Method of reducing the proteolytic degradation of bacillus thuringiensis insecticidal toxic protein

Information

  • Patent Grant
  • 5962264
  • Patent Number
    5,962,264
  • Date Filed
    Friday, May 29, 1998
    26 years ago
  • Date Issued
    Tuesday, October 5, 1999
    25 years ago
Abstract
The present invention is based on the discovery, isolation, sequencing and characterization of two protease genes present in B.t. One is an alkaline protease gene generally designated "apr." The other is a neutral protease gene generally designated "npr." The invention also includes genetically disabling the apr and the npr genes to reduce proteolytic activity of the proteases encoded by the genes, and using the disabled genes in insecticidal B.t. constructs along with one or more B.t. protein toxin genes. These resulting B.t. constructs are useful for the enhanced production of B.t. toxin protein. The B.t. toxin protein recovered from the fermentation production of these B.t. constructs also exhibits improved stability with respect to its insecticidal activity.
Description

FIELD OF THE INVENTION
The present invention relates to an alkaline protease gene (apr) and a neutral protease gene (npr) derived from a Bacillus thuringiensis (B.t.) strain, genetically disabled apr and npr genes, insecticidal B.t. strain constructs containing a genetically disabled apr gene and/or npr gene, an insecticide composition containing the disabled genes or the constructs including the disabled genes, and a method for using the disabled genes and their constructs.
BACKGROUND OF THE INVENTION
Bacillus thuringiensis ( "B.t.") is a gram-positive soil bacterium that produces proteinaceous crystalline inclusions during sporulation. These B.t. crystal proteins are often highly toxic to specific insects. Insecticidal activities have been identified for crystal proteins from various B.t. strains against insect larvae from the insect orders Lepidoptera (caterpillars), Diptera (mosquitos, flies) and Coleoptera (beetles).
Recently, certain B.t. strains and B.t. crystal proteins have been reported as having activity against non-insect species such as nematodes. The term "insecticidal," as used herein with reference to B.t. strains and their crystal proteins, is intended to include such pathogenic activities against non-insect species.
Individual B.t. crystal proteins, also called delta-endotoxins or parasporal crystals or toxin proteins, can differ extensively in their structure and insecticidal activity. These insecticidal proteins are encoded by genes typically located on large plasmids, greater than 30 megadaltons (mDa) in size, that are found in B.t. strains. A number of these B.t. toxin genes have been cloned and the insecticidal crystal protein products characterized for their specific insecticidal properties. A good review of cloned B.t. toxin genes and crystal proteins is given by Hofte et al., Microbiol. Rev. 53:242-255 (1989), who also propose a useful nomenclature and classification scheme that has been adopted here.
The insecticidal properties of B.t. have been long recognized, and B.t. strains have been incorporated in commercial biological insecticide products for over thirty years. Commercial B.t. insecticide formulations typically contain dried B.t. fermentation cultures whose crystal protein is toxic to various insect species.
Traditional commercial B.t. bioinsecticide products are derived from "wild-type" B.t. strains, i.e., purified cultures of B.t. strains isolated from natural sources. Newer commercial B.t. bioinsecticide products are based on genetically altered B.t. strains, such as the transconjugant B.t. strains described in U.S. Pat. No. 5,080,897 issued to Gonzalez, Jr., et al. on Jan. 14, 1992, and in U.S. Pat. No. 4,935,353 issued to Burges et al. on Jun. 19, 1990.
Recombinant B.t. strains, with novel complements of B.t. toxin genes providing wide spectrum and/or enhanced insecticidal activity, are likely to be incorporated into commercial B.t. bioinsecticides in the foreseeable future.
All B.t.-based bioinsecticides have the advantage of being selectively toxic to specific target insect species without exhibiting any toxicity towards vertebrates. A drawback to B.t. bioinsecticides is that the persistence of insecticidal activity is limited. The insecticidal half-life of B.t. bioinsecticides is typically less than one week in duration, even with protective adjuvants that are typically employed in commercial B.t. formulations.
Studies on loss of insecticidal activity in B.t. proteins have identified solar irradiation as a cause and have recommended the use of photoprotectants in B.t. formulations; see, for example, Pozsgay et al., J. Invertebr. Pathol. 50:246-253 (1987) and Morris, Canadian Entomol. 115:1215-1227 (1983): Cell encapsulation and cell treatment technologies such as described in U.S. Pat. Nos. 4,695,455 and 4,695,462, both issued to Barnes et al. on Sep. 22, 1987, have also been employed to protect the insecticidal toxin activity of the B.t. protein against environmental factors.
It has long been recognized that the insecticidal activity of B.t. proteins is induced, at least in part, by the action of proteolytic enzymes on B.t. protein which has been ingested by a susceptible insect species. Hofte et al., Microbiol. Rev. 53:242-255 (1989), note that B.t. crystalline protein dissolves in the larval insect midgut and that many of these B.t. proteins are protoxins that are proteolytically converted into smaller toxic polypeptides, i.e., activated toxin, in the insect midgut.
Researchers have reported the existence of proteases in B.t., but the role of these proteases in the insecticidal activity of B.t. proteins or, more generally, in the physiology of B.t. is unclear because of the contradictory results reported.
The role of B.t. proteases in B.t. protein solubilization is described by Chestukhina et al., Biokhimiya 43:857-864 (1978), who carried out dissolution studies with B.t. crystalline proteins and concluded that degradation of B.t. proteins during dissolution was facilitated by the presence of serine proteases, metalloproteases and leucine antipeptidase in the B.t. crystal protein. Similarly, Thurley et al., FEMS Microbiol. Lett. 27:221-225 (1985), reported that a cystein-like crystal-associated protease assisted in the solubilization of a B.t. crystal protein.
A role of B.t. proteases in insecticidal activity is described by Chilcott et al., FEMS Microbiol. Lett. 18:37-41 (1983), who reported that two different proteolytic activities were associated with B.t. crystal protein and that B.t. with reduced proteolytic activity exhibited lower insect toxicity. Bulla, Jr. et al., J. Bacteriol. 130:375-383 (1977), likewise concluded that B.t. crystal proteins have an autolytic activity which apparently involves a sulfhydryl protease that is activated under alkaline conditions (such as found in an insect midgut) and that renders the B.t. protein insecticidal.
An opposite conclusion was reached by Pfannensteil et al., FEMS Microbiol. Lett. 21:39-42 (1984), who reported that B.t. crystal protein treated to reduce the crystal-associated protease activity exhibited no difference in insecticidal activity from the untreated crystal protein (which was from the same B.t. subspecies as that of Chilcott et al.). A similar conclusion was reached by Bibilos et al., Canad. J. Microbiol. 34:740-747 (1988) who described the role of B.t. proteases, primarily neutral metalloproteases, in effecting activation of B.t. protein protoxin to active toxin, but concluded that this is unnecessary, since the same result is accomplished in the insect midgut, presumably by insect-derived proteases.
In contrast to the results reported by Chilcott et al. and Pfannensteil et al., Pearson et al., J. Appl. Bacteriol. 65:195-202 (1988), proposed a negative role for B.t. proteases in the insecticidal activity of B.t. crystal protein. Pearson et al. concluded that more than one type of protease was present in B.t. crystal protein produced by sporulated, lysed B.t. cells and that a decline of insecticidal activity might be associated with proteolytic action.
Some B.t. proteases have been identified, at least in part, in the literature. Li et al., Applied Microbiol. 39:354-361 (1975), describe a partially purified extracellular metalloprotease from B.t. having a molecular mass of about 38 kilodaltons (kDa). Lecadet et al., Eur. J. Biochem. 79:329-338 (1977), describe an extracellular serine protease from B.t. having a molecular mass of about 23 kDa. Stepanov et al., Biochem. Biophys. Res. Comm. 100:1680-1687 (1981), disclose the N-terminal amino acid sequence of a purified extracellular serine protease from B.t. Kunitate et al. , Agric. Biol. Chem. 53:3251-3256 (1989), describe a purified SH-containing serine protease from B.t. whose N-terminal sequence was similar to that reported by Stepanov et al. for their purified protease.
An isolated, cloned B.t. protease gene is described by Lovgren et al., Molecul. Microbiol. 4:2137-2146 (1990), who report the nucleotide sequence of a B.t. derived gene that encodes a neutral metalloprotease, which was found to be toxic when injected into a lepidopteran insect.
The nucleotide sequence of the promoter region of a B.t. protease gene is disclosed by Geiser in PCT International Patent Publication No. WO 92/14826 dated Sep. 3, 1992, of Ciba-Geigy AG, where the promoter is operatively linked with a heterologous gene, such as .beta.-galactosidase.
Although the published literature on the cloning and characterization of B.t.-derived protease genes is limited, much work has been carried out on identifying proteases and protease genes in other Bacillus species, particularly Bacillus subtilis: see Pero et al., "Proteases" in Bacillus subtilis and other Gram-Positive Bacteria, Amer. Soc. Microbiol. , Washington, D.C., 1993, pages 939-952. The cloning of the subtilisin gene of B. subtilis, which encodes an alkaline protease (also called subtilisin or serine protease), is reported by Stahl et al. , J. Bacteriol. 158:411-418 (1984). Another B. subtilis protease gene, one that encodes a neutral metalloprotease, was cloned by Yang et al., J. Bacteriol. 160:15-21 (1984), who used a deleted version of the neutral protease gene to displace the wild-type neutral protease gene in B. subtilis. Proteolytic activity in the mutant was only 20% of the wild-type strain, and another mutant, deleted in both the alkaline protease gene and the neutral protease gene, produced no detectable levels of proteolytic activity. A major extracellular protease of Bacillus cereus was purified by Sidler et al., Biol. Chem. Hoppe-Seyler 367:643-657 (1986), who reported the N-terminal amino acid sequence to be 45% homologous to that of the B. subtilis neutral protease.
U.S. Pat. No. 4,828,994, issued to Fahnestock et al. on May 9, 1989, discloses production of genetically altered strains of Bacillus subtilis, which is rendered incapable of synthesizing the proteolytic enzyme subtilisin by replacing the native chromosomal DNA comprising the subtilisin gene with a DNA sequence comprising a subtilisin gene which has an inactivating DNA sequence inserted therein. The purpose is to insert into the subtilisin gene a functional gene coding for a protein which confers a phenotypic trait, such as resistance to a selected antibiotic to facilitate identification of the altered microorganism and subsequent transfer of the inactivated gene into other bacterial strains. "Subtilisin" as used by Fahnestock et al. refers to the enzyme alkaline serine protease, without regard to the species of Bacillus in which it is produced.
U.S. Pat. No. 4,766,077, issued to Orser et al. on Aug. 23, 1988, relates to a method for modifying ice nucleation bacteria in vitro to confer an ice nucleation deficient phenotype. Modification is accomplished by deletion, substitution, insertion, inversion or transversion of a DNA segment within the gene locus responsible for the ice nucleation phenotype. The mutations are limited to the particular gene locus so that the modified microorganisms are genetically stable and free from random mutations which might adversely affect their competitive fitness. The modified microorganisms are useful for prevention of frost damage to susceptible plant hosts.
SUMMARY OF THE INVENTION
The present invention is based on the discovery, isolation, sequencing and characterization of two protease genes present in B.t. One is an alkaline protease gene generally designated "apr." The other is a neutral protease gene generally designated "npr." The invention also includes genetically disabling the apr and the npr genes to reduce proteolytic activity of the protease encoded by the genes, and using the disabled genes in insecticidal B.t. constructs along with one or more B.t. protein toxin genes. These resulting B.t. constructs are useful for the enhanced production of B.t. toxin protein. The B.t. toxin protein recovered from the fermentation production of these B.t. constructs also exhibits improved stability with respect to its insecticidal activity.
One aspect of the present invention relates to a B.t. protease gene disabled from coding for protease capable of degrading B.t. insecticidal toxic protein, whereby protease expressed by an organism containing the disabled protease gene has reduced proteolytic activity against the toxic protein compared to protease encoded by a counterpart protease gene that has not been disabled.
Another aspect of the present invention relates to a recombinant construct comprising a cloned gene encoding a B.t. insecticidal toxic protein and a disabled B.t. protease gene disabled from coding for protease capable of degrading B.t. insecticidal toxic protein, whereby protease expressed by an organism containing the disabled protease gene has reduced proteolytic activity against the toxic protein compared to protease encoded by a counterpart protease gene that has not been disabled.
Still another aspect of the present invention relates to a method of reducing the proteolytic degradation of a B.t. insecticidal toxic protein in a composition comprising the toxic protein, the method comprising including in the composition a B.t. protease gene disabled from coding for protease capable of degrading the toxic protein, whereby protease expressed by an organism within the composition containing the disabled protease gene has reduced proteolytic activity against the toxic protein compared to protease encoded by a counterpart protease gene that has not been disabled, thereby resulting in reduced proteolytic activity against the toxic protein.





BRIEF DESCRIPTION OF THE DRAWINGS
FIG. 1 consists of FIGS. 1A and 1B and depicts the nucleotide sequence for the apr gene, the B.t. alkaline protease gene (SEQ ID NO:1) of this invention. The deduced amino acid sequence of the Apr alkaline protease protein (SEQ ID NO:2), encoded by the open reading frame extending from nucleotide base positions 225 to 1415 (excluding the. terminal stop codon), is also shown. The restriction endonuclease cleavage site for SstI at nucleotide position 954 within the apr gene is also shown.
FIG. 2 consists of FIGS. 2A through 2C and depicts the nucleotide sequence for the npr gene, the B.t. neutral protease gene (SEQ ID NO:3) of this invention. The deduced amino acid sequence of the Npr neutral protease protein (SEQ ID NO:4), encoded by the open reading frame extending from nucleotide base positions 182 to 1879 (excluding the terminal stop codon), is also shown. The restriction endonuclease cleavage sites for NdeI within the npr gene are also shown.
