Detection of fungal pathogens using the polymerase chain reaction

Information

  • Patent Application
  • 20040029255
  • Publication Number
    20040029255
  • Date Filed
    July 21, 2003
    21 years ago
  • Date Published
    February 12, 2004
    20 years ago
Abstract
The present invention relates to the use of primers in polymerase chain reaction assays for the detection of fungal pathogens Colletotrichum acutatum, Alternaria spp., and Cladosporium carpophilum. Specific primers are identified as being useful for the identification of fungal isolates using PCR based techniques. Also described are novel extraction buffer solutions for use in isolating DNA from an organism, methods of extracting DNA from tissue, and methods of performing PCR analysis on DNA extracted from tissue.
Description


FIELD OF THE INVENTION

[0001] The present invention relates to the use of primers in polymerase chain reaction assays for the detection of stone fruit and nut, in particular almond pathogens Colletotrichum acutatum, Alternaria spp., and Cladosporium carpophilum. The use of these primers enables the detection of specific isolates of fungal pathogens and the monitoring of disease development in plant populations. The present-invention also relates to novel extraction buffer solutions, methods of extracting DNA from tissue, and methods of performing PCR analysis on DNA extracted from tissue.



BACKGROUND OF THE INVENTION

[0002] Diseases in plants cause considerable crop loss from year to year resulting both in economic deprivation to farmers and, in many parts of the world, to shortfalls in the nutritional provision for local populations. The widespread use of fungicides has provided considerable security against plant pathogen attack. However, despite $1 billion worth of expenditure on fungicides, worldwide crop losses amounted to approximately 10% of crop value in 1981 (James, 1981; Seed Sci. & Technol. 9: 679-685).


[0003] The severity of the destructive process of disease depends on the aggressiveness of the pathogen and the response of the host. One aim of most plant breeding programs is to increase the resistance of host plants to disease. Typically, different races of pathogens interact with different varieties of the same crop species differentially, and many sources of host resistance only protect against specific pathogen races. Furthermore, some pathogen races show early signs of disease symptoms, but cause little damage to the crop. Jones and Clifford (1983; Cereal Diseases, John Wiley) report that virulent forms of the pathogen are expected to emerge in the pathogen population in response to the introduction of resistance into host cultivars and that it is therefore necessary to monitor pathogen populations. In addition, there are several documented cases of the evolution of fungal strains that are resistant to particular fungicides. As early as 1981, Fletcher and Wolfe (1981; Proc. 1981 Brit. Crop Prot. Conf.) contended that 24% of the powdery mildew populations from spring barley and 53% from winter barley showed considerable variation in response to the fungicide triadimenol and that the distribution of these populations varied between varieties, with the most susceptible variety also giving the highest incidence of less susceptible types. Similar variation in the sensitivity of fungi to fungicides has been documented for wheat mildew (also to triadimenol), Botrytis (to benomyl), Pyrenophora (to organomercury), Pseudocercosporella (to MBC-type fungicides) and Mycosphaerella fijiensis to triazoles to mention just a few (Jones and Clifford; Cereal Diseases, John Wiley, 1983).


[0004] Commercial almond growers are faced with a number of fungi that infect their crops in diverse ways. The impact of these pathogens on tree growth depends on a number of factors, and the cause is not immediately apparent from the symptoms a diseased tree may present. Vascular pathogens invade and plug the xylem vessels, thereby halting movement of water and nutrients up from roots (Integrated Pest Management for Almonds, U. California Division of Agriculture and Natural resources publication 3308 (1985)). Symptoms often reflect a partial or complete cut-off from food or water as vascular tissues are closed. Thus, symptoms of crown and root rots of almond, as well as wilts caused by pathogens infecting leaf and branch tissues, may appear very similar to one another; and similar to the consequences of environmental conditions such as the availability of nutrients and water and factors affecting their uptake.


