963




3404




3405




5908




5909






964




3406




3407




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965




3408




3409




5912




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966




3410




3411




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967




3412




3413




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968




3414




3415




5918




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969




3416




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970




3418




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971




3420




3421




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972




3422




3423




5926




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973




3424




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974




3426




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975




3428




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976




3430




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977




3432




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978




3434




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979




3436




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980




3438




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981




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986




3450




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5954




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987




3454




3455




5958




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988




3456




3457




5960




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989




3458




3459




5962




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990




3460




3461




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991




3462




3463




5966




5967






992




3464




3465




5968




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993




3466




3467




5970




5971






994




3468




3469




5972




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995




3470




3471




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996




3472




3473




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997




3474




3475




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998




3476




3477




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999




3478




3479




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1000




3480




3481




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1001




3482




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1002




3484




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1003




3486




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5990




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1004




3488




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1005




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1006




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1007




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6000




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1008




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1009




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1016




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1021




3526




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1024




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1026




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1033




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1035




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1036




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1037




3562




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1038




3564




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6068




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1039




3566




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6070




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1040




3568




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6072




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1041




3570




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1042




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1047




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1049




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1051




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1052




3600




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1053




3602




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6106




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1054




3604




3605




6108




6109






1055




3606




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6110




6111






1056




3608




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6112




6113






1057




3610




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1058




3612




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6116




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1059




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1060




3616




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6120




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1061




3618




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6122




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1062




3620




3621




6124




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1063




3622




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1064




3624




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6128




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1065




3626




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6130




6131






1066




3628




3629




6132




6133






1067




3630




3631




6134




6135






1068




3632




3633




6136




6137






1069




3634




3635




6138




6139






1070




3636




3637




6140




6141






1071




3638




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6142




6143






1072




3640




3641




6144




6145






1073




3642




3643




6146




6147






1074




3644




3645




6148




6149






1075




3646




3647




6150




6151






1076




3648




3649




6152




6153






1077




3652




3653




6156




6157






1078




3654




3655




6158




6159






1079




3656




3657




6160




6161






1080




3658




3659




6162




6163






1081




3660




3661




6164




6165






1082




3662




3663




6166




6167






1083




3666




3667




6170




6171






1084




3668




3669




6172




6173






1085




3672




3673




6176




6177






1086




3674




3675




6178




6179






1087




3676




3677




6180




6181






1088




3678




3679




6182




6183






1089




3680




3681




6184




6185






1090




3682




3683




6186




6187






1091




3684




3685




6188




6189






1092




3686




3687




6190




6191






1093




3688




3689




6192




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1094




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3691




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1095




3692




3693




6196




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1096




3694




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6198




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1097




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3697




6200




6201






1098




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6202




6203






1099




3702




3703




6206




6207






1100




3700




3701




6204




6205






1101




3704




3705




6208




6209






1102




3706




3707




6210




6211






1103




3708




3709




6212




6213






1104




3714




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6218




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1105




3720




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6224




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1106




3722




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1107




3724




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6228




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1108




3726




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6230




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1109




3728




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1110




3730




3731




6234




6235






1111




3732




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1112




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1113




3736




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1114




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6244




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1115




3738




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1116




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6246




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1117




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1118




3746




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6250




6251






1119




3748




3749




6252




6253






1120




3750




3751




6254




6255






1121




3754




3755




6258




6259






1122




3756




3757




6260




6261






1123




3758




3759




6262




6263






1124




3760




3761




6264




6265






1125




3762




3763




6266




6267






1126




3766




3767




6270




6271






1127




3770




3771




6274




6275






1128




3772




3773




6276




6277






1129




3776




3777




6280




6281






1130




3774




3775




6278




6279






1131




3778




3779




6282




6283






1132




3780




3781




6284




6285






1133




3782




3783




6286




6287






1134




3784




3785




6288




6289






1135




3788




3789




6292




6293






1136




3786




3787




6290




6291






1137




3794




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6298




6299






1138




1372




1373




3876




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1139




1378




1379




3882




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1140




1384




1385




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1141




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1391




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1142




1408




1409




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1146




1474




1475




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1147




1528




1529




4032




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1148




1560




1561




4064




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1149




1578




1579




4082




4083






1150




1600




1601




4104




4105






1151




1602




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4106




4107






1152




1608




1609




4112




4113






1153




1610




1611




4114




4115






1154




1654




1655




4158




4159






1155




1660




1661




4164




4165






1156




1680




1681




4184




4185






1157




1682




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4186




4187






1158




1692




1693




4196




4197






1159




1702




1703




4206




4207






1160




1706




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4210




4211






1161




1716




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4220




4221






1162




1718




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4222




4223






1163




1730




1731




4234




4235






1164




1748




1749




4252




4253






1165




1780




1781




4284




4285






1166




1794




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4298




4299






1167




1798




1799




4302




4303






1168




1814




1815




4318




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1169




1816




1817




4320




4321






1170




1820




1821




4324




4325






1171




1822




1823




4326




4327






1172




1830




1831




4334




4335






1173




1832




1833




4336




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1174




1838




1839




4342




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1175




1844




1845




4348




4349






1176




1870




1871




4374




4375






1177




1880




1881




4384




4385






1178




1882




1883




4386




4387






1179




1884




1885




4388




4389






1180




1932




1933




4436




4437






1181




1968




1969




4472




4473






1182




1982




1983




4486




4487






1183




2036




2037




4540




4541






1184




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4590




4591






1185




2098




2099




4602




4603






1186




2126




2127




4630




4631






1187




2132




2133




4636




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1188




2166




2167




4670




4671






1189




2168




2169




4672




4673






1190




2184




2185




4688




4689






1191




2240




2241




4744




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1192




2276




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1193




2300




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4804




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1194




2302




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4806




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1195




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1196




2336




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1197




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4952




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1198




2452




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4956




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1199




2484




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1200




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5016




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1208




2670




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5174




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1209




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1210




2708




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2730




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5234




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1212




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5238




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1213




2746




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5250




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1214




2802




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5306




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1215




2898




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1216




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1217




2988




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5492




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1218




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5602




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1220




3118




3119




5622




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1221




3126




3127




5630




5631






1222




3208




3209




5712




5713






1223




3242




3243




5746




5747






1224




3294




3295




5798




5799






1225




3312




3313




5816




5817






1226




3318




3319




5822




5823






1227




3320




3321




5824




5825






1228




3322




3323




5826




5827






1229




3332




3333




5836




5837






1230




3334




3335




5838




5839






1231




3358




3359




5862




5863






1232




3372




3373




5876




5877






1233




3452




3453




5956




5957






1234




3492




3493




5996




5997






1235




3514




3515




6018




6019






1236




3538




3539




6042




6043






1237




3540




3541




6044




6045






1238




3576




3577




6080




6081






1239




3578




3579




6082




6083






1240




3580




3581




6084




6085






1241




3590




3591




6094




6095






1242




3650




3651




6154




6155






1243




3664




3665




6168




6169






1244




3670




3671




6174




6175






1245




3710




3711




6214




6215






1246




3712




3713




6216




6217






1247




3716




3717




6220




6221






1248




3718




3719




6222




6223






1249




3752




3753




6256




6257






1250




3764




3765




6268




6269






1251




3768




3769




6272




6273






1252




3790




3791




6294




6295






1253




3792




3793




6296




6297






1254




6300




6301




6376




6377






1255




6302




6303




6378




6379






1256




6304




6305




6380




6381






1257




6306




6307




6382




6383






1258




6308




6309




6384




6385






1259




6310




6311




6386




6387






1260




6312




6313




6388




6389






1261




6314




6315




6390




6391






1262




6316




6317




6392




6393






1263




6318




6319




6394




6395






1264




6320




6321




6396




6397






1265




6322




6323




6398




6399






1266




6324




6325




6400




6401






1267




6326




6327




6402




6403






1268




6328




6329




6404




6405






1269




6330




6331




6406




6407






1270




6332




6333




6408




6409






1271




6334




6335




6410




6411






1272




6336




6337




6412




6413






1273




6338




6339




6414




6415






1274




6340




6341




6416




6417






1275




6342




6343




6418




6419






1276




6344




6345




6420




6421






1277




6346




6347




6422




6423






1278




6348




6349




6424




6425






1279




6350




6351




6426




6427






1280




6352




6353




6428




6429






1281




6354




6355




6430




6431






1282




6356




6357




6432




6433






1283




6358




6359




6434




6435






1284




6360




6361




6436




6437






1285




6362




6363




6438




6439






1286




6364




6365




6440




6441






1287




6366




6367




6442




6443






1288




6368




6369




6444




6445






1289




6370




6371




6446




6447






1290




6372




6373




6448




6449






1291




6374




6375




6450




6451
























TABLE 5









SEQ ID




or.