FIG. 3 is a linear structural map of plasmid pEG1140, a 14.7 kilobase (kb) plasmid containing the cloned apr gene on a 12 kb EcoRI DNA fragment inserted into plasmid vector pUC18, shown by the labeled open segment. The location and orientation of the apr gene are shown by the arrow. Locations of various restriction endonuclease cleavage sites are shown in this Figure and in subsequent Figures.
FIG. 4 is a linear structural map of plasmid pEG1194, a 7.1 kb plasmid that contains the wild type apr gene on a 4.3 kb XbaI-EcoRI DNA fragment subcloned from plasmid pEG1140 (FIG. 3) into plasmid vector pUC18, shown by the labeled open segment. The short line segment marked "1 kb" to the right of the linear structural map in FIG. 4 indicates the approximate size of 1 kilobase for the linear structural maps of FIGS. 3 and 4.
FIG. 5 is a linear structural map of plasmid pEG1203, a 6.2 kb plasmid containing a genetically disabled apr gene designated as the "apr1" allele, on a 3.1 kb XbaI-EcoRI DNA fragment inserted into plasmid vector pUC18, shown by the labeled open segment. The short line segment marked "1 kb" to the right of the linear structural map in FIG. 5 indicates the approximate size of 1 kilobase for the linear structural maps shown in FIGS. 5 and 6.
FIG. 6 is a linear structural map of plasmid pEG1212, a 10.3 kb plasmid that was derived from plasmid pEG491 into which the 3.1 kb XbaI-EcoRI apr1-containing DNA fragment of plasmid pEG1203 (FIG. 5) was subcloned. The open segment of plasmid pEG1212 represents plasmid pEG491, which contains an antibiotic resistance marker gene, chloramphenicol acetyl transferase (Cat), and a temperature sensitive Bacillus replicon (Ts rep).
FIG. 7 is a linear structural map of plasmid pEG1224, a 6.2 kb plasmid that contains a truncated portion of the open reading frame of the npr gene, designated as the "npr1" allele, on a 3.4 kb HindIII DNA fragment inserted into plasmid vector pUC18, shown by the labeled open segment. The location of the npr1 allele is shown. The short line segment marked "1 kb" to the right of the linear structural map in FIG. 7 indicates the approximate size of 1 kilobase in the linear structural maps shown in FIGS. 7 and 8.
In FIGS. 7 through 14, restriction sites are indicated by: H=HindIII, N=NdeI, P=PstI, B=BamHI, A=Asp718, X=XbaI, R=EcoRI, and MCS=multiple cloning site containing sites for Asp718 and PstI.
FIG. 8 is a linear structural map of plasmid pEG1228, an 11.6 kb plasmid that contains another truncated portion of the npr gene, designated as the "npr2" allele, on an 8.0 kb PstI DNA fragment inserted into plasmid vector pUC18, shown by the labeled open segment.
FIG. 9 is a linear structural map of plasmid pEG1233, a 6.6 kb plasmid that contains the npr2 allele on a 3.9 kb BamHI-PstI DNA fragment, subcloned from plasmid pEG1228 (FIG. 8) into plasmid vector pUC18, shown by the labeled open segment. The short line segment marked "1 kb" to the right of the linear structural map in FIG. 9 indicates the approximate size of 1 kilobase in the linear structural maps shown in FIGS. 9 and 10.
FIG. 10 is a linear structural map of plasmid pEG1244, a 10.2 kb plasmid containing the cloned npr gene, with its entire open reading frame, on a 7.5 kb BamHI-XbaI DNA fragment inserted into plasmid vector pUC18, shown by the labeled open segment.
FIG. 11 is a linear structural map of plasmid pEG1235 a 6.4 kb plasmid that contains a genetically disabled version of the npr gene, designated as "npr3", on a 3.7 kb BamHI-PstI DNA fragment, derived from NdeI digestion and religation of plasmid pEG1233 (FIG. 9). The short line segment marked "1 kb" to the right of the linear structural map in FIG. 11 indicates the approximate size of 1 kilobase in the linear structural maps shown in FIGS. 11 and 12.
FIG. 12 is a linear structural map of plasmid pEG1243, a 5.7 kb plasmid containing a 2.8 kb EcoRI DNA fragment from plasmid pNN101 blunt-end ligated into the NdeI site of plasmid vector pUC18, shown by the labeled open segment. The location of a chloramphenicol antibiotic resistance marker gene, chloramphenicol acetyl transferase (Cat), contained on the pNN101-derived segment, is also shown. "R/N" indicates the ligation of EcoRI and NdeI sites, "MCS" indicates a multiple cloning site in the pUC18 DNA segment and "cat" indicates the approximate location of the Cat antibiotic resistance marker gene in the 2.8 kb EcoRI fragment from plasmid pNN101.
FIG. 13 is a linear structural map of plasmid pEG1283, a 4.5 kb plasmid that contains the npr gene within a 1.7 kb XbaI DNA restriction fragment ligated into the XbaI site of plasmid vector pUC18. The 1.7 kb DNA fragment contains only the coding region of the npr gene beginning at nucleotide 182 and ending at nucleotide 1882 as shown in FIG. 2. The short line segment marked "1 kb" to the right of the linear structural map in FIG. 13 indicates the approximate size of 1 kilobase in the linear structural maps shown in FIGS. 13 and 14.
FIG. 14 is of a linear structural map of plasmid pEG1245, a 9.4 kb plasmid that contains the npr3 allele on a 3.7 kb Asp718-PstI DNA fragment subcloned from plasmid pEG1235 (FIG. 11) into the Asp718-PstI sites of plasmid pEG1243 (FIG. 12), shown by the labeled open rectangular segment in FIG. 14.





MICROORGANISM DEPOSITS
To assure the availability of materials to those interested members of the public upon issuance of a patent on the present application, deposits of the microorganism listed in the following Table 1 were made prior to filing the present application with the ARS Patent Collection, Agricultural Research Service Culture Collection (NRRL), 1815 North University Street, Peoria, Ill. 61604.
These microorganism deposits were made under the provisions of the "Budapest Treaty on the International Recognition of the Deposit of Microorganisms for the Purpose of Patent Procedure." All restrictions on the availability to the public of these deposited microorganisms will be irrevocably removed upon issuance of a United States patent based on this application.
TABLE 1______________________________________Cell Recombinant NRRL Accession Date ofType Strain Plasmid Number Deposit______________________________________B. t. EG2371 none NRRL B-18209 23 Apr '87B. t. EG7283 pEG1111 NRRL B-21111 9 Jun '93 (cryET5.sup.+ apr.sup.+)B. t. EG10368 none NRRL B-21125 30 Jun '93E. coli EG7940 pEG1194 (apr.sup.+) NRRL B-21342 11 Oct '94B. t. EG7950 pEG1212 (apr1) NRRL B-21343 11 Oct '94B. t. EG10654 none NRRL B-21344 11 Oct '94E. coli EG7978 pEG1233 (npr2) NRRL B-21345 11 Oct '94E. coli EG11447 pEG1245 (npr3) NRRL B-21346 11 Oct '94B. t. EG10624 none NRRL B-21347 11 Oct '94E. coli EG11466 pEG1283 (npr.sup.+) NRRL B-21358 29 Nov '94______________________________________
DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENTS
The present invention is based on the discovery, identification, isolation, sequencing, characterization, genetic disablement and use of the alkaline protease gene ("apr") (SEQ ID NO:1), and the neutral protease gene ("npr") (SEQ ID NO:3) from B.t. While the presently preferred embodiment of the apr and npr genes, disabled genes based upon them and proteins encoded by them are derived from B.t. strain EG2371, the present invention is not so limited in scope. It is believed, based on the study set forth in Example 17 below that the apr and npr protease genes isolated and sequenced herein are found in a great many other subspecies or varieties of B.t. bacteria.
The present invention covers those gene nucleotide base sequences that encode the amino acid sequences of the indicated proteins, since variations may be made in the nucleotide base sequences which do not affect the amino acid sequence of the gene product, since the degeneracy of the genetic code is well known to those skilled in the art. Moreover, there may be some variations, including deletions, additions, substitutions, inversions or truncations in the coding region of the nucleotide base sequence which allow expression of the respective genes and production of functionally equivalent forms of the insecticidal crystal proteins or proteases as desired. Thus, these types of non-disabling mutants, variants, homologs, recombinant or genetically engineered derivatives thereof, which may be determined without undue experimentation by those of ordinary skill in the art with reference to the present specification, are to. be considered within the scope of the appended claims, since they are fully equivalent to the specifically disclosed and claimed subject matter.
It has been shown that proteins of identical structure and function may be constructed by changing the amino acid sequence, if such changes do not alter the protein secondary structure (Kaiser and Kezdy, Science, 223, pp. 249-255 (1984)). Single amino acid substitutions have been introduced by site-directed mutagenesis at various position of CryIA(a) toxin protein without altering the insecticidal properties of the parent toxin (Ge et al., Proc. Natl. Acad. Sci. USA, 86, pp. 4037-4041 (1989). The present invention includes mutants of the amino acid sequences disclosed herein which have an unaltered protein secondary structure or, if the structure is altered, where the substantially equivalent biological activity is retained in the mutant or derivative.
The foregoing types of non-disabling modification, mutation, variation must be and hereby are distinguished from those modifications to the apr or npr genes that are specifically intended to disable the gene from encoding protease which could adversely affect the beneficial insecticidal toxic crystal proteins used in pest control. Thus, an important aspect of the present invention is the intentional selective disabling modification of the protease genes, as set forth below.
The apr gene encodes the B.t. alkaline protease protein Apr (SEQ ID NO:2). The npr gene encodes the B.t. neutral protease protein Npr (SEQ ID NO:4). The apr gene was cloned from B.t. strain EG2371 using the gene specific oligonucleotide WD168 (SEQ ID NO:5). The npr gene was cloned from B.t. strain EG2371 using the gene specific oligonucleotides WD205 (SEQ ID NO:6) and WD206 (SEQ ID NO:7).
While the identification, isolation and sequencing of the apr and npr genes and their associated Apr and Npr proteins are important first steps in the present invention, the primary value of the present invention is the subsequent discovery that both the apr and npr genes may be disabled (as described in detail in illustrative Examples 2, 3, 11 and 12) to the extent that microorganisms containing them exhibit markedly lower proteolytic activity with respect to counterpart microorganisms containing non-disabled protease genes (as described in detail in illustrative Examples 4 and 13). The result of the reduced proteolytic activity is that the microorganisms containing both insecticidal crystal toxic protein genes and the disabled protease genes are capable of producing higher levels of insecticidal crystal proteins (as described in detail in illustrative Examples 5, 8 and 14) and are capable of producing crystal proteins having increased stability during storage (as described for instance in Examples 9 and 15). The basis for the increased crystal protein production and stability is the fact that proteases degrade proteins. The insecticidal activity of the strains containing the disabled protease genes is not adversely affected and may be enhanced (as described in detail in illustrative Examples 6 and 16).
Based on the foregoing research, the present invention is directed to a B.t. protease gene disabled from coding for protease capable of degrading B.t. insecticidal toxic protein, whereby protease expressed by an organism containing the disabled protease gene has reduced proteolytic activity against the toxic protein compared to protease encoded by a counterpart protease gene that has not been disabled.
There are two preferred protease genes with respect to the present invention, although the concept of the present invention is believed to be applicable to any B.t. protease genes.
One presently preferred protease gene is the apr gene having the nucleotide base sequence illustrated in FIG. 1 and set forth in SEQ ID NO:1, or any equivalent, non-disabled modified mutant, derivative or recombinant thereof capable, when not disabled, of encoding the Apr alkaline protease protein having a deduced amino acid sequence of 397 amino acids as illustrated in FIG. 1 and set forth in SEQ ID NO:2, with a molecular mass of 42,339 Da. The apr gene was cloned, isolated and sequenced as set forth in Example 1 below.
Another presently preferred protease gene is the npr gene having the nucleotide base sequence illustrated in FIG. 2 and set forth in SEQ ID NO:3, or any equivalent, non-disabled modified mutant, derivative or recombinant thereof capable, when not disabled, of encoding the Npr neutral protease protein having a deduced amino acid sequence of 566 amino acids as illustrated in FIG. 2 and set forth in SEQ ID NO:4, with a molecular mass of 60,982 Da. The npr gene was cloned, isolated and sequenced as set forth in Example 10 below.
Once the desired protease genes are identified and characterized, they are modified in a manner to intentionally disable their ability to effectively code for protease. Thus, the disabling modification should render protease produced by the microorganism containing the disabled protease genes less proteolytically active against the desirable toxic proteins produced by the microorganism than a counterpart protease gene that has not been disabled.
The present invention also relates to a method for disabling the apr gene so that strains of B.t. containing the disabled gene produce an increased level of crystal protein. The method comprises cloning and sequencing the apr gene, deleting an essential portion of the cloned apr gene in vitro, yielding the disabled apr1 allele. See illustrative Example 2. A plasmid vector containing the disabled apr1 allele may then be constructed and subsequently used to disable the apr gene in vivo, as explained in illustrative Example 3. Since many varieties of B.t. contain the wild-type apr gene, as demonstated amply in Example 17, the apr gene in all of these varieties can be disabled in vivo as described herein to enhance the production of their respective insecticidal crystal proteins. The plus symbol ("+") following a gene signifies the presence of the wild-type gene. A minus symbol ("-") signifies the absence of a phenotype (e.g., EG10368 Cry.sup.- apr.sup.+ indicates absence of crystal toxin proteins and the presence of the wild-type apr gene).