[0005] Some pathogens cause infections that are limited to branches, foliage, and fruit. Several of the fungi and bacteria that cause disease in almonds have been found to infect orchards during the fall months and over-winter in host tissues. During the spring, they produce localized lesions or larger infections that become evident after environmental conditions such as a recent rain or irrigation promote the growth of the pathogens.


[0006] The same pathogens that cause economic problems in almond orchard management also affect other crops. For instance, Cladosporium carpophilum has a host range that extends over stone fruits. For example, in addition to the scabs it causes in almond crops, C. carpophilum also causes scabs in peaches, nectarines, apricots, plums, and cherries (Compendium of Stone Fruit Diseases, Ogawa, J. M.; Zehr, E. I.; Bird, G. W.; Ritchie, D. F.; Uriu, K.; Uyemoto, J. K. eds., p. 11 (1995 APS Press, St. Paul, Minn.)).


[0007] Alternaria spp. has been documented as causing infection on many economically important crops. To date, it has been reported to cause alternaria blight of peas, and alternaria leaf spots have been reported on peanuts, almonds, corn, cotton, and in all soybean growing areas of the world (Compendium of Soybean Diseases, 4th Ed. Hartman, G. L.; Sinclair, J. B.; Rupe, J. C. eds., pp. 12-13 (1999, APS Press, St. Paul, Minn.)); (Compendium of Cotton Diseases, Watkins, G. M. ed., p. 28 (1981, APS Press, St. Paul, Minn.); Compendium of Pea Diseases, Hagedorn, D. J., ed., p. 15 (1984, APS Press, St. Paul, Minn.)); (Compendium of Peanut Diseases, Porter, D. M.; Smith, D. H.; Rodriguez-Kabana, R. eds. Pp. 13 (1984, APS Press, St. Paul, Minn.); (Compendium of Stone Fruit Diseases, Ogawa, J. M.; Zehr, E. I.; Bird, G. W.; Ritchie, D. F.; Uriu, K.; Uyemoto, J. K. eds.,p. 11 (1995 APS Press, St. Paul, Minn.)); and Compendium of Corn Diseases, 3rd Ed. White, D. G., ed., p. 25 (1999, APS Press, St. Paul, Minn.)). Alternaria spp. is responsible for widespread leaf and pod spots on beans grown in Brazil, Cananda, Costa Rica, Colombia, Chile, East Africa, England, Mexico, the United States, and Venezuela (Compendium of Bean Diseases, Hall, R. ed., p. 14 (1991, APS Press, St. Paul, Minn.)). Alternaria spp. also form lesions on potatoes and the leaves of other solanaceous crops; (Compendium of Potato Diseases, Hooker, W. J. ed., p. 44 (1981, APS Press, St. Paul, Minn.)) and appear as secondary infections on sugar beet leaves (Compendium of Beet Diseases and Insects, Whitney, E. D., Duffus, J. E. eds., p. 11 (1991 APS Press, St. Paul, Minn.)). It causes grain molds in sorghum (Compendium of Sorghum Diseases, Frederiksen, R. A. ed., p. 36 (1986 APS Press, St. Paul, Minn.)) and is one cause of black mold rot of tomato (Compendium of Tomato Diseases, Jones, J. B.; Jones, J. P.; Stall, R. E.; Zitter, T. A., eds., p. 46 (1991 APS Press, St. Paul, Minn.)). Alternaria spp. also causes fruit spot of papaya, a major disease in orchards located in dry areas and in mangos (Compendium of Tropical Fruit Diseases, Ploetz, R. C.; Zentmyer, G. A.; Nishijima, W. T.; Rohrbach, K. G.; Ohr, H. D., eds., pp. 34 and 58 (1994 APS Press, St. Paul, Minn.)).


[0008]

Colletotrichum acutatum
has been reported to infect a large number of fruit crops including avocado, strawberry, almond, apple, and peach. C. acutatum causes post-harvest fruit diseases in avocado and mango. C. acutatum is also known to cause both post-bloom fruit drop and key lime anthracnose in citrus crops (see Freeman, S. et al. ,1998, Plant Disease Vol. 82, No. 6, pp. 596-605).