5′ position

























1292




F




1229848






1293




F




1227874






1294




F




1018






1295




F




1229162






1296




F




1588






1297




F




1229711






1298




F




2253






1299




F




369






1300




F




3381






1301




F




1508






1302




F




4042






1303




F




2126






1304




F




5735






1305




F




3843






1306




F




7832






1307




F




5909






1308




F




8887






1309




F




7010






1310




F




10139






1311




F




8175






1312




F




10640






1313




F




8799






1314




F




10997






1315




F




9037






1316




F




12458






1317




F




10572






1318




F




14187






1319




F




12365






1320




F




15529






1321




F




13629






1322




F




17626






1323




F




15699






1324




F




20909






1325




F




19006






1326




F




21800






1327




F




19927






1328




F




23462






1329




F




21557






1330




F




25637






1331




F




23729






1332




F




25997






1333




F




24071






1334




F




26727






1335




F




24828






1336




F




27528






1337




F




25628






1338




F




28643






1339




F




26765






1340




F




29202






1341




F




27313






1342




F




29793






1343




F




27835






1344




F




31488






1345




F




29639






1346




F




31957






1347




F




30050






1348




F




33570






1349




F




31666






1350




F




34564






1351




F




32664






1352




F




35783






1353




F




33875






1354




F




37597






1355




F




35741






1356




F




39135






1357




F




37236






1358




F




38939






1359




F




37038






1360




F




40872






1361




F




38972






1362




F




42825






1363




F




40923






1364




F




43563






1365




F




41652






1366




F




44531






1367




F




42623






1368




F




45150






1369




F




43250






1370




F




45478






1371




F




43579






1372




F




46755






1373




F




44874






1374




F




47347






1375




F




45386






1376




F




47818






1377




F




45897






1378




F




48893






1379




F




46995






1380




F




49907






1381




F




48000






1382




F




51088






1383




F




49169






1384




F




52651






1385




F




50721






1386




F




53065






1387




F




51176






1388




F




53516






1389




F




51611






1390




F




54242






1391




F




52351






1392




F




55058






1393




F




53159






1394




F




56274






1395




F




54348






1396




F




57078






1397




F




55156






1398




F




58343






1399




F




56392






1400




F




61103






1401




F




59177






1402




F




59701






1403




F




57802






1404




F




61887






1405




F




59971






1406




F




62255






1407




F




60348






1408




F




63515






1409




F




61557






1410




F




63657






1411




F




61761






1412




F




64088






1413




F




62196






1414




F




64422






1415




F




62537






1416




F




65072






1417




F




63140






1418




F




65978






1419




F




64088






1420




F




67046






1421




F




65146






1422




F




67466






1423




F




65580






1424




F




68569






1425




F




66686






1426




F




68609






1427




F




66688






1428




F




70423






1429




F




68479






1430




F




71099






1431




F




69206






1432




F




71829






1433




F




69935






1434




F




73745






1435




F




71931






1436




F




76942






1437




F




75022






1438




F




77404






1439




F




75556






1440




F




78133






1441




F




76192






1442




F




79079






1443




F




77122






1444




F




79471






1445




F




77481






1446




F




79670






1447




F




77816






1448




F




80236






1449




F




78356






1450




F




81108






1451




F




79182






1452




F




83024






1453




F




81158






1454




F




83786






1455




F




81886






1456




F




84739






1457




F




82821






1458




F




84866






1459




F




82967






1460




F




85175






1461




F




83240






1462




F




85690






1463




F




83790






1464




F




86397






1465




F




84507






1466




F




88470






1467




F




86563






1468




F




89038






1469




F




87121






1470




F




91017






1471




F




89146






1472




F




93075






1473




F




91147






1474




F




93846






1475




F




91948






1476




F




94410






1477




F




92561






1478




F




95447






1479




F




93541






1480




F




96074






1481




F




94197






1482




F




97706






1483




F




95841






1484




F




98142






1485




F




96292






1486




F




99925






1487




F




98011






1488




F




101229






1489




F




99338






1490




F




101429






1491




F




99552






1492




F




102137






1493




F




100237






1494




F




102600






1495




F




100657






1496




F




103330






1497




F




101429






1498




F




103877






1499




F




101966






1500




F




104336






1501




F




102469






1502




F




108182






1503




F




106280






1504




F




111814






1505




F




109911






1506




F




112412






1507




F




110553






1508




F




113442






1509




F




111571






1510




F




113891






1511




F




112010






1512




F




114990






1513




F




113112






1514




F




115684






1515




F




113776






1516




F




116526






1517




F




114656






1518




F




117731






1519




F




115825






1520




F




118292






1521




F




116389






1522




F




119593






1523




F




117685






1524




F




120231






1525




F




118292






1526




F




122278






1527




F




120382






1528




F




122610






1529




F




120682






1530




F




123309






1531




F




121390






1532




F




126113






1533




F




124213






1534




F




128975






1535




F




127091






1536




F




134603






1537




F




132806






1538




F




136249






1539




F




134352






1540




F




137680






1541




F




135756






1542




F




137680






1543




F




135799






1544




F




138035






1545




F




136135






1546




F




139266






1547




F




137363






1548




F




140208






1549




F




138351






1550




F




141636






1551




F




139735






1552




F




142808






1553




F




140900






1554




F




144272






1555




F




142372






1556




F




145217






1557




F




143335






1558




F




146527






1559




F




144645






1560




F




146965






1561




F




145086






1562




F




147455






1563




F




145501






1564




F




148810






1565




F




146904






1566




F




151964






1567




F




150062






1568




F




154064






1569




F




152113






1570




F




154888






1571




F




152963






1572




F




155418






1573




F




153558






1574




F




156528






1575




F




154606






1576




F




157433






1577




F




155516






1578




F




158771






1579




F




156842






1580




F




159105






1581




F




157219






1582




F




159657






1583




F




157761






1584




F




160240






1585




F




158316






1586




F




160675






1587




F




158778






1588




F




161289






1589




F




159402






1590




F




161918






1591




F




159979






1592




F




162214






1593




F




160297






1594




F




163996






1595




F




162045






1596




F




165189






1597




F




163288






1598




F




166730






1599




F




164828






1600




F




168243






1601




F




166327






1602




F




168907






1603




F




167064






1604




F




169129






1605




F




167294






1606




F




170632






1607




F




168692






1608




F




171229






1609




F




169381






1610




F




171553






1611




F




169614






1612




F




172433






1613




F




170533






1614




F




173217






1615




F




171316






1616




F




174567






1617




F




172680






1618




F




175342






1619




F




173479






1620




F




175709






1621




F




173752






1622




F




176909






1623




F




175009






1624




F




176704






1625




F




174761






1626




F




177608






1627




F




175709






1628




F




179259






1629




F




177384






1630




F




179719






1631




F




177800






1632




F




181629






1633




F




179743






1634




F




182851






1635




F




180952






1636




F




184230






1637




F




182335






1638




F




184870






1639




F




182962






1640




F




185241






1641




F




183348






1642




F




185611






1643




F




183685






1644




F




186336






1645




F




184445






1646




F




188059






1647




F




186171






1648




F




190828






1649




F




188956






1650




F




191294






1651




F




189428






1652




F