Similarly to the apr gene, the cloned, disabled npr gene, designated the "npr3" allele, can be used to disable the npr gene in many B.t. strains. A method of doing so includes cloning and sequencing the npr gene, deleting an essential portion of the cloned npr gene in vitro to yield the npr3 allele. See illustrative Example 11. The npr3 allele is capable of disabling the npr gene in vivo, as set forth in illustrative Example 12. Since many varieties of B.t. contain the wild-type npr.sup.+ gene, as demonstrated in Example 17, in all varieties containing the npr.sup.+ gene, the npr.sup.+ gene can be disabled in vivo in the manner described hereinafter.
While Examples 2 and 11 respectively describe specific in vitro deletions of certain portions of the DNA sequences of the apr and npr genes yielding the apr1 and npr3 alleles, respectively, there are a number of other ways in which the apr and npr genes can be effectively disabled in a manner that will reduce their proteolytic activity.
An example of an effective disabling modification would be a single nucleotide deletion occurring at the beginning of either the apr or npr gene that would produce a translational reading frameshift. Such a frameshift would disable the apr or npr gene. Protease production by the gene could be disrupted if the regulatory regions or the coding regions of the protease genes are disrupted.
A goal is to disrupt and eliminate the production of protease so that the B.t. insecticidal crystal protein toxins will not be degraded by the proteases. This results in increased yield of the insecticidal crystal protein toxins and their enhanced stability in the absence of proteases which would otherwise degrade them.
In addition to disabling the apr and npr genes by deleting nucleotides, causing a transitional reading frameshift, disabling proteolytic modifications would also be possible by other techniques including insertions, substitutions, inversions or transversions of nucleotides within the gene's DNA that would effectively prevent the formation of proteases that would degrade the desirable B.t. insecticidal crystal protein toxins.
It is also within the capabilities of one skilled in the art to disable the apr and npr genes by the use of less specific methods. Examples of less specific methods would be the use of chemical mutagens such as hydroxylamine or nitrosoguanidine or the use of radiation mutagens such as gamma radiation or ultraviolet radiation to randomly mutate genes in B.t. strains. Such mutated B.t. strains could, by chance, contain disabled apr and npr genes such that the genes were no longer capable of producing protease proteins. The presence of the desired disabled genes could be detected by routine screening techniques.
Another aspect of the present invention relates to a recombinant construct comprising a gene encoding a B.t. insecticidal toxic protein and a disabled B.t. protease gene disabled from coding for protease capable of degrading B.t. insecticidal toxic protein, whereby protease expressed by an organism containing the disabled protease gene has reduced proteolytic activity against the toxic protein compared to protease encoded by a counterpart protease gene that has not been disabled. Examples 8 and 14 provide illustrative explanations of such constructs involving the disabled apr1 and npr3 genes, respectively.
Moreover, while Examples 8 and 14 demonstrate the utility of the disabled protease genes and the formation of illustrative recombinant constructs containing them with only a few exemplary insecticidal toxic crystal protein genes and their associated toxic proteins, the present invention is not so limited. Thus, for example, substantially all known and, it is believed, even yet to be discovered toxic proteins and/or their genes could be used effectively in recombinant constructs including disabled protease genes. Non-limiting examples of such toxic proteins are CryI-type, CryII-type, CryIII-type, CryIV-type, CryV-type, CryET1, Cry ET4 and CryET5 protein, and mixtures thereof. These are all well documented and available insecticidal toxic proteins, encoded by the following respective genes, all of which are also known and available: cryI-type, cryII-type, cryIII-type, cryIV-type, cryV-type, cryET1, cryET4 and cryET5 genes, and mixtures thereof.
Still another aspect of the present invention relates to a method of reducing the proteolytic degradation of a B.t. insecticidal toxic protein in a composition comprising the toxic protein, the method comprising including in the composition a B.t. protease gene disabled from coding for protease capable of degrading the toxic protein, whereby protease expressed by an organism within the composition containing the disabled protease gene has reduced proteolytic activity against the toxic protein compared to protease encoded by a counterpart protease gene that has not been disabled, thereby resulting in reduced proteolytic activity against the toxic protein.
To perform the foregoing method, one skilled in the art and familiar with this disclosure would merely apply its teachings of how to make and use the disabled protease genes and B.t. constructs as described herein.
Alternatively, one skilled in the art could use the methods of chemical mutagenesis or radiation mutagenesis to randomly mutate B.t. strains and thus by chance disable protease genes. A significant disadvantage of these random mutagenesis methods is that with these methods, genes other than the ones encoding specific protease proteins would also likely be mutated. In contrast to random methods of mutagenesis, the methods described herein are completely specific for disabling only the apr and npr genes and no other genes are affected.
Once the proteolytically modified genes have been created, they can be included in cultures and other formulations typically used to produce B.t. insecticidal crystal protein toxins. The usual production of such toxins would not be affected adversely by the presence of the disabled genes and, to the contrary, due to the reduced proteolytic activity, crystal protein toxin production is enhanced.
The resulting crystal protein toxins can be used as the active ingredient insecticidal formulations or compositions. Likewise, the recombinant constructs or strains of the present invention or even the disabled protease genes of the present invention could be incorporated into any desired insecticidal compostion. Such insecticidal formulations or compositions typically contain agriculturally acceptable carriers or adjuvants in addition to the active ingredient and are prepared and used in a manner well known to those skilled in the art.
The crystal protein toxins may be employed in insecticidal formulations in isolated or purified form, e.g., as the crystal protein itself. Alternatively, they may be present in the recovered fermentation solids, obtained from culturing of a Bacillus strain, e.g., Bacillus thuringiensis or other microorganism host carrying the appropriate gene capable of producing the desired crystal protein. The crystal protein is usually associated with the B.t. bacterium which produced the protein, as an intimate mixture of crystal protein, cell debris and spores, if any, in the recovered fermentation solids. The recovered fermentation solids containing the crystal protein may be dried, if desired, prior to incorporation in the insecticidal formulation. Genetically engineered or transformed B.t. strains or other host microorganisms containing a recombinant plasmid that expresses a cloned toxin gene to produce the desired protein toxin, obtained by recombinant DNA procedures, may also be used.
The formulations or compositions of this invention containing the insecticidal protein as the active component are applied at an insecticidally effective amount which will vary depending on such factors as, for example, the specific insects to be controlled, the specific plant or crop to be treated and the method of applying the insecticidally active compositions.
The insecticide compositions are made by formulating the insecticidally active component with the desired agriculturally acceptable carrier. The formulated compositions may be in the form of a dust or granular material, or a suspension in oil (vegetable or mineral), or water or oil/water emulsions, or as a wettable powder, or in combination with any other carrier material suitable for agricultural application. Suitable agricultural carriers can be solid or liquid and are well known in the art. The term "agriculturally acceptable carrier" covers all adjuvants, e.g., inert components, dispersants, surfactants, tackifiers, binders, etc. that are ordinarily used in insecticide formulation technology; these are well known to those skilled in insecticide formulation.
The formulations containing the insecticidal protein and one or more solid or liquid adjuvants are prepared in known manners, e.g., by homogeneously mixing, blending and/or grinding the insecticidally active protein component with suitable adjuvants using conventional formulation techniques.
The insecticidal compositions of this invention are applied to the environment of the target lepidopteran insect, typically onto the foliage of the plant or crop to be protected, by conventional methods, preferably by spraying. Other application techniques, e.g., dusting, sprinkling, soaking, soil injection, seed coating, seedling coating or spraying, or the like, are also feasible and may be required for insects that cause root or stalk infestation. These application procedures are well known in the art.
The present invention will now be described in greater detail with reference to the following specific, illustrative examples that should not be construed as limiting the scope of the claimed invention.
EXAMPLES
Example 1
Cloning of B.t. apr Gene
An alkaline protease gene (apr) was cloned from a B.t. strain as follows.
B.t. var. kurstaki strain EG2371, a transconjugant B.t. strain that is described in U.S. Pat. No. 5,080,897 issued to Gonzalez, Jr. et al. on Jan. 14, 1992, was selected since it is the active ingredient in a commercial B.t. product, Cutlass bioinsecticide (Ecogen Inc., Langhorne, Pa., the assignee of the present invention).
An oligonucleotide probe designated WD168 was synthesized having the following sequence: 5'-TGG ACA CCA AAT GAT CCA TAT TTT AAT AAT CAA TAT GG-3' (SEQ ID NO:5). This nucleotide sequence was based on an N-terminal amino acid sequence of a purified serine protease reported by Stepanov et al., Biochem. Biophys Res. Comm. 100:1680-1687 (1981).
Oligonucleotide probe WD168 was radioactively labeled with T4 kinase and gamma-.sup.32 P-ATP and used as a probe in Southern blot experiments carried out on total DNA from B.t. strain EG2371. The labeled probe specifically hybridized to a 12 kb EcoRI DNA fragment of B.t. strain EG2371.
A pUC18 plasmid library containing EcoRI DNA fragments of approximately 12 kb from B.t. strain EG2371 was constructed in E. coli. From this library, one E. coli colony, designated EG7299, was identified which specifically hybridized with the labeled WD168 probe.
Analysis of E. coli strain EG7299 showed that it contained a 14.7 kb plasmid, designated pEG1140, comprising the plasmid vector pUC18 plus a WD168-hybridizing fragment of 12 kb. A restriction map of plasmid pEG1140 is shown in FIG. 3.
Using plasmid pEG1140, a 4.3 kb XbaI-EcoRI restriction fragment was subcloned from pEG1140 onto the plasmid vector pUC18 to yield a 7.1 kb plasmid designated pEG1194. The E. coli strain harboring pEG1194 is designated EG7940. A restriction map of plasmid pEG1194 is shown in FIG. 4.
DNA sequencing of plasmid pEG1194 by the dideoxy method of Sanger et al., "DNA sequencing with chain-terminating inhibitors," Proc. Natl. Acad. Sci. USA 74:5463-5467 (1977), revealed that the 4.3 kb XbaI-EcoRI fragment contained an open reading frame that was designated as the "apr" gene. The apr gene was a wild type gene.
The nucleotide sequence of the apr gene (SEQ ID NO:1) is shown in FIG. 1. The apr gene has a coding region extending from nucleotide positions 225 to 1418 (including the TAA stop codon). The restriction site for SstI at nucleotide 954 within the apr gene is also shown in FIG. 1, and this restriction site was utilized in the next Example.
The amino acid sequence of the alkaline protease protein, designated Apr (SEQ ID NO:2), encoded by the apr gene is also shown in FIG. 1. The amino acid sequence of the Apr protein, as deduced from the DNA sequence of the apr gene, contains 397 amino acids. The molecular mass of the deduced Apr protein is 42,339 Da.
Comparisons of the Apr amino acid sequence against other polypeptides in computer databases revealed that it shows 75% identity with the thermitase proteolytic protein of Thermoactinomyces vulgaris, described by Meloun et al., "Complete primary structure of thermitase from Thermoactinomyces vulgaris and its structural features related to the subtilisin-type proteinases," FEBS Letters 183:195-200 (1985), and 41% identity to the subtilisin type alkaline protease protein of B. subtilis, described by Stahl et al., J. Bacteriol. 158:411-418 (1984).
The upstream portion of the apr gene, which includes the gene regulatory region, extending from nucleotide positions 1 to 615 in FIG. 1, and shown in FIG. 4, was discovered to be 99.8% identical to the exoproteinase gene promoter at nucleotide positions 485 to 1100 reported by Geiser in PCT International Patent Application Publication No. WO 92/14826 of Ciba-Geigy AG, published Sep. 3, 1992.
Example 2
In Vitro Deletion Modification of the apr Gene
A genetically disabled version of the apr gene was prepared as follows, by deletion of a portion of the DNA within the coding region of the apr gene.
Plasmid pEG1194, described in Example 1 and shown in FIG. 4, was digested with the restriction endonuclease enzyme SstI which cuts at nucleotide position 954 of the apr gene shown in FIG. 1. After the SstI digestion, approximately 2 .mu.g of the linearized plasmid pEG1194 was treated with 2 units of Bal 31 exonuclease for approximately 3-10 minutes at 30.degree. C. This treatment resulted in the deletion of approximately 600 nucleotides on each side of the original SstI restriction site. Bal 31 exonuclease is an enzyme that digests the ends of both DNA strands, and the size of the deletion is controlled by varying the incubation time, temperature and enzyme concentration.
The Bal 31-treated plasmid strands were then religated with T4 DNA ligase to yield a 6.2 kb plasmid pEG1203. A restriction map of plasmid pEG1203 is shown in FIG. 5. Plasmid pEG1203 is made of plasmid vector pUC18 plus a 3.1 kb XbaI-EcoRI DNA restriction fragment. The 3.1 kb fragment also contains a deleted version of the apr gene which is missing approximately 600 nucleotides on each side of the original SstI restriction site and is called herein a "disabled" gene or DNA construct. This disabled version of the apr gene is a genetically disabled apr gene that was designated as the "apr1" allele. Plasmid pEG1203 containing the apr1 allele was utilized as described in Example 3.
Example 3
In Vivo Deletion Modification of the apr Gene
A genetically disabled version of the apr gene, the apr1 allele, described in Example 2, was introduced into B.t. strain EG2371 via homologous recombination as explained below, to replace the wild-type apr gene with the apr1 allele. The following homologous recombination method is similar to that of Delecluse et al., J. Bacteriol. 173:3374-3381 (1991), was used. Delecluse et al. (1991) describe the disabling of the cytA in B.t. var. israelensis. Delecluse et al. (1991) deleted a portion of the cloned B.t. cytA gene in vitro and subsequently used the in vitro deleted cytA gene to displace, in vivo, the wild-type cytA gene in B.t. var. israelensis by homologous recombination.