[0009] In view of the above, there is a real need for the development of technology that will allow the identification of specific races of pathogenic fungi early in the infection process. By identifying the specific race of a pathogen before disease symptoms become evident in the crop stand, the agriculturist can assess the likely effects of further development of the pathogen in the crop variety in which it has been identified and can choose an appropriate fungicide if such application is deemed necessary.



SUMMARY OF THE INVENTION

[0010] The present invention is drawn to methods of identification of different pathotypes of plant pathogenic fungi. The invention provides Internal Transcribed Spacer (ITS) DNA sequences that show variability between different fungal pathotypes. Such DNA sequences are useful in the method of the invention as they can be used to derive primers for use in polymerase chain reaction (PCR)-based diagnostic assays. These primers generate unique fragments in PCR reactions in which the DNA template is provided by specific fungal pathotypes and can thus be used to identify the presence or absence of specific pathotypes in host plant material before the onset of disease symptoms.


[0011] In a preferred embodiment, the invention provides ITS-derived diagnostic primers for the detection of Colletotrichum acutatum, Alternaria spp., and Cladosporium carpophilum.


[0012] This invention provides the possibility of assessing potential damage in a specific crop variety/pathogen strain relationship and of utilizing judiciously the diverse armory of fungicides that is available. Furthermore, the invention can be used to provide detailed information on the development and spread of specific pathogen races over extended geographical areas. The invention provides a method of detection that is especially suitable for diseases with a long latent phase.


[0013] Kits useful in the practice of the invention are also provided. The kits find particular use in the identification of Colletotrichum acutatum, Alternaria spp., and Cladosporium carpophilum.


[0014] The invention also provides methods for preparing an extract of DNA from tissue using novel DNA extraction buffer. The invention further provides for methods for performing PCR analysis on DNA extracted from tissue using the novel DNA extraction buffer and methods of preparing an extract of DNA.