192686






1653




F




190788






1654




F




193380






1655




F




191474






1656




F




193388






1657




F




191474






1658




F




193977






1659




F




192059






1660




F




195480






1661




F




193585






1662




F




195868






1663




F




193969






1664




F




197913






1665




F




196013






1666




F




199088






1667




F




197213






1668




F




202776






1669




F




200876






1670




F




204467






1671




F




202497






1672




F




205584






1673




F




203664






1674




F




206940






1675




F




205063






1676




F




207560






1677




F




205587






1678




F




208048






1679




F




206139






1680




F




209923






1681




F




208023






1682




F




210455






1683




F




208569






1684




F




211049






1685




F




209147






1686




F




211596






1687




F




209705






1688




F




212226






1689




F




210311






1690




F




213832






1691




F




211960






1692




F




214866






1693




F




212921






1694




F




215173






1695




F




213307






1696




F




215800






1697




F




213957






1698




F




216489






1699




F




214549






1700




F




216980






1701




F




215100






1702




F




217665






1703




F




215793






1704




F




218039






1705




F




216071






1706




F




218476






1707




F




216560






1708




F




218769






1709




F




216809






1710




F




220020






1711




F




218128






1712




F




221210






1713




F




219275






1714




F




222497






1715




F




220601






1716




F




223292






1717




F




221403






1718




F




223775






1719




F




221877






1720




F




224250






1721




F




222377






1722




F




224906






1723




F




223008






1724




F




225283






1725




F




223418






1726




F




226670






1727




F




224770






1728




F




227849






1729




F




225937






1730




F




228185






1731




F




226269






1732




F




228393






1733




F




226512






1734




F




229334






1735




F




227499






1736




F




230761






1737




F




228846






1738




F




231287






1739




F




229334






1740




F




231731






1741




F




229927






1742




F




232865






1743




F




231027






1744




F




232865






1745




F




231027






1746




F




234315






1747




F




232394






1748




F




234823






1749




F




232865






1750




F




235154






1751




F




233245






1752




F




236429






1753




F




234520






1754




F




237268






1755




F




235271






1756




F




238047






1757




F




236162






1758




F




238636






1759




F




236736






1760




F




239957






1761




F




238047






1762




F




241373






1763




F




239482






1764




F




242017






1765




F




240072






1766




F




242740






1767




F




240829






1768




F




243281






1769




F




241373






1770




F




244244






1771




F




242345






1772




F




246052






1773




F




244179






1774




F




247581






1775




F




245697






1776




F




249216






1777




F




247244






1778




F




251003






1779




F




249137






1780




F




252064






1781




F




250189






1782




F




252900






1783




F




251000






1784




F




253718






1785




F




251855






1786




F




254993






1787




F




253138






1788




F




256414






1789




F




254509






1790




F




257283






1791




F




255383






1792




F




257279






1793




F




255379






1794




F




258061






1795




F




256107






1796




F




259005






1797




F




257128






1798




F




261075






1799




F




259195






1800




F




261551






1801




F




259650






1802




F




262535






1803




F




260611






1804




F




262960






1805




F




261060






1806




F




264509






1807




F




262614






1808




F




265837






1809




F




263925






1810




F




266239






1811




F




264367






1812




F




267185






1813




F




265286






1814




F




267909






1815




F




266037






1816




F




268594






1817




F




266756






1818




F




269299






1819




F




267505






1820




F




271044






1821




F




269121






1822




F




271737






1823




F




269838






1824




F




272558






1825




F




270645






1826




F




273007






1827




F




271098






1828




F




273463






1829




F




271500






1830




F




273922






1831




F




272057






1832




F




275083






1833




F




273094






1834




F




275495






1835




F




273554






1836




F




275739






1837




F




273878






1838




F




276229






1839




F




274371






1840




F




276548






1841




F




274638






1842




F




277098






1843




F




275178






1844




F




277358






1845




F




275448






1846




F




277609






1847




F




275739






1848




F




278314






1849




F




276386






1850




F




279310






1851




F




277385






1852




F




280627






1853




F




278702






1854




F




281471






1855




F




279559






1856




F




282239






1857




F




280288






1858




F




283832






1859




F




281933






1860




F




284384






1861




F




282486






1862




F




285373






1863




F




283473






1864




F




285919






1865




F




284059






1866




F




286742






1867




F




284879






1868




F




287216






1869




F




285329






1870




F




287671






1871




F




285751






1872




F




288273






1873




F




286323






1874




F




288618






1875




F




286685






1876




F




288273






1877




F




286323






1878




F




289723






1879




F




287836






1880




F




289508






1881




F




287667






1882




F




290750






1883




F




288858






1884




F




291142






1885




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104947






3998




B




103754






3999




B




105653






4000




B




104281






4001




B




106192






4002




B




104786






4003




B




106618






4004




B




108635






4005




B




110512






4006




B




112299






4007




B




114196






4008




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112839






4009




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4010




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4011




B




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4012




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4013




B




116272






4014




B




114932






4015




B




116831






4016




B




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4017




B




117886






4018




B




116781






4019




B




118702






4020




B




118284






4021




B




120181






4022




B




118749






4023




B




120691






4024




B




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4025




B




122009






4026




B




120691






4027




B




122601






4028




B




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4029




B




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4030




B




123173






4031




B




125141






4032




B




123579






4033




B




125526






4034




B




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4035




B




128539






4036




B




129398






4037




B




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4038




B




134942






4039




B




136814






4040




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136628






4041




B




138531






4042




B




138117






4043




B




139995






4044




B




138531






4045




B




140363






4046




B




138525






4047




B




140361






4048




B




139778






4049




B




141692






4050




B




140577






4051




B




142487






4052




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142067






4053




B




143981






4054




B




142919






4055




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144787






4056




B




144478






4057




B




146417






4058




B




145520






4059




B




147378






4060




B




146972






4061




B




148872






4062




B




147545






4063




B




149452






4064




B




147756






4065




B




149677






4066




B




148484






4067




B




150382






4068




B




152436






4069




B




154325






4070




B




154353






4071




B




156228






4072




B




155395






4073




B




157286






4074




B




155740






4075




B




157613






4076




B




157002






4077




B




158902






4078




B




157861






4079




B




159764






4080




B




159219






4081




B




161121






4082




B




159569






4083




B




161484






4084




B




160221






4085




B




162109






4086




B




160670






4087




B




162572






4088




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161075






4089




B




162983






4090




B




161789






4091




B




163728






4092




B




162380






4093




B




164291






4094




B




162671






4095




B