Plasmid pEG491 contains a temperature-sensitive Bacillus vector pTV32Ts (described by Youngman et al., in "Regulation of Procaryotic Development, Smith et al., eds., Amer. Soc. Microbiol., Washington, D.C., pp. 65-68 (1989), ligated into the BamHI site of the E. coli plasmid vector pUC18. Plasmid pEG491 is capable of replicating at 30.degree. C. where it confers chloramphenicol resistance to B.t. cells, but it cannot replicate at 42.degree. C.
Plasmid pEG1203 from Example 2, containing the apr1 gene, and plasmid pEG491, having temperature-sensitive replication, were digested with restriction enzymes XbaI and EcoRI. The mixture containing both digested plasmids was ligated with T4 ligase. The mixture was electroporated into B.t. strain EG10368 and chloramphenicol resistant colonies were selected at 30.degree. C. B.t. var. kurstaki strain EG10368 is an apr.sup.+, acrystalliferous (crystal negative or Cry.sup.- strain that does not produce crystal protein) B.t. strain that is readily transformable with plasmids containing various cloned B.t. toxin protein genes. B.t. strain EG10368 is described in U.S. Pat. No. 5,322,687 issued to Donovan et al. on Jun. 21, 1994.
One chloramphenicol resistant B.t. colony, designated EG7950, was studied further. Analysis of EG7950 showed that the strain contained a 10.3 kb plasmid, designated pEG1212, that contained the 3.1 kb XbaI-EcoRI restriction fragment of pEG1203 including the apr1 allele plus the 6.1 kb XbaI-EcoRI fragment of pEG491 including the temperature-sensitive replication. A restriction map of pEG1212 is shown in FIG. 6.
Plasmid pEG1212 was isolated from B.t. strain EG7950 by a standard alkaline cell lysis procedure and was then transformed into B.t. strain EG2371 by electroporation (Macaluso et al., J. Bacteriol. 173:1353-1356 (1991)).
B.t. strain EG2371 transformants harboring plasmid pEG1212 formed chloramphenicol resistant colonies at 30.degree. C. Plasmid pEG1212 contains the apr1 allele and can replicate in B.t. at 30.degree. C. conferring chloramphenicol resistance. pEG1212 cannot replicate in B.t. at 42.degree. C. and can confer chloramphenicol resistance to B.t. at 42.degree. C. only if the plasmid integrates, by homologous recombination, into the chromosomal site of the apr gene. Cells from one chloramphenicol resistant colony were grown at 42.degree. C. in the presence of chloramphenicol. Culturing the cells under these conditions forced plasmid pEG1212 to insert by homologous recombination into the chromosome of the transformant B.t. strain EG2371 at the site of the wild-type apr gene.
The cells were then grown in the absence of antibiotic for several generations in order to allow plasmid pEG1212 to excise out of the chromosome and to become lost from the cultured cells. Cells that had lost plasmid pEG1212 would be sensitive to chloramphenicol.
The dynamics of homologous recombination and excision are such that, in a certain fraction of the chloramphenicol sensitive cells, the apr.sup.+ gene would have been replaced by the apr1 allele. Accordingly, several chloramphenicol sensitive colonies were examined by Southern blot DNA analysis in order to identify colonies in which a 4.3 kb XbaI-EcoRI DNA restriction fragment containing the apr.sup.+ gene was replaced by a 3.1 kb XbaI-EcoRI DNA fragment containing the apr1 allele.
In this procedure, total DNA was extracted from several chloramphenicol sensitive colonies and the DNA was digested with XbaI and with EcoRI. The double digested DNA was electrophoresed through an agarose gel, and the DNA was blotted onto a nitrocellulose filter. The filter was probed with plasmid pEG1194 which had been radioactively labeled. The pEG1194 probe hybridized with a 3.1 kb XbaI-EcoRI DNA fragment from one colony. That colony was designated as B.t. strain EG10587. B.t. strain EG10587 is a derivative of B.t. strain EG2371 in which the apr1 allele has replaced the apr.sup.+ gene and thus contains a genetically disabled, modified apr gene.
Example 4
Proteolytic Activity of B.t. Strains EG2371 (apr.sup.+) and EG10587 (apr1)
B.t. strain EG10587 (apr1) is genetically identical with B.t. strain EG2371 (apr.sup.+) with the exception that B.t. strain EG10587 contains the apr1 allele in place of the apr.sup.+ gene of strain EG2371, as described in Example 3. The respective proteolytic activities of cell cultures of B.t. strains EG10587 and EG2371 were evaluated using the azoalbumin assay method described by Sarath et al., in Proteolytic Enzymes, A Practical Approach, Beynon et al., eds., IRL Press, Oxford, U.K., p. 28, (1989).
Each B.t. strain was grown overnight at 30.degree. C. in DSG sporulation medium. DSG sporulation medium is 0.8% (w/v) Difco nutrient broth, 0.5% (w/v) glucose, 10 mM K.sub.2 HPO.sub.4, 10 mM KH.sub.2 PO.sub.4, 1 mM Ca(NO.sub.3).sub.2, 0.5 MM MgSO.sub.4, 10 mM MnCl.sub.2, 10 mM FeSO.sub.4. Cells from each culture were pelleted by centrifugation, and the resulting supernatants were tested for proteolytic activity by the azoalbumin method. 150 .mu.l of supernatant were added to 250 .mu.l of 2% azoalbumin, 50 mM Tris.HCl pH 8.0 and the mixture was incubated at 37.degree. C. for 30 minutes. 1.0 ml of 10.5% trichloroacetic acid was added, the solution was mixed thoroughly and centrifuged at 8000.times.g for 5 min. 0.6 ml of the supernatant was transferred to a 1 cm cuvette containing 0.7 ml of 1.0 M NaOH. The absorbance at 440 nm was determined spectrophotometrically. The numerical value of the absorbance at 440 nm represents the proteolytic activity of the supernatant.
The proteolytic activity of B.t. strain EG10587, containing the genetically disabled apr1 allele, was determined to be only about 10-20% of the activity measured for B.t. strain EG2371 (apr.sup.+).
The study of the following Example was conducted to determine the effect of the reduced proteolytic activity of the disabled protease gene versus the non-disabled apr gene with respect to the production of proteins by the respective strains.
Example 5
Production of B.t. Proteins by B.t Strains EG2371 (apr.sup.+) and EG10587 (apr1)
B.t. strains EG2371 (apr.sup.+) and EG10587 (apr1), described in Examples 3 and 4, each contains an identical complement of B.t. toxin genes: cryIA(a), cryIA(b), cryIA (c), and cryIIA. The cryI-type genes produce large amounts of CryI-type crystalline protein of about 130 kilodaltons (kDa) and the cryII-type gene produces large amounts of crystalline protein of about 72 kDa.
Crystal protein production was evaluated for these two B.t. strains by growing each strain for four days at a temperature of 30.degree. C. in DSG medium, until the B.t. cells had sporulated and lysed, releasing the crystalline protein and spores.
The lysed B.t. cells, spores and protein crystals were pelleted by centrifugation, and the pellet was suspended in deionized water. The suspension was treated with sodium hydroxide (0.1 N NaOH final concentration) to solubilize the crystalline proteins, and the solubilized proteins were fractionated by SDS polyacrylamide gel electrophoresis. After staining With Coomassie blue, the protein on the gels was quantified by densitometric scanning.
This protein quantification demonstrated that on a volume basis of the culture grown, B.t. strain EG10587 (apr1) produced about 2 to about 2.4 times the amount of CryI-type crystal protein as the isogenic B.t. strain EG2371 (apr.sup.+) produced. This demonstrated that deletion-type disablement of the apr gene from B.t. strain EG2371 results in significantly increased yields of CryI-type crystal protein. Since apr.sup.+ is no longer present in EG10587, having been replaced by apr1 which cannot express protease to degrade the crystal protein, a better yield of CryI-type of proteins is achieved.
Growth of B.t. strains EG2371 (apr.sup.+) and EG10587 (apr1) in other culture media, such as C2 medium, also resulted in more CryI-type protein being produced by B.t. strain EG10587 (apr1), but the increase was not as large. C2 medium is described in W. Donovan et al., Mol. Gen. Genet. 214, pp. 365-372 (1988) and contains 1% glucose, 0.2% peptone, 0.5% NZ amine-A casein hydrolysate (Sheffield Products) 0.2% yeast extract, 15 mM (NH.sub.4).sub.2 SO.sub.4, 23 mM KH.sub.2 PO.sub.4, 27 mM K.sub.2 HPO.sub.4, 1 mM MgSO.sub.4.7H.sub.2 O, 600 mM CaCl.sub.2, 250 mM MnCl.sub.2, 17 mm ZnSO.sub.4.7H.sub.2 O, 17 mM CuSO.sub.4.5H.sub.2 O and 2 mM FeSO.sub.4.7H.sub.2 O.
CryIIA protein production in the two B.t. strains did not appear to be affected by the presence or absence of the apr gene in the B.t. strains, since the amount of CryIIA protein appeared approximately the same for the two B.t strains. This result indicates that the CryIIA protein is not degraded to any significant extent by alkaline protease.
Example 6
Insecticidal Activity of B.t. Proteins from B.t. Strains EG2371 (apr.sup.+) and EG10587 (apr1)
The CryI-type proteins in the B.t. crystal mixtures produced by isogenic B.t. strains EG2371 (apr.sup.+) and EG10587 (apr1), described in Example 5, were evaluated for insecticidal activity against three lepidopteran insect species.
B.t. strains EG2371 and EG10587 were grown at 30.degree. C. in DSG medium for four days until sporulation and cell lysis occurred. The amounts of CryI-type crystal proteins in the sporulated cultures were determined by SDS-PAGE analysis, Coomassie blue staining and densitometer tracing. Cultures of EG2371 and EG10587 contained approximately equal amounts of CryIIA protein. In each culture, the amount of CryIIA protein was approximately 10% of the amount of CryI-type proteins and therefore, CryIIA does not significantly affect insect bioassay results. The sporulated cultures containing known amounts of CryI crystal proteins were diluted in 0.005% Triton.RTM. X-100 (v/v).
PLC.sub.50 values of purified CryI-type crystal protein mixtures were determined against Spodoptera exigua (beet armyworm), Trichoplusia ni (cabbage looper) and Plutella xylostella (diamondback moth) using the bioassay procedures described by Donovan et al. in U.S. Pat. No. 5,322,687 issued Jun. 21, 1994, which is hereby incorporated herein by reference.
The PLC.sub.50 dose is that amount of B.t. protein that killed half of the insects tested, i.e., the median lethal concentration.
Results of these bioassay studies, summarized in Table 2 below, showed no statistical difference in insecticidal activity for the three lepidopteran insect species tested, regardless of whether the CryI-type protein mixture was obtained from an apr.sup.+ B.t. strain or an apr1 B.t. strain.
TABLE 2______________________________________ PLC.sub.50 (ng CryI-type protein/well)B. t. strain S. exigua T. ni P. xylostella______________________________________EG2371 (apr.sup.+) 52 (43-61)* 10 (8.9-12) 4.8 (4.3-5.3)EG10587 (apr1) 69 (56-85) 13 (11-15) 4.3 (3.9-4.7)______________________________________ *range in parentheses indicates 95% confidence level.
Example 7
Construction of Crystal-negative B.t. Strain Containing the apr1 Allele
A derivative of B.t. strain EG10368, described in Example 3 above, was constructed in which the alkaline protease gene apr was genetically disabled by replacement with a modified apr gene, i.e., the apr1 allele. This was accomplished by utilizing plasmid pEG1212 (apr1), described in Example 3, which was electroporated into B.t. strain EG10368 using conventional techniques to yield chloramphenicol resistant B.t. colonies at 30.degree. C. One chloramphenicol resistant colony was grown at a temperature of 42.degree. C. to force the integration, by homologous recombination, of plasmid pEG1212 (apr1) into the chromosome of B.t. strain EG10368 at the site of the apr gene. This procedure was essentially the same as that described in Example 3. Subsequently, the B.t. cells were grown for several generations in the absence of antibiotic, and chloramphenicol sensitive colonies were identified.
Total DNA was isolated from several chloramphenicol sensitive colonies, and the DNA from each colony was digested with XbaI and EcoRI. The double digested DNA was electrophoresed through an agarose gel and blotted onto a nitrocellulose filter. The filter was probed with plasmid pEG1194 (apr.sup.+), described in Example 1, that had been radioactively labeled.
The labeled plasmid pEG1194 (apr.sup.+) hybridized to a 3.1 kb XbaI-EcoRI fragment from total DNA of one chloramphenicol sensitive B.t. colony. This colony, designated as B.t. strain EG10654, contained the apr1 allele in place of the apr.sup.+ gene originally present in the parent strain B.t. strain EG10368. B.t. strain EG10654 is genetically disabled with respect to the apr gene and was used in the next Example to construct recombinant B.t. strains containing cloned B.t. toxin genes.
Example 8
Production of B.t. CryIIB Protein, CryIIIB3 Protein and CryET5 Protein in apr1 B.t. Strain Constructs
Three recombinant B.t. strain constructs were prepared in which the alkaline protease gene apr had been genetically disabled and replaced with apr1, to demonstrate enhanced production of three B.t. crystal proteins, CryIIB, CryIIIB3 and CryET5, in the apr1 B.t. strains.
B.t. strain EG10654, an acrystalliferous B.t. strain described in Example 7, was employed as a host strain since it contained the apr1 allele, a genetically disabled, modified version of the apr gene. For comparison, the isogenic B.t. strain EG10368 (Cry.sup.- apr.sup.+), also described in Example 7, was used as a host strain, since it contained the apr.sup.+ gene.