BRIEF DESCRIPTION OF THE SEQUENCES IN THE SEQUENCE LISTING

[0015] SEQ-ID-NO: 1 Oligonucleotide Primer ITS1


[0016] SEQ-ID-NO: 2 Oligonucleotide Primer ITS2


[0017] SEQ-ID-NO: 3 Oligonucleotide Primer ITS3


[0018] SEQ-ID-NO: 4 Oligonucleotide Primer ITS4


[0019] SEQ-ID-NO: 5 Oligonucleotide Primer FORWARD


[0020] SEQ-ID-NO: 6 Oligonucleotide Primer REVERSE


[0021] SEQ-ID-NO: 7 Oligonucleotide Primer CaINT-1


[0022] SEQ-ID-NO: 8 Oligonucleotide Primer CaINT-2


[0023] SEQ-ID-NO: 9 Oligonucleotide Primer CaInt2


[0024] SEQ-ID-NO: 10 Oligonucleotide Primer JB677


[0025] SEQ-ID-NO: 11 Oligonucleotide Primer JB678


[0026] SEQ-ID-NO: 12 Oligonucleotide Primer JB679


[0027] SEQ-ID-NO: 13 Oligonucleotide Primer Alal-1


[0028] SEQ-ID-NO: 14 Oligonucleotide Primer Alal-2


[0029] SEQ-ID-NO: 15 Oligonucleotide Primer Alal-3


[0030] SEQ-ID-NO: 16 Oligonucleotide Primer Alal-4


[0031] SEQ-ID-NO: 17 Oligonucleotide Primer Alal-5


[0032] SEQ-ID-NO: 18 Oligonucleotide Primer Alal-6


[0033] SEQ-ID-NO: 19 Oligonucleotide Primer Alt1


[0034] SEQ-ID-NO: 20 Oligonucleotide Primer Alt2


[0035] SEQ-ID-NO: 21 Oligonucleotide Primer Vcarp1


[0036] SEQ-ID-NO: 22 Oligonucleotide Primer Vcarp2


[0037] SEQ-ID-NO: 23 Oligonucleotide Primer Vcarp3


[0038] SEQ-ID-NO: 24 Oligonucleotide Primer Vcarp4


[0039] SEQ-ID-NO: 25 Oligonucleotide Primer Vcarp5


[0040] SEQ-ID-NO: 26 Oligonucleotide Primer Vcarp6


[0041] SEQ-ID-NO: 27 Oligonucleotide Primer Vcarp7


[0042] SEQ-ID-NO: 28 Oligonucleotide Primer JB677.1


[0043] SEQ-ID-NO: 29 Oligonucleotide Primer JB677.2


[0044] SEQ-ID-NO: 30 Oligonucleotide Primer JB677.3



DETAILED DESCRIPTION OF THE INVENTION

[0045] The present invention provides unique DNA sequences that are useful in identifying different pathotypes of plant pathogenic fungi. Particularly, the DNA sequences can be used as primers in PCR-based analysis for the identification of fungal pathotypes. The DNA sequences of the invention include the Internal Transcribed Spacer (ITS) sequences of the ribosomal RNA gene regions of particular fungal pathogens as well as primers derived from these regions that are capable of identifying the particular pathogen. ITS DNA sequences from different pathotypes within a pathogen species or-genus, which vary between the different members of the species or genus, can be used to identify those specific members.


[0046] Biomedical researchers have, used: PCR-based techniques for some time and with moderate success to detect pathogens in infected animal tissues. Only recently, however, has this technique been applied to detect plant pathogens. The presence of Gaumannomyces graminis in infected wheat has been detected using PCR of sequences specific to the pathogen mitochondrial genome (Schlesser et al., 1991; Applied and Environ. Microbiol. 57: 553-556), and random amplified polymorphic DNA (i.e. RAPD) markers were able to distinguish numerous races of Gremmeniella abietina, the causal agent of scleroderris canker in conifers. U.S. Pat. No. 5,585,238.(herein incorporated by reference in its entirety) describes primers derived from the ITS sequences of the ribosomal RNA gene region of strains of Septoria, Pseudocercosporella, and Mycosphaerella and their use in the identification of these fungal isolates using PCR-based techniques. In addition, U.S. Pat. No. 5,955,274 (herein incorporated by reference in its entirety) describes primers derived from the ITS sequences of the ribosomal RNA gene region of strains of Fusarium and their use in the identification of these fungal isolates using PCR-based techniques. Furthermore, U.S. Pat. No. 5,800,997 (herein incorporated by reference in its entirety) describes primers derived from the ITS sequences of the ribosomal RNA gene region of strains of Cercospora, Helminthosporium, Kabatiella, and Puccinia and their use in the identification of these fungal isolates using PCR-based techniques.


[0047] Ribosomal genes are suitable for use as molecular probe targets because of their high copy number. Despite the high conservation between mature rRNA sequences, the non-transcribed and transcribed spacer sequences are usually poorly conserved and are thus suitable as target sequences for the detection of recent evolutionary divergence. Fungal rRNA genes are organized in units, each of which encodes three mature subunits of 18S (small subunit), 5.8S, and 28S (large subunit). These subunits are separated by two Internal Transcribed Spacers, ITS1 and ITS2, of around 300 bp (White et al., 1990; In: PCR Protocols; Eds.: Innes et al.; pages 315-322). In addition, the transcriptional units are separated by non-transcribed spacer sequences (NTSs). ITS and NTS sequences are particularly suitable for the detection of specific pathotypes of different fungal pathogens.


[0048] The DNA sequences of the invention are from the Internal Transcribed Spacer sequences of the ribosomal RNA gene region of different plant pathogens. The ITS DNA sequences from different pathotypes within a pathogen species or genus vary among the different members of the species or genus. Once having determined the ITS sequences of a pathogen, these sequences can be aligned with other ITS sequences. In this manner, primers can be derived from the ITS sequences. That is, primers can be designed based on regions within the ITS sequences that contain the greatest differences in sequence among the fungal pathotypes. These sequences and primers based on these sequences can be used to identify specific pathogens.