164573






4096




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164340






4097




B




166222






4098




B




165693






4099




B




167632






4100




B




166627






4101




B




168472






4102




B




168668






4103




B




170565






4104




B




169244






4105




B




171102






4106




B




169734






4107




B




171575






4108




B




171259






4109




B




173158






4110




B




171701






4111




B




173585






4112




B




172018






4113




B




173925






4114




B




172759






4115




B




174706






4116




B




173718






4117




B




175602






4118




B




174902






4119




B




176765






4120




B




175869






4121




B




177781






4122




B




176181






4123




B




178083






4124




B




177158






4125




B




179120






4126




B




177599






4127




B




179539






4128




B




177928






4129




B




179888






4130




B




179693






4131




B




181621






4132




B




180070






4133




B




181968






4134




B




182017






4135




B




183925






4136




B




182865






4137




B




184809






4138




B




184640






4139




B




186551






4140




B




185253






4141




B




187108






4142




B




185703






4143




B




187661






4144




B




186129






4145




B




188059






4146




B




186395






4147




B




188339






4148




B




188056






4149




B




189840






4150




B




191218






4151




B




193089






4152




B




191880






4153




B




193768






4154




B




193026






4155




B




194899






4156




B




193709






4157




B




195592






4158




B




194284






4159




B




196187






4160




B




194284






4161




B




196187






4162




B




196032






4163




B




197932






4164




B




196298






4165




B




198245






4166




B




198296






4167




B




200200






4168




B




199677






4169




B




201577






4170




B




203050






4171




B




204943






4172




B




204776






4173




B




206682






4174




B




205877






4175




B




207768






4176




B




207568






4177




B




209477






4178




B




208009






4179




B




209935






4180




B




208490






4181




B




210396






4182




B




209832






4183




B




211779






4184




B




210948






4185




B




212834






4186




B




211360






4187




B




213221






4188




B




212036






4189




B




213948






4190




B




212409






4191




B




214308






4192




B




214299






4193




B




216199






4194




B




215173






4195




B




217077






4196




B




215689






4197




B




217544






4198




B




216374






4199




B




218284






4200




B




216932






4201




B




218839






4202




B




217507






4203




B




219410






4204




B




218089






4205




B




220031






4206




B




218491






4207




B




220380






4208




B




218839






4209




B




220716






4210




B




219152






4211




B




221152






4212




B




220125






4213




B




221963






4214




B




221602






4215




B




223507






4216




B




222939






4217




B




224878






4218




B




223791






4219




B




225688






4220




B




224019






4221




B




225909






4222




B




224491






4223




B




226407






4224




B




225279






4225




B




227131






4226




B




225798






4227




B




227692






4228




B




227030






4229




B




228925






4230




B




228032






4231




B




229939






4232




B




228555






4233




B




230455






4234




B




228925






4235




B




230828






4236




B




229587






4237




B




231371






4238




B




231239






4239




B




233111






4240




B




231737






4241




B




233660






4242




B




232306






4243




B




234186






4244




B




233044






4245




B




234873






4246




B




234599






4247




B




236504






4248




B




233738






4249




B




235682






4250




B




235454






4251




B




237347






4252




B




235569






4253




B




237469






4254




B




236954






4255




B




238812






4256




B




237891






4257




B




239761






4258




B




238568






4259




B




240472






4260




B




239227






4261




B




241122






4262




B




240341






4263




B




242266






4264




B




241805






4265




B




243697






4266




B




242570






4267




B




244401






4268




B




243155






4269




B




245067






4270




B




243636






4271




B




245538






4272




B




244754






4273




B




246679






4274




B




246248






4275




B




248169






4276




B




248035






4277




B




249968






4278




B




249397






4279




B




251305






4280




B




251305






4281




B




253161






4282




B




252487






4283




B




254380






4284




B




253274






4285




B




255156






4286




B




254230






4287




B




256130






4288




B




255120






4289




B




256980






4290




B




256331






4291




B




258223






4292




B




257706






4293




B




259578






4294




B




258488






4295




B




260396






4296




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258089






4297




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260005






4298




B




259202






4299




B




261035






4300




B




261140






4301




B




263031






4302




B




261834






4303




B




263716






4304




B




263031






4305




B




264890






4306




B




263293






4307




B




265179






4308




B




264599






4309




B




266560






4310




B




266208






4311




B




268109






4312




B




266867






4313




B




268783






4314




B




267558






4315




B




269472






4316




B




268249






4317




B




270042






4318




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269121






4319




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271051






4320




B




269709






4321




B




271643






4322




B




271051






4323




B




272920






4324




B




271761






4325




B




273662






4326




B




272570






4327




B




274469






4328




B




273370






4329




B




275313






4330




B




273884






4331




B




275821






4332




B




274219






4333




B




276115






4334




B




274796






4335




B




276716






4336




B




275980






4337




B




277886






4338




B




276241






4339




B




278138






4340




B




276716






4341




B




278625






4342




B




277185






4343




B




279054






4344




B




277489






4345




B




279380






4346




B




277886






4347




B




279722






4348




B




278125






4349




B




280012






4350




B




278841






4351




B




280733






4352




B




279577






4353




B




281466






4354




B




280672






4355




B




282564






4356




B




281767






4357




B




283676






4358




B




282564






4359




B




284462






4360




B




284311






4361




B




286210






4362




B




284740






4363




B




286647






4364




B




285998






4365




B




287975






4366




B




286210






4367




B




288110






4368




B




287201






4369




B




289106






4370




B




287803






4371




B




289737






4372




B




288217






4373




B




290112






4374




B




288417






4375




B




290319






4376




B




289106






4377




B




290961






4378




B




289459






4379




B




291358






4380




B




289914






4381




B




291796






4382




B




290477






4383




B




292423






4384




B




290381






4385




B




292309






4386




B




291463






4387




B




293372






4388




B




292104






4389




B




293999






4390




B




293027






4391




B




294951






4392




B




293507






4393




B




295409






4394




B




293999






4395




B




295838






4396




B




294889






4397




B




296750






4398




B




295312






4399




B




297219






4400




B




296373






4401




B




298305






4402




B




298114






4403




B




299985






4404




B




298656






4405




B




300623






4406




B




299027






4407




B




300899






4408




B




299805






4409




B




301692






4410




B




300722






4411




B




302621






4412




B




301846






4413




B




303706






4414




B




302660






4415




B




304642






4416




B




303066






4417




B




304962






4418




B




303626






4419




B




305479






4420




B




304643






4421




B




306514






4422




B




305479






4423




B




307390






4424




B




306459






4425




B




308393






4426




B




307662






4427




B




309601






4428




B




308298






4429




B




310153






4430




B




309145






4431




B




311044






4432




B




310468






4433




B




312338






4434




B




311437






4435




B




313337






4436




B




311857






4437




B




313860






4438




B




311857






4439




B




313860






4440




B




313015






4441




B




314911