CryIIB is a lepidopteran-toxic B.t. protein, related to CryIIA, that is made by the cryIIB B.t. toxin gene. Both the cryIIB gene and CryIIB protein are described in U.S. Pat. No. 5,073,632 issued to Donovan on Dec. 17, 1991, which is hereby incorporated by reference. CryIIIB3 is a coleopteran-toxic B.t. protein that is made by the cryIIIB3 B.t. toxin gene. The cryIIIB3 gene and CryIIIB3 protein are described in U.S. Pat. No. 5,264,364 issued to Donovan et al. on Nov. 23, 1993 (wherein the cryIIIB3 gene is referred to as the cryIIIC(b) gene), which is hereby incorporated herein by reference. CryET5 is a CryI-type lepidopteran-toxic B.t. protein that is made by the cryET5 B.t. toxin gene. The cryET5 gene and CryET5 protein are described in U.S. Pat. No. 5,322,687 issued to Donovan et al. on Jun. 21, 1994.
The cloned cryIIB gene, carried on recombinant plasmid pEG259 (described by Dankocsik et al., Molec. Microbiol. 4:2087-2094 (1990)), was introduced into the isogenic B.t. strains EG10654 (apr1) and EG10368 (apr.sup.+) by conventional recombinant DNA techniques to yield transformant B.t. strains EG11437 (cryIIB.sup.+ apr1) and EG11442 (cryIIB.sup.+ apr.sup.+), respectively. The cloned cryIIIB3 gene, carried on recombinant plasmid pEG272 (described by Donovan et al. in U.S. Pat. No. 5,264,364) was likewise introduced into the isogenic B.t. strains EG10654 (apr1) and EG10368 (apr.sup.+) by conventional recombinant DNA techniques to yield transformant B.t. strains EG11438 (cryIIIB3.sup.+ apr1) and EG11441 (cryIIIB3.sup.+ apr.sup.+), respectively.
The cloned cryET5 gene, carried on recombinant plasmid pEG1111 (described by Donovan et al. in U.S. Pat. No. 5,322,687) was likewise introduced into the isogenic B.t. strains EG10654 (apr1) and EG10368 (apr.sup.+) to yield transformant B.t. strains EG11435 (cryET5.sup.+ apr1) and EG7283 (cryET5.sup.+ apr.sup.+), respectively.
For evaluation of the respective B.t. crystal protein production by each of these recombinant B.t. strains, all four were grown at a temperature of 30.degree. C. in DSG medium for 3-4 days, until sporulation of the B.t. cells had occurred and crystalline B.t. protein was produced.
Using the same procedure as described in Example 5, the quantity (weight per volume) of B.t. protein produced by each of the B.t. cultures was determined by SDS-PAGE analysis, Coomassie blue staining and densitometer measurements. The results of these analyses indicated that, in two of three cases, the apr-disabled B.t. strains, i.e., the strains containing the apr1 allele, produced significantly more B.t. protein than the B.t. strains containing the apr gene.
For the CryIIB protein producing strains, B.t. strain EG11437 (cryIIB.sup.+ apr1) produced about 1.4 to about 5 times the amount of B.t. protein than B.t. strain EG11442 (cryIIB.sup.+ apr.sup.+) in which the apr gene had not been disabled.
For the CryET5 protein producing strains, B.t. strain EG11435 (cryET5.sup.+ apr1) produced about 1.5 to about 5 times the amount of B.t. protein than B.t. strain EG7283 (cryET5.sup.+ apr.sup.+) in which the apr gene had not been disabled.
For the CryIIIB3 protein producing strains, B.t. strain EG11438 (cryIIIB3.sup.+ apr1) produced a similar amount of CryIIIB3 protein as did B.t. strain EG11441 (cryIIIB3.sup.+ apr.sup.w +) in which the apr gene had not been disabled.
Example 9
Storage Stability of B.t. Proteins from apr1 B.t. Strain Constructs
The storage stability of the B.t. crystal proteins produced by the six recombinant B.t. strain constructs described in Example 8 was evaluated, over a seven-day period after being stored at a temperature of about 22.degree. C. Sporulated cultures of the six recombinant B.t. strains, containing either the CryET5 crystal protein (B.t. strains EG11435 (cryET5.sup.+ apr1) and EG7283 (cryET5.sup.+ apr.sup.+)), the CryIIB protein (B.t. strains EG11437 (cryIIB.sup.+ apr1) and EG11442 (cryIIIB.sup.+ apr.sup.+)) or the CryIIIB3 protein (B.t. strains EG11438 (cryIIIB3.sup.+ apr1) and EG11441 (cryIIIB3.sup.+ apr.sup.+)) were analyzed at two time points, immediately after recovery of the sporulated cultures and after seven days. The amount of B.t. crystal protein in each of the samples was quantified by SDS-PAGE analysis, Coomassie blue staining and densitometer analysis.
Results of the procedures showed that the lepidopteran toxic CryET5 protein (of about 130 kDa) and the lepidopteran toxic CryIIB protein (of about 70 kDa) were equally stable, regardless of whether produced by an apr.sup.+ B.t. strain or an apr1 B.t. strain. This demonstrated that there were no adverse affects on stability of such proteins produced in greater amounts by the apr1 allele compared to the amount produced by the apr.sup.+ gene.
The coleopteran toxic CryIIIB3 protein (of about 73 kDa) produced by the apr1 B.t. strain EG11438 (cryIIIB3.sup.+ apr1) was stable over the seven-day period, but CryIIIB3 protein produced by the apr.sup.+ B.t. strain EG11441 (cryIIIB3.sup.+ apr.sup.+) was degraded to a lower molecular weight form of about 70 kDa. This result demonstrated that genetic disabling of the apr gene improved the storage stability of the full-length CryIIIB3 protein.
Example 10
Cloning of B.t. npr Gene
A neutral protease gene (npr) was cloned from the same B.t. var. kurstaki strain EG2371 used in other Examples above.
In initial unsuccessful attempts to clone a neutral protease gene in B.t. strain EG2371, oligonucleotide probes were designed based on the published sequence of the B. subtilis neutral protease gene, disclosed by Yang et al., J. Bacteriol. 160:15-21 (1984). The use of two B. subtilis neutral protease gene specific oligonucleotides as probes led to the cloning, subcloning and DNA sequencing of several DNA restriction fragments of B.t. strain EG2371. Although the cloned restriction fragments specifically hybridized to the oligonucleotide probes, extensive analysis of the cloned DNA fragments that hybridized to the probes failed to yield any evidence of a neutral protease gene in these cloned DNA fragments from B.t. strain EG2371.
Despite this lack of success in these initial attempts, a renewed effort was undertaken to clone a neutral protease gene isolated from B.t. strain EG2371 using different oligonucleotide probes, based on the amino acid. sequence of a neutral protease protein from Bacillus cereus, as reported by Sidler et al., Biol. Chem. Hoppe-Seyler 367:643-657 (1986).
One oligonucleotide probe designated WD205 was synthesized having the following sequence: 5'-GAA ATT GAT GTA ATT GGA CAT GAA TTA ACA CAT GCA GT-3' (SEQ ID NO:6). A second oligonucleotide probe designated WD206 was synthesized having the following sequence: 5'-ATG GTA TAT GGA GAA GGA GAT GGA GTA ACA TTT AC-3' (SEQ ID NO:7).
Oligonucleotide probes WD205 and WD206 were radioactively labeled with T4 kinase and gamma-.sup.32 P-ATP and used as probes in Southern blot experiments carried out on total DNA from B.t. strain EG2371. Both labeled probes specifically hybridized to two DNA fragments of B.t. strain EG2371: a 3.5 kb (approximate size) HindIII DNA restriction fragment and a 3.4 kb (approximate size) EcoRI DNA restriction fragment.
A pUC18 plasmid library containing HindIII DNA fragments of approximately 3-4 kb from B.t. strain EG2371 was constructed in E. coli. From this library, one E. coli colony, designated EG7971, was identified which specifically hybridized with the labeled WD206 probe.
Analysis of E. coli strain EG7971 showed that it contained a 6.2 kb plasmid, designated pEG1224, which consisted of the plasmid vector pUC18 plus a WD206hybridizing HindIII fragment of 3.4 kb. A restriction map of plasmid pEG1224 is shown in FIG. 7.
Dideoxy DNA sequencing of plasmid pEG1224 revealed that the 3.4 kb HindIII fragment contained a truncated open reading frame, and this was designated as npr1. As shown in FIG. 7, the npr1 open reading frame is truncated by the HindIII restriction site of plasmid pEG1224.
The effort to clone the complete npr open reading frame included the following steps. Plasmid pEG1224 was radioactively labeled for use as a probe in Southern blot experiments carried out on total DNA from B.t. strain EG2371. The labeled probe specifically hybridized to a unique PstI DNA restriction fragment of approximately 8.0 kb from the B.t. strain EG2371 total DNA.
A pUC18 plasmid library containing PStI DNA fragments of about 8 kb from B.t. strain EG2371 was constructed in E. coli. From this library, one E. coli colony, designated EG7973, was identified which specifically hybridized with the purified 3.4 kb HindIII npr1 fragment of plasmid pEG1224, whose restriction map is shown in FIG. 7.
Analysis of E. coli. strain EG7973 showed that it contained an 11.6 kb plasmid, designated pEG1228, which was made of the plasmid vector pUC18 plus an 8.0 kb PstI DNA restriction fragment that specifically hybridized to the 3.4 kb HindIII npr1 probe. A restriction map of plasmid pEG1228 is shown in FIG. 8.
Dideoxy DNA sequencing of plasmid pEG1228 revealed that the 8.0 kb PstI fragment contained a truncated open reading frame which was designated npr2. As shown in FIG. 8, the npr2 open reading frame is truncated by the PstI restriction site of plasmid pEG1228.
Using plasmid pEG1228, a 3.9 kb BamHI-PstI restriction fragment containing the npr2 open reading frame was subcloned from pEG1228 onto the plasmid vector pUC18 to yield a 6.6 kb plasmid designated pEG1233. A restriction map of plasmid pEG1233 is shown in FIG. 9.
The complete npr gene was finally cloned by the following procedure. The 3.9 kb BamHI-PstI npr2 fragment of plasmid pEG1233, shown in FIG. 9, was labeled for use as a probe in Southern blot experiments carried out on total DNA from B.t. strain EG2371. The labeled probe specifically hybridized to a BamHI-XbaI DNA restriction fragment of approximately 7.5 kb from B.t. strain EG2371 total DNA.
A pUC18 plasmid library containing BamHI-XbaI DNA fragments of about 7.5 kb from B.t. strain EG2371 was constructed in E. coli. From repeated screening of this library, one E. coli colony, designated EG7993, was eventually identified which specifically hybridized with the 3.9 kb BamHI-PstI npr2 fragment of plasmid pEG1233.
Analysis of E. coli. strain EG7993 showed that it contained a 10.2 kb plasmid, designated pEG1244, which comprises the plasmid vector pUC18 plus a 7.5 kb BamHI-XbaI DNA restriction fragment that specifically hybridized to the 3.9 kb BamHI-PstI npr2 fragment of plasmid pEG1233. A restriction map of plasmid pEG1244 is shown in FIG. 10.
DNA sequencing of portions of plasmids pEG1244 and pEG1233 confirmed that the 7.5 kb BamHI-XbaI DNA fragment of plasmid pEC1244 contained the complete open reading frame of the full-length neutral protease gene, npr. E. coli strain EG7993, containing plasmid pEG1244 whose restriction map is shown in FIG. 10, grew very slowly when cultured, and this suggested that the presence of the cloned, full-length npr gene, or its Npr protein product was toxic to E. coli.
The nucleotide sequence of the npr gene (SEQ ID NO:3) is shown in FIG. 2. The npr gene has a coding region extending from nucleotide positions 182 to 1882 (including the TAA stop codon). NdeI restriction sites within the npr gene at nucleotides 744, 750 and 1053 are also shown in FIG. 2. Use of these restriction sites is discussed in subsequent Examples.
The amino acid sequence of the neutral protease protein, designated Npr (SEQ ID NO: 4), encoded by the npr gene is also shown in FIG. 2. The amino acid sequence of the Npr protein, as deduced from the DNA sequence of the npr gene, contains 566 amino acids. The molecular mass of the deduced Npr protein is 60,982 Da.
Comparisons of the Npr amino acid sequence against other polypeptides in computer databases revealed that a portion of the Npr protein shows 98.7% identity with the 317 amino acids of the neutral protease protein of B. cereus, reported by Sidler et al. , Biol. Chem. Hoppe-Seyler 367:643-657 (1986). The Npr protein showed no amino acid sequence identity with a previously-reported B.t. protease, the protease of B.t. var. alesti described by Lovgren et al., Molec. Microbiol. 4:2137-2146 (1990) and little identity (52% in the C-terminal moiety) with the B. subtilis neutral protease protein described by Yang et al., J. Bacteriol. 160:15-21 (1984). The Npr neutral protease protein (SEQ ID NO:4) shows no amino acid sequence identity with the Apr alkaline protease protein (SEQ ID NO:2) of this invention, described in Example 1.
To obtain a full length npr gene that was not toxic to E. coli cells, the npr regulatory sequences were eliminated by use of the polymerase chain reaction (PCR). Elimination of the npr regulatory sequences was accomplished in the following manner.
Two oligonucleotides, designated WD280 and WD281, homologous to the beginning and end, respectively, of the npr coding region were synthesized. WD280 has the nucleotide sequence 5'-TTT CTA GAT GAA AAA GAA GAG TTT AGC AT-3' (SEQ ID NO:8) and, starting with the eighth nucleotide, it is homologous to the beginning of the npr DNA sequence from nucleotides 182 to 203 (FIG. 2). WD281 has the nucleotide sequence 5'-TTT CTA GAT TAG TTA ATA CCA ACA GCA CTA-3' (SEQ ID NO:9) and, starting with the ninth nucleotide, it is complementary to the end of the npr DNA sequence from nucleotides 1882 to 1861 (FIG. 2). Each oligonucleotide contains an XbaI DNA restriction site (5'-TCTAGA-3') at its 5' end. Oligonucleotides WD280 and WD281, and plasmid pEG1244 were used together in a PCR reaction using the GeneAmp PCR Reagent Kit according to the directions of the manufacturer (Perkin Elmer Cetus, Norwalk, Conn. The PCR reaction generated a DNA fragment having a size of 1.7 kb. The 1.7 kb fragment was digested with DNA restriction enzyme XbaI, and was ligated into the XbaI site of plasmid vector pUC18 yielding a 4.5 kb plasmid designated pEG1283. A restriction map of pEG1283 is shown in FIG. 13.
Plasmid pEG1283 comprises the pUC18 plasmid containing an inserted 1.7 kb XbaI DNA restriction fragment. The 1.7 kb DNA fragment contains only the coding region of the npr gene beginning at nucleotide 182 and ending at nucleotide 1882 of FIG. 2. The E. coli strain harboring pEG1283 is designated EG11466. EG11466 cells were found to grow well in LB medium containing 50 .mu.g/ml ampicillin.
Example 11
In Vitro Deletion of the npr Gene
A genetically disabled version of the npr gene was prepared as follows, by deletion of a portion of the DNA within the coding region of npr2, the truncated npr allele described in Example 10.
Plasmid pEG1233, described in Example 10 and shown in FIG. 9, was digested with the restriction endonuclease enzyme NdeI, which cuts three times within npr2, the truncated npr gene.
The NdeI-digested plasmid pEG1233 was then religated with T4 DNA ligase, and the ligation mixture was transformed into E. coli. One ampicillin resistant E. coli transformant colony was designated as E. coli strain EG7980 and was identified as containing a 6.4 kb plasmid, designated as pEG1235, made of the pUC18 plasmid vector plus a 3.7 kb BamHI-PstI DNA restriction fragment. A restriction map of plasmid pEG1235 is shown in FIG. 11.
Plasmid pEG1235 contains a disabled version of the npr gene, actually being a disabled version of the npr2 allele, missing approximately 300 base pairs from the middle of the allele. The modified npr allele in plasmid pEG1235 was designated npr3. The deleted 300 bp segment constitutes the portion of the npr2 truncated gene fragment which was eliminated during NdeI digestion of plasmid pEG1233 (npr2) and its subsequent religation to yield plasmid pEG1235. The respective restriction maps are shown in FIGS. 9 and 11.
Example 12
In Vivo Deletion of the npr Gene
A genetically disabled version of the npr gene, the modified npr3 allele that is described in Example 11, was introduced into a B.t. strain (EG10368, described above in Example 3) via homologous recombination as described below, to replace a wild-type npr gene with the npr3 allele. The homologous recombination method employed was similar, in many respects, to that utilized in Example 3.
An integration vector was constructed as follows, to permit in vivo deletion of the npr gene in B.t. A 2.8 kb EcoRI fragment containing a chloramphenicol resistance determinant (a marker gene) from plasmid pNN101, described by Norton et al., Plasmid 13:211-214 (1985), was blunt-end ligated into the NdeI restriction site of plasmid pUC18, resulting in a 5.7 kb plasmid designated pEG1243. A restriction map of plasmid pEG1243 is shown in FIG. 12. Plasmid pEG1243 is capable of replicating in E. coli, conferring ampicillin and chloramphenicol resistance, but cannot replicate in B.t.
Using plasmid pEG1235 described in Example 10, having the restriction map shown in FIG. 11, a 3.7 kb Asp718-PstI DNA fragment was subcloned from plasmid pEG1235 into the unique Asp718-PstI site of plasmid pEG1243, resulting in a 9.4 kb plasmid designated pEG1245. A restriction map of plasmid pEG1245 is shown in FIG. 14. In FIG. 14, the open rectangular segment indicates plasmid pEG1243. Plasmid pEG1245 contains the npr3 allele and is able to replicate in E. coli, conferring ampicillin and chloramphenicol resistance, but cannot replicate in B.t. Plasmid pEC1245 can confer chloramphenicol resistance to B.t. only if it integrates, by homologous recombination, into the chromosomal site of the npr gene.
Plasmid pEG1245 was transformed by standard methods into E. coli strain GM2163 (Macaluso et al., 1991) yielding strain EG11447. Plasmid pEG1245 was subsequently isolated from EG11447 and the plasmid was used in the experiments described below.
Approximately 10 .mu.g of plasmid pEG1245 was electroporated by conventional techniques into cells of B.t. var. kurstaki strain EG10368 (Cry.sup.- npr.sup.+), described in Example 7. The electroporated B.t. cells were then spread into LB agar plates containing chloramphenicol and incubated for two days at a temperature of 30.degree. C. After this time, fifty chloramphenicol resistant B.t. colonies appeared on the plates.
Southern blot analyses of DNA extracted from six chloramphenicol resistant B.t. colonies, using pEG1245 as a hybridization probe, showed that the DNA from each of the six colonies contained both the wild-type npr.sup.+ gene and the modified npr3 allele. This result indicated that for each of the six B.t. colonies examined, plasmid pEG1245 had integrated into the B.t. chromosome by homologous recombination at the site of the npr.sup.+ gene.
Three of these chloramphenicol resistant B.t. colonies were grown separately in LB nutrient medium at a temperature of 30.degree. C. in the absence of chloramphenicol. After extended growth for about thirty generations, chloramphenicol-sensitive B.t. colonies were identified.
Total DNA was prepared from sixteen chloramphenicol sensitive colonies, and the DNA was analyzed by Southern blot analysis using radioactively labeled plasmid pEG1245 as a hybridization probe. The Southern blot analysis demonstrated that in four of the sixteen chloramphenicol sensitive B.t. colonies, the npr.sup.+ gene had been replaced by the npr3 allele. The four strains containing the npr3 allele contained pEG1245-hybridizing DNA restriction fragments that were approximately 300 nucleotides shorter than the pEG1245-hybridizing DNA restriction fragments from the npr.sup.+ strains.
One of the four colonies containing the npr3 allele was designated B.t. strain EG10624 and was utilized in subsequent Examples. B.t. strain EG10624 is a derivative of B.t. strain EG10368 in which the npr3 allele has replaced the npr.sup.+ gene and thus contains a genetically disabled, modified (deleted) and truncated npr gene.
The remaining twelve chloramphenicol sensitive B.t. colonies contained the npr.sup.+ gene. The npr3 allele had apparently been excised during the multiple generation culturing.
Example 13
Proteolytic Activity of B.t. Strains EG10368 (npr.sup.+) and EG10624 (npr3)
B.t. strain EG10624 (npr3) is genetically identical with B.t. strain EG10368 (Cry.sup.- npr.sup.+) with the exception that B.t. strain EG10624 contains the npr3 allele in place of the npr.sup.+ gene of strain EG10368, as described in Example 12. The respective proteolytic activities of cell cultures of B.t. strains EG10624 and EG10368 were evaluated using the azoalbumin assay method described by Sarath et al., in Proteolytic Enzymes, A Practical Approach, Beynon et al., eds., IRL Press, Oxford, U.K., p. 28 (1989).
Each B.t. strain was grown overnight at 30.degree. C. in DSG sporulation medium. Cells from each culture were pelleted by centrifugation, and the resulting supernatants were tested for proteolytic activity as described in Example 4.
The proteolytic activity of B.t. strain EG10624 (npr3) containing a genetically disabled npr gene, was determined to be only about 12-25% of the activity measured for B.t. strain EG10368 (npr.sup.+), containing the wild-type npr gene.
Example 14
Production of B.t. CryET5 Protein, CryIIB Protein and CrvIIIB3 Protein in npr3 B.t. Strain Constructs
Three recombinant B.t. strain constructs were prepared in which the neutral protease gene npr had been genetically disabled, to see if there would be enhanced production of three B.t. crystal proteins, CryET5, CryIIB and CryIIIB3, in the npr3 B.t. strains.
B.t. strain EG10624, an acrystalliferous B.t. strain described in Examples 12 and 13, was employed as the host strain, since it contained the npr3 allele, a genetically disabled, truncated and modified version of the npr gene. For comparison, the isogenic B.t. strain EG10368 (Cry.sup.- npr.sup.+), also described in the previous two Examples, was used as a host strain, since it contained the npr.sup.+ gene.
The lepidopteran-toxic CryIIB and CryET5 proteins and their respective cryIIB and cryET5 genes were the same as described previously, in connection with Example 8.
CryIIIB3 is a coleopteran-toxic B.t. protein that is made by the cryIIIB3 B.t. toxin gene as discussed above and as described in U.S. Pat. No. 5,264,364 issued to Donovan et al. on Nov. 23, 1993 (where the cryIIIB3 gene is referred to as the cryIIIC(b) gene).
The cloned cryET5 gene, carried on recombinant plasmid pEG1111 (described by Donovan et al. in U.S. Pat. No. 5,322,687) was introduced into the isogenic B.t. strains EG10624 (npr3) and EG10368 (npr.sup.+) (EG10368 is both apr.sup.+ and npr.sup.+) by conventional recombinant DNA techniques to yield transformant B.t. strains EG7995 (cryET5.sup.+ npr3) and EG7283 (cryET5.sup.+ npr.sup.+), respectively.
The cloned cryIIb gene, carried on recombinant plasmid pEG259 (described by Dankocsik et al., Molec. Microbiol. 4:2087-2094 (1990)) was likewise introduced into the isogenic B.t. strains EG10624 (npr3) and EG10368 (npr.sup.+) to yield transformant B.t. strains EG7998 (cryIIB.sup.+ npr3) and EG11442 (cryIIB.sup.+ npr.sup.+), respectively.
The cloned cryIIIB3 gene, carried on recombinant plasmid pEG272 (described by Donovan et al. in U.S. Pat. No. 5,264,364) was likewise introduced into the isogenic B.t. strains EG10624 (npr3) and EG10368 (npr.sup.+) to yield transformant B.t. strains EG7994 (cryIIIB3.sup.+ npr3) and EG11441 (cryIIIB3.sup.+ npr.sup.+), respectively.
For evaluation of the respective B.t. crystal protein production by each of these recombinant B.t. strains, all six were grown at a temperature of 30.degree. C. in DSG sporulation medium for 3-4 days, until sporulation of the B.t. cells had occurred and crystalline B.t. protein was produced.
Using the same procedure as described in Example 5, the quantity (weight per volume) of B.t. protein produced by each of the B.t. cultures was determined by SDS-PAGE analysis, Coomassie blue staining and densitometer measurements. The results of this analysis indicated that the npr-disabled B.t. strains, i.e., containing the npr3 allele, produced much more B.t. protein than the npr-containing B.t. strains.
For the CryET5 protein producing strains, B.t. strain EG7995 (cryET5.sup.+ npr3) produced about 2 to about 3 times more B.t. protein than did B.t. strain EG7283 (cryET5.sup.+ npr.sup.+) in which the npr gene had not been disabled.
For the CryIIB protein producing strains, B.t. strain EG7998 (cryIIB.sup.+ npr3) produced about 1.5 to about 3 times more B.t. protein than did B.t. strain EG11442 (cryIIB.sup.+ npr.sup.+) in which the npr gene had not been disabled.
For the CryIIIB3 protein producing strains, B.t. strain EG7994 (cryIIIB3.sup.+ npr3) produced about 1.3 to about 1.6 times more B.t. protein than did B.t. strain EG11441 (cryIIIB3.sup.+ npr.sup.+) in which the npr gene had not been disabled.
Example 15
Storage Stability of B.t. Proteins from npr3 B.t. Strain Constructs
The storage stability of the B.t. crystal proteins produced by the six recombinant B.t. strain constructs described in Example 15 was evaluated, over a seven day period after being stored at a temperature of about 22.degree. C.
Sporulated cultures of the six recombinant B.t. strains, containing CryET5 crystal protein (B.t. strains EG7995 (cryET5.sup.+ npr3) and EG7283 (cryET5.sup.+ npr)) or CryIIB protein (B.t. strains EG7998 (cryIIB.sup.+ npr3) and EG11442 (cryIIB.sup.+ npr.sup.+)) or CryIIIB3 protein (B.t. strains EG7994 (cryIIIB3.sup.+ npr3) and EG11441 (cryIIIB3.sup.+ npr.sup.+)), were analyzed at two time points, immediately after recovery of the sporulated cultures and after seven days. The amount of B.t. crystal protein in each of the samples was quantified by SDS-PAGE analysis, Coomassie blue staining and densitometer analysis.
Results of the procedures showed that the lepidopteran-toxic CryET5 protein (of about 130 kDa) and the coleopteran-toxic CryIIIB3 protein (of about 70 kDa) were equally stable, regardless of whether produced by an npr.sup.+ B.t. strain or an npr3 B.t. strain.
For the lepidopteran-toxic CryIIB protein (of about 70 kDa) the situation was remarkably different. CryIIB protein produced by npr3 B.t. strain EG7998 (cryIIB.sup.+ npr3) was stable over the seven day period, but CryIIB protein produced by npr.sup.+ B.t. strain EG11442 (cryIIB.sup.+ npr.sup.+) was completely degraded during the storage at about 22.degree. C. over the seven day period. Genetic disabling of the neutral protease gene npr thus has a highly positive impact on the storage stability of CryIIB protein produced by such npr3 B.t. strains.
Example 16
Insecticidal Activity of B.t. Protein from B.t. Strains EG7283 (npr.sup.+) and EG7995 (npr3)
The CryET5 protein produced respectively by isogenic B.t. strains EG7283 (npr.sup.+) and EG7995 (npr3), described in Example 15, was evaluated for insecticidal activity against two lepidopteran insect species.