4442




B




313687






4443




B




315549






4444




B




313866






4445




B




315784






4446




B




314911






4447




B




316804






4448




B




315809






4449




B




317701






4450




B




316382






4451




B




318284






4452




B




318881






4453




B




320778






4454




B




321262






4455




B




323214






4456




B




321665






4457




B




323565






4458




B




322571






4459




B




324461






4460




B




323425






4461




B




325316






4462




B




324095






4463




B




325977






4464




B




325135






4465




B




327001






4466




B




326634






4467




B




328557






4468




B




328081






4469




B




322959






4470




B




328719






4471




B




330596






4472




B




328893






4473




B




330825






4474




B




329590






4475




B




331485






4476




B




331127






4477




B




333069






4478




B




332679






4479




B




334592






4480




B




334790






4481




B




336673






4482




B




336311






4483




B




338267






4484




B




337572






4485




B




339431






4486




B




338545






4487




B




340463






4488




B




339058






4489




B




341011






4490




B




339740






4491




B




341628






4492




B




340366






4493




B




342354






4494




B




343265






4495




B




345125






4496




B




344126






4497




B




345957






4498




B




344391






4499




B




346291






4500




B




345324






4501




B




347236






4502




B




346289






4503




B




348198






4504




B




347090






4505




B




348914






4506




B




347292






4507




B




349158






4508




B




347946






4509




B




349851






4510




B




350799






4511




B




352598






4512




B




351313






4513




B




353223






4514




B




352400






4515




B




354357






4516




B




353522






4517




B




355411






4518




B




354620






4519




B




356610






4520




B




355158






4521




B




357057






4522




B




355676






4523




B




357681






4524




B




356995






4525




B




358866






4526




B




356173






4527




B




358074






4528




B




359607






4529




B




361536






4530




B




359550






4531




B




361442






4532




B




360135






4533




B




362033






4534




B




361536






4535




B




363461






4536




B




364013






4537




B




365905






4538




B




364716






4539




B




366707






4540




B




365000






4541




B




366941






4542




B




365513






4543




B




367447






4544




B




365892






4545




B




367873






4546




B




366877






4547




B




368725






4548




B




369265






4549




B




371167






4550




B




370088






4551




B




371988






4552




B




370669






4553




B




372611






4554




B




372871






4555




B




374773






4556




B




373315






4557




B




375227






4558




B




373665






4559




B




375592






4560




B




374428






4561




B




376335






4562




B




375355






4563




B




377248






4564




B




375913






4565




B




377796






4566




B




376483






4567




B




378318






4568




B




377873






4569




B




379798






4570




B




380040






4571




B




381898






4572




B




380699






4573




B




382561






4574




B




381249






4575




B




383174






4576




B




381689






4577




B




383629






4578




B




383282






4579




B




385161






4580




B




383789






4581




B




385647






4582




B




385560






4583




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387427






4584




B




386760






4585




B




388588






4586




B




387508






4587




B




389369






4588




B




388984






4589




B




390900






4590




B




390387






4591




B




392260






4592




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391202






4593




B




393055






4594




B




392044






4595




B




393959






4596




B




392615






4597




B




394499






4598




B




393218






4599




B




395123






4600




B




393909






4601




B




395807






4602




B




394566






4603




B




396498






4604




B




395027






4605




B




396931






4606




B




395531






4607




B




397467






4608




B




396227






4609




B




398132






4610




B




398070






4611




B




399935






4612




B




399189






4613




B




400970






4614




B




400351






4615




B




402208






4616




B




401465






4617




B




403507






4618




B




401705






4619




B




403666






4620




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402461






4621




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404410






4622




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403507






4623




B




405356






4624




B




404421






4625




B




406295






4626




B




406160






4627




B




408052






4628




B




407645






4629




B




409450






4630




B




407922






4631




B




409744






4632




B




409039






4633




B




410960






4634




B




410673






4635




B




412559






4636




B




411193






4637




B




413064






4638




B




412049






4639




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413946






4640




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414525






4641




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416425






4642




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415622






4643




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417559






4644




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416072






4645




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417968






4646




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417351






4647




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419259






4648




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417789






4649




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419748






4650




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418569






4651




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420453






4652




B




420345






4653




B




422177






4654




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421003






4655




B




422873






4656




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421819






4657




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423675






4658




B




422291






4659




B




424158






4660




B




423186






4661




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425075






4662




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424544






4663




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426443






4664




B




424859






4665




B




426714






4666




B




426302






4667




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428193






4668




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427640






4669




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429523






4670




B




428212






4671




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430111






4672




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428709






4673




B




430627






4674




B




430926






4675




B




432851






4676




B




431681






4677




B




433569






4678




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432324






4679




B




434223






4680




B




433015






4681




B




434902






4682




B




433504






4683




B




435426






4684




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434196






4685




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436042






4686




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436913






4687




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438807






4688




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437475






4689




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439423






4690




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438591






4691




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440490






4692




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4693




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442491






4694




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4695




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442441






4696




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441274






4697




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443135






4698




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441459






4699




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443353






4700




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442412






4701




B




444339






4702




B




443184






4703




B




445100






4704




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783004






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B




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B




1134070






6101




B




1136016






6102




B




1135089






6103




B




1137037






6104




B




1135815






6105




B




1137715






6106




B




1136186






6107




B




1138084