B.t. strains EG7283 (npr.sup.+) and EG7995 (npr3) were grown at 30.degree. C. in DSG medium for four days until sporulation and cell lysis occurred. The amounts of CryET5 crystal proteins in the sporulated cultures were determined by SDS-PAGE analysis, Coomassie blue staining and densitometer tracing. The sporulated cultures containing known amounts of CryET5 crystal proteins were diluted in 0.005% Triton X 100.RTM. (v/v).
PLC.sub.50 values of the CryET5 protein contained in sporulated cultures of the two isogenic B.t. strains EG7283 (npr.sup.+) and EG7995 (npr3) were determined against Ostrinia nubilalis (European corn borer) and Trichoplusia ni (cabbage looper). Bioassay procedures similar to those described for Example 6 were employed.
Results of these bioassay studies, summarized in Table 3 below, showed no statistical difference in insecticidal activity for the two inspect species tested, regardless of whether the CryET5 protein was obtained from an npr.sup.+ B.t. strain or an npr3 B.t. strain.
TABLE 3______________________________________ PLC.sub.50 (ng CryET5/well)B. t. strain O. nubilalis T. ni______________________________________EG7283 (npr.sup.+) 85 (66-110)* 34 (27-43)EG7995 (npr3) 112 (81-164) 22 (18-27)______________________________________ *Range in parentheses indicates 95% confidence level.
Example 17
Widespread Occurrence of the apr and npr Genes in B.t. Strains
The apr and npr genes were cloned from B.t. strain EG2371, a variety kurstaki strain. To determine whether the apr and npr genes were present in other varieties of B.t., the following experiment was conducted. Sixteen varieties of B.t. were selected from Ecogen Inc.'s strain collection: kurstaki, aizawa, thuringiensis, kenya, pakistani, morrisoni, israelensis, entomocidus, tolworthi, dendrolimus, sotto, alesti, subtoxicus, toumanoffi, galleriae and japonensis. Total DNA was extracted from each of the sixteen strains by standard procedures. The DNA was digested with restriction enzyme HindIII and the digested DNA was size fractionated by electrophoresis through an agarose gel. The DNA was blotted from the agarose gel to a nitrocellulose filter and the filter was incubated with the cloned apr gene that had been radioactively labeled with .sup.32 P-dATP plus Klenow. After incubation, the filter was washed and exposed to X-ray film. Analysis of the resulting autoradiogram showed that the labeled apr gene probe hybridized to a DNA restriction fragment from each of the sixteen B.t. strains. This result demonstrated that the apr gene is present in all sixteen varieties of B.t.
In a similar experiment, the radioactively labeled, cloned npr gene was incubated with a nitrocellulose filter containing digested DNA from each of the sixteen varieties of B.t. mentioned above. The filter was washed and exposed to X-ray film. Analysis of the resulting autoradiogram showed that the labeled npr gene probe hybridized to a DNA restriction fragment from each of the is sixteen B.t. strains. This result demonstrated that the npr gene is present in all sixteen varieties of B.t.
The present invention may be embodied in other specific forms without departing from the spirit or essential attributes thereof and, accordingly, reference should be made to the appended claims, rather than to the foregoing specification as indicating the scope of the invention.
__________________________________________________________________________# SEQUENCE LISTING- (1) GENERAL INFORMATION:- (iii) NUMBER OF SEQUENCES: 9- (2) INFORMATION FOR SEQ ID NO:1:- (i) SEQUENCE CHARACTERISTICS:#pairs (A) LENGTH: 1750 base (B) TYPE: nucleic acid (C) STRANDEDNESS: double (D) TOPOLOGY: circular- (ii) MOLECULE TYPE: DNA (genomic)#ID NO:1: (xi) SEQUENCE DESCRIPTION: SEQ- AAAAGGAATG ACTCATACAT GATGAGCGTT CCTTTTTTCA TCCCCTCTTT TA - #CTTAATTA 60- CTATCATTAA AAATATATTT ATATCAATAT TTACTCCTTT TTATTCCTTC AA - #AAGTTTTT 120- CACATAAATG TCATAAATCG TATGGTTTAA CTATATAGTT GAAAAGGAAT GC - #GACATTAA 180- GGTGTCACTG AAAAACTCAT CCAAGAAAAG GGAGGAAAAA TCTTTTGAAA AA - #CAAAATCA 240- TCGTTTTCCT ATCTGTTTTG TCATTTATTA TTGGTGGTTT CTTCTTTAAC AC - #GAATACTT 300- CAAGCGCTGA AACATCATCT ACTGATTACG TTCCTAACCA ATTAATCGTT AA - #GTTCAAAC 360- AAAATGCATC TTTAAGTAAT GTGCAATCTT TTCATAAATC TGTCGGAGCT AA - #TGTCTTAT 420- CTAAAGATGA TAAGTTAGGT TTTGAAGTCG TACAATTTTC AAAAGGTACT GT - #AAAAGAAA 480- AAATAAAGAG CTATAAAAAT AATCCAGATG TGGAATATGC AGAACCGAAT TA - #TTACGTTC 540- ACGCCTTTTG GACTCCAAAC GACCCATATT TTAATAATCA ATACGGGTTA CA - #AAAGATTC 600- AAGCTCCACA AGCTTGGGAT AGCCAACGAA GTGATCCTGG TGTAAAAGTA GC - #TATTATTG 660- ATACAGGAGT TCAAGGCTCA CACCCTGATC TGGCTTCGAA AGTAATTTAC GG - #GCATGATT 720- ATGTTGATAA CGACAATACA TCTGATGATG GTAATGGTCA TGGTACACAT TG - #CGCTGGAA 780- TTACTGGAGC ACTTACGAAT AACAGCGTCG GAATTGCTGG TGTTGCCCCA CA - #AACTTCAA 840- TTTATGCTGT CCGCGTATTA GATAATCAAG GAAGTGGTAC TCTTGATGCT GT - #AGCGCAAG 900- GTATTCGAGA AGCTGCTGAT TCGGGTGCAA AAGTAATTAG TTTAAGTTTA GG - #AGCTCCAA 960- ATGGTGGTAC TGCATTACAA CAAGCCGTTC AATATGCATG GAATAAAGGC TC - #TGTTATAG1020- TTGCAGCTGC TGGAAATGCT GGAAATACAA AAGCTAATTA CCCTGCTTAT TA - #CAGCGAAG1080- TAATTGCAGT TGCTTCTACA GATCAATCAG ATAGAAAATC TTCATTCTCT AC - #TTATGGTA1140- GCTGGGTAGA TGTTGCAGCA CCAGGTTCAA ATATATATTC AACATATAAA GG - #AAGCACGT1200- ATCAATCATT AAGTGGTACA TCTATGGCAA CACCTCATGT TGCAGGAGTC GC - #AGCTCTTT1260- TAGCAAATCA AGGATATAGC AATACACAAA TCCGCCAAAT TATTGAGTCT AC - #TACTGATA1320- AAATTAGTGG TACAGGTACG TACTGGAAAA ACGGTAGAGT CAATGCATAT AA - #GGCTGTAC1380- AATACGCTAA GCAATTACAA GAAAATAAAG CTTCTTAAGA AAACTTTAAT CA - #GTCGATCT1440- ACCATGAATG CAGAATAAAA TAGAAGGAGA GACTTCTATA ATTAAAGCCT CT - #CCTTCTTA1500- CAAACTATAT TACTCTCCCT GCTTTTTAAC CATATGTAAA TACAGTACAA AA - #TCCATCAT1560- TGTCGATGAA TGACCAAGTT GACGAATCAT CGCTGTTATA TTTCCTCTAT GA - #TATGTACC1620- ATGATTTACG ACATGTTGCA CTAATTCTAA AATCGAAGTT TCTAATTTCC CT - #ACGTATGG1680- ATTCTCAATA ACAAATACAG CATTCACATC TTGTATTGTA ATTAAAAACT CT - #TTATATTG1740# 1750- (2) INFORMATION FOR SEQ ID NO:2:- (i) SEQUENCE CHARACTERISTICS:#acids (A) LENGTH: 397 amino (B) TYPE: amino acid (C) STRANDEDNESS: single (D) TOPOLOGY: linear- (ii) MOLECULE TYPE: protein#ID NO:2: (xi) SEQUENCE DESCRIPTION: SEQ- Met Lys Asn Lys Ile Ile Val Phe - # Leu Ser Val Leu Ser Phe IleIle# 15- Gly Gly Phe Phe Phe Asn Thr Asn - # Thr Ser Ser Ala Glu Thr SerSer# 30- Thr Asp Tyr Val Pro Asn Gln Leu - # Ile Val Lys Phe Lys Gln AsnAla# 45- Ser Leu Ser Asn Val Gln Ser Phe - # His Lys Ser Val Gly Ala AsnVal# 60- Leu Ser Lys Asp Asp Lys Leu Gly - # Phe Glu Val Val Gln Phe SerLys# 80- Gly Thr Val Lys Glu Lys Ile Lys - # Ser Tyr Lys Asn Asn Pro AspVal# 95- Glu Tyr Ala Glu Pro Asn Tyr Tyr - # Val His Ala Phe Trp Thr ProAsn# 110- Asp Pro Tyr Phe Asn Asn Gln Tyr - # Gly Leu Gln Lys Ile Gln AlaPro# 125- Gln Ala Trp Asp Ser Gln Arg Ser - # Asp Pro Gly Val Lys Val AlaIle# 140- Ile Asp Thr Gly Val Gln Gly Ser - # His Pro Asp Leu Ala Ser LysVal# 160- Ile Tyr Gly His Asp Tyr Val Asp - # Asn Asp Asn Thr Ser Asp AspGly# 175- Asn Gly His Gly Thr His Cys Ala - # Gly Ile Thr Gly Ala Leu ThrAsn# 190- Asn Ser Val Gly Ile Ala Gly Val - # Ala Pro Gln Thr Ser Ile TyrAla# 205- Val Arg Val Leu Asp Asn Gln Gly - # Ser Gly Thr Leu Asp Ala ValAla# 220- Gln Gly Ile Arg Glu Ala Ala Asp - # Ser Gly Ala Lys Val Ile SerLeu# 240- Ser Leu Gly Ala Pro Asn Gly Gly - # Thr Ala Leu Gln Gln Ala ValGln# 255- Tyr Ala Trp Asn Lys Gly Ser Val - # Ile Val Ala Ala Ala Gly AsnAla# 270- Gly Asn Thr Lys Ala Asn Tyr Pro - # Ala Tyr Tyr Ser Glu Val IleAla# 285- Val Ala Ser Thr Asp Gln Ser Asp - # Arg Lys Ser Ser Phe Ser ThrTyr# 300- Gly Ser Trp Val Asp Val Ala Ala - # Pro Gly Ser Asn Ile Tyr SerThr# 320- Tyr Lys Gly Ser Thr Tyr Gln Ser - # Leu Ser Gly Thr Ser Met AlaThr# 335- Pro His Val Ala Gly Val Ala Ala - # Leu Leu Ala Asn Gln Gly TyrSer# 350- Asn Thr Gln Ile Arg Gln Ile Ile - # Glu Ser Thr Thr Asp Lys IleSer# 365- Gly Thr Gly Thr Tyr Trp Lys Asn - # Gly Arg Val Asn Ala Tyr LysAla# 380- Val Gln Tyr Ala Lys Gln Leu Gln - # Glu Asn Lys Ala Ser# 395- (2) INFORMATION FOR SEQ ID NO:3:- (i) SEQUENCE CHARACTERISTICS:#pairs (A) LENGTH: 1960 base (B) TYPE: nucleic acid (C) STRANDEDNESS: double (D) TOPOLOGY: circular- (ii) MOLECULE TYPE: DNA (genomic)#ID NO:3: (xi) SEQUENCE DESCRIPTION: SEQ- TAAGAAAATA TTGAAAAAAC CCCTTTCCAA TCGGAAAGGG GTTTTTTCAA TA - #TTTGTTCC 60- TCAAAATTCT ACAAAACTTG AGAAATAAAT TAATTGAATT TTTAGTATAT TA - #ATAGTGGA 120- AACATAATGC TAATATGAAA CTACTCTTTT TCAAAAAATT TTTTATTAGG GG - #GAAGGTTA 180- TATGAAAAAG AAGAGTTTAG CATTAGTGTT AGCGACAGGA ATGGCAGTTA CA - #ACGTTTGG 240- AGGGACAGGC TCTGCGTTTG CGGATTCTAA AAATGTGCTC TCTACTAAGA AG - #TACAATGA 300- GACGGTGCAG TCACCTGAGT TTATTTCTGG TGATCTAACT GAAGCAACTG GC - #AAGAAAGC 360- AGAATCTGTT GTGTTTGATT ACTTAAACGC AGCAAAAGGT GATTACAAGC TA - #GGGGAAAA 420- GAGTGCACAA GATTCTTTCA AAGTGAAACA AGTGAAGAAA GATGCTGTAA CT - #GATTCAAC 480- AGTAGTACGT ATGCAACAAG TTTACGAAGG AGTGCCTGTA TGGGGTTCTA CT - #CAAGTAGC 540- TCACGTAAGT AAGGACGGTT CTTTAAAAGT ATTGTCTGGA ACAGTTGCAC CT - #GATTTAGA 600- CAAAAAGGAA AAGTTGAAAA ATAAAAATAA GATTGAAGGC GCAAAAGCAA TT - #GAAATCGC 660- GCAGCAAGAT TTAGGGGTAA CACCGAAATA TGAAGTAGAA CCAAAAGCGG AC - #TTATATGT 720- ATATCAAAAC GGTGAGGAAA CAACATATGC ATATGTTGTA AATCTAAACT TC - #TTAGATCC 780- AAGCCCAGGA AACTACTACT ATTTCATTGA GGCAGACAGC GGTAAAGTAT TA - #AATAAGTT 840- TAATACAATT GATCATGTGA CGAATGATGA TAAGTCACCA GTTAAGCAAG AG - #GCTCCTAA 900- ACAGGATGCG AAAGCTGTTG TAAAGCCTGT AACAGGAACG AATAAAGTAG GA - #ACTGGTAA 960- AGGCGTACTA GGAGATACGA AGTCTCTTAA TACAACGTTA TCTGGATCAT CT - #TACTACTT1020- ACAAGATAAT ACACGCGGGG CAACGATTTT CACATATGAT GCGAAAAACC GT - #TCAACATT1080- ACCAGGAACA TTATGGGCAG ATGCAGATAA TGTTTTCAAT GCAGCGTATG AT - #GCAGCAGC1140- GGTAGATGCT CATTACTATG CGGGTATCAC GTATGATTAC TATAAGAATA CA - #TTTAATCG1200- TAATTCAATT AATGATGCAG GAGCGCCGTT AAAATCAACA GTTCATTACG GA - #AGTAATTA1260- TAACAATGCA TTCTGGAACG GATCACAGAT GGTATACGGA GATGGTGATG GT - #GTAACATT1320- TACTTCATTA TCTGGTGGAA TTGATGTAAT TGGTCACGAG TTAACGCATG CT - #GTTACGGA1380- AAATAGTTCA AATCTAATTT ATCAAAATGA ATCAGGGGCT TTAAATGAAG CG - #ATTTCTGA1440- TATCTTTGGT ACTTTAGTAG AATTCTATGA TAACCGTAAC CCGGATTGGG AG - #ATTGGTGA1500- AGATATTTAC ACACCTGGTA AAGCAGGAGA CGCGCTTCGC TCTATGAGTG AT - #CCTACGAA1560- GTATGGTGAT CCAGACCATT ATTCTAAGCG TTACACTGGT TCAAGTGATA AC - #GGTGGCGT1620- TCATACAAAC AGCGGCATTA TTAATAAACA AGCTTATTTA TTAGCAAATG GC - #GGTACGCA1680- TTACGGTGTA ACTGTAAATG GTATCGGCAA AGATAAATTA GGTGCGATTT AC - #TACCGTGC1740- AAATACACAG TATTTCACGC AATCTACTAC ATTTAGTCAA GCTCGTGCTG GT - #GCAGTACA1800- AGCTGCAGCA GACTTATATG GTGCAAATTC TGCTGAAGTA GCAGCAGTTA AG - #CAATCATT1860- TAGTGCTGTT GGTATTAACT AAGGACTTAA CGGATAGCTA TTAATAAAAT AC - #CTCAAAAA1920# 1960 GCTC CTTCTTTATT TTTTTCTCCA- (2) INFORMATION FOR SEQ ID NO:4:- (i) SEQUENCE CHARACTERISTICS:#acids (A) LENGTH: 566 amino (B) TYPE: amino acid (C) STRANDEDNESS: single (D) TOPOLOGY: linear- (ii) MOLECULE TYPE: protein#ID NO:4: (xi) SEQUENCE DESCRIPTION: SEQ- Met Lys Lys Lys Ser Leu Ala Leu - # Val Leu Ala Thr Gly Met AlaVal# 15- Thr Thr Phe Gly Gly Thr Gly Ser - # Ala Phe Ala Asp Ser Lys AsnVal# 30- Leu Ser Thr Lys Lys Tyr Asn Glu - # Thr Val Gln Ser Pro Glu PheIle# 45- Ser Gly Asp Leu Thr Glu Ala Thr - # Gly Lys Lys Ala Glu Ser ValVal# 60- Phe Asp Tyr Leu Asn Ala Ala Lys - # Gly Asp Tyr Lys Leu Gly GluLys# 80- Ser Ala Gln Asp Ser Phe Lys Val - # Lys Gln Val Lys Lys Asp AlaVal# 95- Thr Asp Ser Thr Val Val Arg Met - # Gln Gln Val Tyr Glu Gly ValPro# 110- Val Trp Gly Ser Thr Gln Val Ala - # His Val Ser Lys Asp Gly SerLeu# 125- Lys Val Leu Ser Gly Thr Val Ala - # Pro Asp Leu Asp Lys Lys GluLys# 140- Leu Lys Asn Lys Asn Lys Ile Glu - # Gly Ala Lys Ala Ile Glu IleAla# 160- Gln Gln Asp Leu Gly Val Thr Pro - # Lys Tyr Glu Val Glu Pro LysAla# 175- Asp Leu Tyr Val Tyr Gln Asn Gly - # Glu Glu Thr Thr Tyr Ala TyrVal# 190- Val Asn Leu Asn Phe Leu Asp Pro - # Ser Pro Gly Asn Tyr Tyr TyrPhe# 205- Ile Glu Ala Asp Ser Gly Lys Val - # Leu Asn Lys Phe Asn Thr IleAsp# 220- His Val Thr Asn Asp Asp Lys Ser - # Pro Val Lys Gln Glu Ala ProLys# 240- Gln Asp Ala Lys Ala Val Val Lys - # Pro Val Thr Gly Thr Asn LysVal# 255- Gly Thr Gly Lys Gly Val Leu Gly - # Asp Thr Lys Ser Leu Asn ThrThr# 270- Leu Ser Gly Ser Ser Tyr Tyr Leu - # Gln Asp Asn Thr Arg Gly AlaThr# 285- Ile Phe Thr Tyr Asp Ala Lys Asn - # Arg Ser Thr Leu Pro Gly ThrLeu# 300- Trp Ala Asp Ala Asp Asn Val Phe - # Asn Ala Ala Tyr Asp Ala AlaAla# 320- Val Asp Ala His Tyr Tyr Ala Gly - # Ile Thr Tyr Asp Tyr Tyr LysAsn# 335- Thr Phe Asn Arg Asn Ser Ile Asn - # Asp Ala Gly Ala Pro Leu LysSer# 350- Thr Val His Tyr Gly Ser Asn Tyr - # Asn Asn Ala Phe Trp Asn GlySer# 365- Gln Met Val Tyr Gly Asp Gly Asp - # Gly Val Thr Phe Thr Ser LeuSer# 380- Gly Gly Ile Asp Val Ile Gly His - # Glu Leu Thr His Ala Val ThrGlu# 400- Asn Ser Ser Asn Leu Ile Tyr Gln - # Asn Glu Ser Gly Ala Leu AsnGlu# 415- Ala Ile Ser Asp Ile Phe Gly Thr - # Leu Val Glu Phe Tyr Asp AsnArg# 430- Asn Pro Asp Trp Glu Ile Gly Glu - # Asp Ile Tyr Thr Pro Gly LysAla# 445- Gly Asp Ala Leu Arg Ser Met Ser - # Asp Pro Thr Lys Tyr Gly AspPro# 460- Asp His Tyr Ser Lys Arg Tyr Thr - # Gly Ser Ser Asp Asn Gly GlyVal# 480- His Thr Asn Ser Gly Ile Ile Asn - # Lys Gln Ala Tyr Leu Leu AlaAsn# 495- Gly Gly Thr His Tyr Gly Val Thr - # Val Asn Gly Ile Gly Lys AspLys# 510- Leu Gly Ala Ile Tyr Tyr Arg Ala - # Asn Thr Gln Tyr Phe Thr GlnSer# 525- Thr Thr Phe Ser Gln Ala Arg Ala - # Gly Ala Val Gln Ala Ala AlaAsp# 540- Leu Tyr Gly Ala Asn Ser Ala Glu - # Val Ala Ala Val Lys Gln SerPhe# 560- Ser Ala Val Gly Ile Asn# 565- (2) INFORMATION FOR SEQ ID NO:5:- (i) SEQUENCE CHARACTERISTICS:#pairs (A) LENGTH: 38 base (B) TYPE: nucleic acid (C) STRANDEDNESS: single (D) TOPOLOGY: linear- (ii) MOLECULE TYPE: other nucleic acid#= "OLIGONUCLEOTIDE"PTION: /desc#ID NO:5: (xi) SEQUENCE DESCRIPTION: SEQ# 38 CATA TTTTAATAAT CAATATGG- (2) INFORMATION FOR SEQ ID NO:6:- (i) SEQUENCE CHARACTERISTICS:#pairs (A) LENGTH: 38 base (B) TYPE: nucleic acid (C) STRANDEDNESS: single (D) TOPOLOGY: linear- (ii) MOLECULE TYPE: other nucleic acid#= "OLIGONUCLEOTIDE"PTION: /desc#ID NO:6: (xi) SEQUENCE DESCRIPTION: SEQ# 38 GACA TGAATTAACA CATGCAGT- (2) INFORMATION FOR SEQ ID NO:7:- (i) SEQUENCE CHARACTERISTICS:#pairs (A) LENGTH: 35 base (B) TYPE: nucleic acid (C) STRANDEDNESS: single (D) TOPOLOGY: linear- (ii) MOLECULE TYPE: other nucleic acid#= "OLIGONUCLEOTIDE"PTION: /desc#ID NO:7: (xi) SEQUENCE DESCRIPTION: SEQ# 35 GAGA TGGAGTAACA TTTAC- (2) INFORMATION FOR SEQ ID NO:8:- (i) SEQUENCE CHARACTERISTICS:#pairs (A) LENGTH: 29 base (B) TYPE: nucleic acid (C) STRANDEDNESS: single (D) TOPOLOGY: linear- (ii) MOLECULE TYPE: other nucleic acid#= "OLIGONUCLEOTIDE"PTION: /desc#ID NO:8: (xi) SEQUENCE DESCRIPTION: SEQ# 29 AAGA GTTTAGCAT- (2) INFORMATION FOR SEQ ID NO:9:- (i) SEQUENCE CHARACTERISTICS:#pairs (A) LENGTH: 30 base (B) TYPE: nucleic acid (C) STRANDEDNESS: single (D) TOPOLOGY: linear- (ii) MOLECULE TYPE: other nucleic acid#= "OLIGONUCLEOTIDE"PTION: /desc#ID NO:9: (xi) SEQUENCE DESCRIPTION: SEQ# 30 TACC AACAGCACTA__________________________________________________________________________
Claims
  • 1. A method of reducing the proteolytic degradation of a Bacillus thuringiensis insecticidal toxic protein in a composition comprising the toxic protein, the method comprising including in the composition a Bacillus thuringiensis protease gene disabled from coding for protease capable of degrading the toxic protein, the protease gene before being disabled being selected from the group consisting of an alkaline protease gene and a neutral protease gene, the alkaline protease gene before being disabled having a nucleotide base sequence coding for the amino acid sequence identified in SEQ ID NO:2, and the neutral protease gene before being disabled has a nucleotide base sequence coding for the amino acid sequence identified in SEO ID NO:4, whereby protease expressed by an organism with in the composition containing the disabled protease gene has reduced proteolytic activity against the toxic protein compared to protease encoded by a counterpart protease gene that has not been disabled, thereby resulting in reduced proteolytic activity against the toxic protein.
  • 2. The method of claim 1 wherein the protease gene before being disabled is the alkaline protease gene.
  • 3. The method of claim 2 wherein the disabled protease gene has the characteristics of an apr1 gene contained in Bacillus thuringiensis strain EG7950 deposited in NRRL with accession number NRRL B-21343.
  • 4. The method of claim 2 wherein the insecticidal toxic protein is selected from the group consisting of CryI-type, CryII-type, CryIII-type, CryIV-type, CryV-type, CryET1, Cry ET4 and CryET5 protein, and mixtures thereof.
  • 5. The method of claim 4 wherein the insecticidal toxic protein is a CryI-type protein.
  • 6. The method of claim 2 further comprising expressing the toxic protein in the composition by including in the composition a gene coding for the insecticidal toxic protein, wherein the gene coding for the toxic protein is a gene selected from the group consisting of a cryI-type, cryII-type, cryIII-type, cryIV-type, cryV-type, cryET1, cryET4 and cryET5 gene, and mixtures thereof.
  • 7. The method of claim 6 wherein the gene coding for the insecticidal toxic protein is a cryI-type gene.
  • 8. The method of claim 2 wherein the composition includes Bacillus thuringiensis strain EG10654 deposited in NRRL with accession number NRRL B-21344.
  • 9. The method of claim 1 wherein the protease gene before being disabled is the neutral protease gene.
  • 10. The method of claim 9 wherein the disabled gene has the characteristics of an npr3 gene contained in Escherichia coli strain EG11447 deposited in NRRL with accession number NRRL B-21346.
  • 11. The method of claim 9 wherein the insecticidal toxic protein is selected from the group consisting of CryI-type, CryII-type, CryIII-type, CryIV-type, CryV-type, CryET1, CryET4 and CryET5 protein, and mixtures thereof.
  • 12. The method of claim 11 wherein the insecticidal toxic protein is a CryI-type protein.
  • 13. The method of claim 9 further comprising expressing the toxic protein in the composition by including in the composition a gene coding for the insecticidal toxic protein, wherein the gene coding for the toxic protein is a gene selected from the group consisting of a cryI-type, cryII-type, cryIII-type, cryIV-type, cryV-type, cryET1, cryET4 and cryET5 gene, and mixtures thereof.
  • 14. The method of claim 13 wherein the gene coding for the insecticidal toxic protein is a cryI-type gene.
  • 15. The method of claim 9 wherein the composition includes Bacillus thuringiensis strain EG10624 deposited in NRRL with accession number NRRT B-21347.
CROSS-REFERENCE TO RELATED APPLICATION

This application is a division of U.S. patent application Ser. No. 08/415,823, filed Mar. 31, 1995, now U.S. Pat. No. 5,759,538.

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Divisions (1)
Number Date Country
Parent 415823 Mar 1995