6108




B




1137365






6109




B




1139255






6110




B




1140364






6111




B




1142228






6112




B




1141611






6113




B




1143485






6114




B




1142478






6115




B




1144291






6116




B




1145907






6117




B




1147783






6118




B




1146953






6119




B




1148846






6120




B




1147769






6121




B




1149703






6122




B




1148415






6123




B




1150357






6124




B




1148758






6125




B




1150658






6126




B




1149462






6127




B




1151258






6128




B




1149932






6129




B




1151845






6130




B




1150814






6131




B




1152747






6132




B




1151409






6133




B




1153285






6134




B




1152540






6135




B




1154341






6136




B




1154863






6137




B




1156751






6138




B




1155886






6139




B




1157813






6140




B




1156963






6141




B




1158871






6142




B




1158093






6143




B




1159947






6144




B




1160998






6145




B




1162864






6146




B




1162864






6147




B




1164740






6148




B




1163244






6149




B




1165090






6150




B




1164244






6151




B




1166175






6152




B




1164517






6153




B




1166482






6154




B




1165167






6155




B




1167100






6156




B




1165789






6157




B




1167710






6158




B




1166376






6159




B




1168228






6160




B




1166872






6161




B




1168764






6162




B




1168598






6163




B




1170498






6164




B




1169447






6165




B




1171347






6166




B




1170043






6167




B




1171947






6168




B




1170689






6169




B




1172616






6170




B




1171556






6171




B




1173507






6172




B




1172305






6173




B




1174210






6174




B




1172562






6175




B




1174508






6176




B




1174018






6177




B




1175899






6178




B




1175429






6179




B




1177348






6180




B




1175793






6181




B




1177675






6182




B




1177347






6183




B




1179199






6184




B




1179316






6185




B




1181171






6186




B




1180309






6187




B




1182212






6188




B




1181048






6189




B




1182918






6190




B




1182162






6191




B




1184078






6192




B




1182528






6193




B




1184437






6194




B




1184078






6195




B




1186015






6196




B




1184698






6197




B




1186540






6198




B




1185631






6199




B




1187530






6200




B




1186079






6201




B




1188004






6202




B




1186704






6203




B




1188610






6204




B




1189251






6205




B




1191165






6206




B




1187609






6207




B




1189506






6208




B




1191165






6209




B




1193050






6210




B




1192378






6211




B




1194291






6212




B




1192265






6213




B




1194114






6214




B




1193058






6215




B




1194987






6216




B




1193224






6217




B




1195115






6218




B




1194035






6219




B




1195955






6220




B




1194384






6221




B




1196265






6222




B




1194291






6223




B




1196205






6224




B




1195955






6225




B




1197863






6226




B




1196570






6227




B




1198423






6228




B




1197051






6229




B




1198951






6230




B




1198058






6231




B




1199931






6232




B




1198960






6233




B




1200867






6234




B




1200490






6235




B




1202395






6236




B




1204512






6237




B




1203426






6238




B




1202606






6239




B




1204532






6240




B




1203139






6241




B




1205063






6242




B




1203691






6243




B




1205597






6244




B




1204382






6245




B




1206284






6246




B




1205249






6247




B




1207170






6248




B




1206651






6249




B




1208536






6250




B




1206976






6251




B




1208862






6252




B




1208092






6253




B




1210002






6254




B




1209115






6255




B




1210973






6256




B




1209979






6257




B




1211892






6258




B




1210739






6259




B




1212639






6260




B




1211761






6261




B




1213680






6262




B




1212985






6263




B




1214894






6264




B




1214299






6265




B




1216189






6266




B




1215132






6267




B




1217036






6268




B




1215714






6269




B




1217542






6270




B




1216541






6271




B




1218462






6272




B




1216828






6273




B




1218677






6274




B




1217166






6275




B




1218973






6276




B




1219876






6277




B




1221743






6278




B




1220892






6279




B




1222895






6280




B




1220288






6281




B




1222189






6282




B




1221657






6283




B




1223517






6284




B




1223930






6285




B




1225828






6286




B




1225211






6287




B




1227132






6288




B




1226090






6289




B




1227979






6290




B




1227132






6291




B




1229039






6292




B




1228061






6293




B




1229948






6294




B




1228293






6295




B




267






6296




B




1228524






6297




B




444






6298




B




267






6299




B




2068






6300




F




25997






6301




F




24032






6302




F




27128






6303




F




25189






6304




F




66744






6305




F




64845






6306




F




70130






6307




F




68200






6308




F




132477






6309




F




130559






6310




F




177854






6311




F




175906






6312




F




208127






6313




F




206180






6314




F




208688






6315




F




206807






6316




F




208732






6317




F




206877






6318




F




210051






6319




F




208141






6320




F




298801






6321




F




296907






6322




F




351495






6323




F




349572






6324




F




419727






6325




F




417822






6326




F




553133






6327




F




551247






6328




F




556301






6329




F




554410






6330




F




593567






6331




F




591675






6332




F




594641






6333




F




592748






6334




F




661934






6335




F




660041






6336




F




706309






6337




F




704409






6338




F




803092






6339




F




801192






6340




F




849060






6341




F




847142






6342




F




913050






6343




F




911152






6344




F




926614






6345




F




924714






6346




F




930121






6347




F




928238






6348




F




986297






6349




F




984362






6350




F




996001






6351




F




994109






6352




F




999731






6353




F




997877






6354




F




1009782






6355




F




1007891






6356




F




1010540






6357




F




1008671






6358




F




1012465






6359




F




1010540






6360




F




1028431






6361




F




1026524






6362




F




1086215






6363




F




1084362






6364




F




1118417






6365




F




1116527






6366




F




1169595






6367




F




1167713






6368




F




1180592






6369




F




1178709






6370




F




1182406






6371




F




1180498






6372




F




1194573






6373




F




1192667






6374




F




1195654






6375




F




1193753






6376




B




26870






6377




B




28721






6378




B




27835






6379




B




29730






6380




B




67456






6381




B




69351






6382




B




70820






6383




B




72708






6384




B




133173






6385




B




135068






6386




B




178637






6387




B




180518






6388




B




208864






6389




B




210727






6390




B




209376






6391




B




211305






6392




B




209483






6393




B




211383






6394




B




210875






6395




B




212766






6396




B




299694






6397




B




301582






6398




B




352312






6399




B




354200






6400




B




420390






6401




B




422291






6402




B




553822






6403




B




555736






6404




B




557050






6405




B




558930






6406




B




594583






6407




B




596527






6408




B




595405






6409




B




597289






6410




B




662614






6411




B




664530






6412




B




707138






6413




B




709063






6414




B




803951






6415




B




805790






6416




B




849771






6417




B




851730






6418




B




913917






6419




B




915796






6420




B




927331






6421




B




929238






6422




B




930857






6423




B




932735






6424




B




986987






6425




B




988912






6426




B




996771






6427




B




998623






6428




B




1000593






6429




B




1002496






6430




B




1010541






6431




B




1012452






6432




B




1011365






6433




B




1013249






6434




B




1013146






6435




B




1015044






6436




B




1029168






6437




B




1031036






6438




B




1087041






6439




B




1088885






6440




B




1119102






6441




B




1121033






6442




B




1170355






6443




B




1172218






6444




B




1181427






6445




B




1183338






6446




B




1183263






6447




B




1185158






6448




B




1195296






6449




B




1197175






6450




B




1196406






6451




B




1198306

























TABLE 6












Chromosomal






clone Name




SEQ ID NO (B)




SEQ ID NO (F)




region











790313H3#




6452




6648




A






790331B1#




6453




6649




A






790233A9#




6454




6650




A






790031G7#




6455




6651




A






890021E4#




6456




6652




A






790021E11#




6457




6653




A






790332G10#




6458




6654




A






790271B6#




6459




6655




A






790253H6#




6460




6656




A






790214E8#




6461




6657




A






790352D2#




6462




6658




A






790373F2#




6463




6659




A






790424A7#




6464




6660




A






790282F3#




6465




6661




A






790272F5#




6466




6662




A






790424F6#




6467




6663




A






890033H11#




6468




6664




A






790264H10#




6469




6665




A






790293A5#




6470




6666




A






790391E8#




6471




6667




A






890022B8#




6472




6668




A






790332B9#




6473




6669




A






790251B9#




6474




6670




A






790344E8#




6475




6671




B






790323F3#




6476




6672




B






790231G2#




6477




6673




B






790341C5#




6478




6674




B






790332H9#




6479




6675




B






890013A8#




6480




6676




B






790394F2#




6481




6677




B






790222G5#




6482




6678




B






790402A10#




6483




6679




B






790283F6#




6484




6680




B






790041H11#




6485




6681




B






790381C7#




6486




6682




B






790213E1#




6487




6683




B






790211C4#




6488




6684




B






790251B5#




6489




6685




B






790043H9#




6490




6686




B






790303F7#




6491




6687




B






790251G5#




6492




6688




B






790044H7#




6493




6689




B






790022E4#




6494




6690




B






790252A8#




6495




6691




B






790313E9#




6496




6692




B






790264G2#




6497




6693




B






790372A4#




6498




6694




B






790411C2#




6499




6695




B






790322B7#




6500




6696




B






790254F7#




6501




6697




B






790323B12#




6502




6698




B






790263E5#




6503




6699




B






790223C8#




6504




6700




B






790231H2#




6505




6701




B






790324E12#




6506




6702




B






790271D7#




6507




6703




B






790222E8#




6508




6704




B






790083G7#




6509




6705




B






790241D3#




6510




6706




B






790303C8#




6511




6707




B






790283F10#




6512




6708




B






790241B7#




6513




6709




B






790373F10#




6514




6710




B






790362F9#




6515




6711




B






790263H8#




6516




6712




B






790393D10#




6517




6713




B






790313D12#




6518




6714




B






890024C6#




6519




6715




B






890024B10#




6520




6716




B






790212E2#




6521




6717




B






790362E10#




6522




6718




B






790344G11#




6523




6719




B






890011D2#




6524




6720




B






790341B11#




6525




6721




B






790064E10#




6526




6722




B






790212E1#




6527




6723




B






790213G5#




6528




6724




B






790331F2#




6529




6725




B






890024B9#




6530




6726




B






790421F5#




6531




6727




B






890014D11#




6532




6728




B






790373F3#




6533




6729




B






790293D4#




6554




6730




B






790211A3#




6535




6731




B






790211H8#




6556




6732




B






790264E7#




6557




6733




B






790292B11#




6538




6734




B






790312A2#




6539




6735




B






890012D5#




6540




6736




B






790012D12#




6541




6737




B






790291E10#




6542




6738




B






790241C9#




6543




6739




B






790343F1#




6544




6740




B






790241D7#




6545




6741




B






790031H7#




6546




6742




B






790081C4#




6547




6743




B






790013B7#




6548




6744




B






790213F3#




6549




6745




B






790292F9#




6550




6746




B






790423F4#




6551




6747




B






790331F3#




6552




6748




B






790222B10#




6553




6749




B






790261G12#




6554




6750




B






790423G10#




6555




6751




B






790392A9#




6556




6752




B






790331B5#




6557




6753




B






70323H3#




6558




6754




B






890014H8#




6559




6755




B






790231B6#




6560




6756




B






790252F7#




6561




6757




B






790392C10#




6562




6758




B






790021D4#




6563




6759




B






790052D10#




6564




6760




B






790261E3#




6565




6761




B






890023E10#




6566




6762




B






790244B7#




6567




6763




B






790383E1#




6568




6764




B






790401B11#




6569




6765




B






790411B5#




6570




6766




B






790423A11#




6571




6767




B






790031A4#




6572




6768




B






790241G3#




6573




6769




B






790044F7#




6574




6770




B






790252B10#




6575




6771




B






790293F9#




6576




6772




B






790282H3#




6577




6773




B






790381C10#




6578




6774




B






790024H5#




6579




6775




B






790354H7#




6580




6776




B






790411F9#




6581




6777




B






790324G10#




6582




6778




B






790014A5#




6583




6779




B






790381F3#




6584




6780




B






790424D3#




6585




6781




B






790394A10#




6586




6782




B






790423C10#




6587




6783




B






790214D6#




6588




6784




B






790214C4#




6589




6785




B






790014F11#




6590




6786




B






790352F10#




6591




6787




B






790381H6#




6592




6788




B






790282G5#




6593




6789




B






790263C8#




6594




6790




B






890022B4#




6595




6791




B






790283C6#




6596




6792




B






790293B2#




6597




6793




B






790073A3#




6598




6794




B






790313E10#




6599




6795




B






790361D3#




6600




6796




B






790014A11#




6601




6797




B






790254G2#




6602




6798




B






790381C6#




6603




6799




B






790424E3#




6604




6800




B






790421G8#




6605




6801




B






790013C3#




6606




6802




B






790263E8#




6607




6803




B






790373C1#




6608




6804




B






790041C1#




6609




6805




B






790344A7#




6610




6806




B






790271D6#




6611




6807




B






790342H2#




6612




6808




B






890021A6#




6613




6809




B






790381E7#




6614




6810




C






790013G10#




6615




6811




C






790254A4#




6616




6812




C






790213D8#




6617




6813




C






790052A4#




6618




6814




C






790213D3#




6619




6815




C






790394D2#




6620




6816




C






790214D2#




6621




6817




C






790014A4#




6622




6818




C






790324H4#




6623




6819




C






790082B4#




6624




6820




C






790324A6#




6625




6821




C






790424A12#




6626




6822




C






790044G8#




6627




6823




C






790323C6#




6628




6824




C






790312G4#




6629




6825




C






790053C11#




6630




6826




C






890022B7#




6631




6827




C






790392A2#




6632




6828




C






890023D8#




6633




6829




C






790301F1#




6634




6830




C






790343A11#




6635




6831




C






790421A2#




6636




6832




C






790271G2#




6637




6833




C






790302G12#




6638




6834




C






790341E5#




6639




6835




C






790283B6#




6640




6836




C






790222A4#




6641




6837




C






790241B8#




6642




6838




C






790014C2#




6643




6839




C






790402C1#




6644




6840




C






790264E9#




6645




6841




C






790242G4#




6646




6842




C






790422F3#




6647




6843




C
























TABLE 7









SEQ ID




or.




5′ position

























6452




B




29372






6453




B




30198






6454




B




31007






6455




B




31126






6456




B




32735






6457




B




32264






6458




B




32898






6459




B




33582






6460




B




33519






6461




B




34836






6462




B




35795






6463




B




35548






6464




B




35825






6465




B




37239






6466




B




36761






6467




B




37045






6468




B




36761






6469




B




37958






6470




B




38636






6471




B




39813






6472




B




41140






6473




B




40575






6474




B




40526






6475




B




501495






6476




B




502410






6477




B




502586






6478




B




503233






6479




B




503749






6480




B




504488






6481




B




504206






6482




B




504310






6483




B




505455






6484




B




505877






6485




B




506655






6486




B




506513






6487




B




507532






6488




B




507742






6489




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508050






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507771






6491




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509120






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509646






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510137






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510953






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511165






6496




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511526






6497




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511993






6498




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513012






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512983






6500




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512781






6501




B




514155






6502




B




515036






6503




B




515287






6504




B




516292






6505




B




516234






6506




B




516337






6507




B




517347






6508




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517005






6509




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516888






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516234






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517560






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517337






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516756






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520123






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520574






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520888






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522217






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523035






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524995






6525




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523477






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523967






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525211






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525215






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525674






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526561






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526715






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527503






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528775






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528249






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530307






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527772






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529406






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527752






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529829






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529635






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530391






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532606






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533407






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534614






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538702






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540278






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540115






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540724






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6572




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540968






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543100






6576




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543820






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544382






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545678






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546683






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547684






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547342






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548946






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549071






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549989






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550426






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550055






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550132






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551400






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551572






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551468






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550849






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552137






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552325






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552583






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553033






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553914






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554354






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555687






6609




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6610




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557054






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556627






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557292






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557050






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817104






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817104






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816920






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820464






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821017






6620




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821379






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821504






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822723






6623




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823298






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823380






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824414






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824204






6627




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825288






6628




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825346






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825403






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826237






6631




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6632




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826838






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828146






6634




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827878






6635




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827571






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B




828472






6637




B




828484






6638




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828691






6639




B




829507






6640




B




829169






6641




B




828763






6642




B




829769






6643




B




831582






6644




B




830481






6645




B




831468






6646




B




831670






6647




B




832293






6648




F




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6649




F




29043






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F




29656






6651




F




30157






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F




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F




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F




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31902






6656




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6659




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34426






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F




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6677




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6679




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6684




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6691




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6692




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510383






6693




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6694




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511188






6695




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6696




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828348






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830281






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830491






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SEQUENCE LISTING











The patent contains a lengthy “Sequence Listing” section. A copy of the “Sequence Listing” is available in electronic form from the USPTO






web site (http://seqdata.uspto.gov/sequence.html?DocID=06559294B1). An electronic copy of the “Sequence Listing” will also be available from the






USPTO upon request and payment of the fee set forth in 37 CFR 1.19(b)(3).












Claims
  • 1. An isolated, recombinant polynucleotide comprising the nucleotide sequence of an open reading frame (ORF) of a Chlamydia pneumoniae genome selected from the group consisting of:a) a nucleotide sequence of ORF195, ORF227, ORF234, ORF1145, ORF1160, ORF1162, ORF1255, ORF1256, ORF1257, ORF1258, or the complement of the nucleotide sequence; and b) a nucleotide sequence encoding the amino acid sequence of SEQ ID NO:195, 227, 234, 1145, 1160, 1162, 1255, 1256, 1257, 1258, or the complement of the nucleotide sequence.
  • 2. The isolated, recombinant polynucleotide of claim 1, wherein the nucleotide sequences is selected from the group consisting of the nucleotide sequence of ORF195, ORF227, ORF234, ORF1145, ORF1160, ORF1162, ORF1255, ORF1256, ORF1257, ORF1258, and the complement of the nucleotide sequence.
  • 3. An isolated, recombinant polynucleotide of claim 1, wherein the nucleotide sequence is selected from the group consisting of the nucleotide sequences encoding the amino acid sequences of SEQ ID NO:195, 227, 234, 1145, 1160, 1162, 1255, 1256, 1257, 1258, and the complement of the nucleotide sequence.
  • 4. The isolated, recombinant polynucleotide of claim 1, further comprising elements necessary to direct the expression of said nucleotide sequence in a host cell.
  • 5. A recombinant host cell comprising the polynucleotide of claim 1 or 4.
  • 6. The polynucleotide of claim 1, 2, or 3, that is found in Chlamydia pneumoniae, but not in Chlamydia trachomatis.
  • 7. A polynucleotide encoding a fusion protein comprising a polynucleotide sequence according to claim 1, 2, or 3, ligated in frame to a polynucleotide encoding a heterologous polypeptide.
  • 8. A recombinant vector containing the polynucleotide of claims 1, 2, 3, or 4.
  • 9. A recombinant vector that contains the polynucleotide of claim 7.
  • 10. A genetically engineered host cell that contains the polynucleotide of claims 1, 2, 3, or 4.
  • 11. A genetically engineered host cell that contains the polynucleotide of claim 7.
  • 12. A method for producing a polypeptide comprising:(a) culturing the genetically engineered host cell of claim 5 under conditions suitable to produce the polypeptide encoded by the polynucleotide; and (b) recovering the polypeptide from the culture.
  • 13. A method for producing a fusion polypeptide comprising:(a) culturing the genetically engineered host cell of claim 11 under conditions suitable to produce the polypeptide encoded by the polynucleotide; and (b) recovering the polypeptide from the culture.
Priority Claims (1)
Number Date Country Kind
97-14673 Nov 1997 FR
CROSS REFERENCE TO RELATED APPLICATION

The present application claims the benefit of U.S. Provisional Application Ser. No. 60/107,078, filed Nov. 4, 1998.

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