[0049] Sequences of representative oligonucleotide primers derived from ITS sequences are disclosed in SEQ-ID-NOs: 1-4 and 7-30. The sequences find use in the PCR-based identification of the pathogens of interest. In a preferred embodiment, the primer comprises a nucleotide sequence of SEQ ID NOS: 10-30.


[0050] The present invention also provides pairs of oligonucleotide primers. In one embodiment, the pair comprises or consists of at least one primer of SEQ ID NO: 1-4 or 7-30. In a preferred embodiment, the pair consists of at least one primer of SEQ ID NO: 10-30.


[0051] In yet other embodiments, a pair of oligonucleotide primers, is selected from the group consisting of: SEQ ID NO:30 and SEQ ID NO:4; SEQ ID NO:27 and SEQ ID NO:4; SEQ ID NO:16 and SEQ ID NO:12; SEQ ID NO:16 and SEQ ID NO:18; SEQ ID NO:17 and SEQ ID NO:12; SEQ ID NO:1 and SEQ ID NO:27; SEQ ID NO:24 and SEQ ID NO:25; and SEQ ID NO:21 and SEQ ID NO:4.


[0052] In preferred embodiments, the pair of oligonucleotide primers consists of SEQ ID NO:16 and SEQ ID NO:12; or SEQ ID NO:16 and 18; or SEQ ID NO:17 and SEQ ID NO:12; or SEQ ID NO:24 and SEQ ID NO:25.


[0053] Methods for the use of the primer sequences of the invention in PCR analysis are well known in the art. For example, see U.S. Pat. Nos. 4,683,195 and 4,683,202, as well as Schlesser et al. (1991) Applied and Environ. Microbiol. 57:553-556. See also, Nazar et al. (1991; Physiol. and Molec. Plant Pathol. 39:1-11), which used PCR amplification to exploit differences in the ITS regions of Verticillium albo-atrum and Verticillium dahliae and therefore distinguish between the two species; and Johanson and Jeger (1993; Mycol. Res. 97: 670-674), who used similar techniques to distinguish the banana pathogens Mycosphaerella fijiensis and Mycospharella musicola.


[0054] The target DNA sequences of the invention can be cloned from fungal pathogens by methods known in the art. In general, the methods for the isolation of DNA from fungal isolates are known. See, Raeder & Broda (1985) Letters in Applied Microbiology 2:17-20; Lee et al. (1990) Fungal Genetics Newsletter 35:23-24; and Lee and Taylor (1990) In: PCR Protocols: A Guide to Methods and Applications, Innes et al. (Eds.); pages 282-287. The ITS rDNA sequences are compared within each pathogen group to locate divergences that might be useful to test in PCR to distinguish the different species and/or strains. From the identification of divergences, numerous primers are synthesized and tested in PCR-amplification. Templates used for PCR-amplification testing are firstly purified pathogen DNA, and subsequently DNA isolated from infected host plant tissue. Thus, it is possible to identify pairs of primers that are diagnostic, i.e. that identify one particular pathogen species or strain but not another species or strain of the same pathogen. Primers are also designed to regions highly conserved among the species to develop genus-specific primers as well as primers that will identify any of several fungal pathogens that cause a particular disease. For example, primers are developed to differentiate Colletotrichum acutatum, Alternaria spp., and Cladosporium carpophilum.


[0055] Preferred primer combinations are able to distinguish between the different species or strains in infected host tissue, i.e. host tissue that is infected with a specific pathogen genus, species or strain. This invention provides numerous primer combinations that distinguish Colletotrichum acutatum, Alternaria spp., and Cladosporium carpophilum. The primers of the invention are designed based on sequence differences among the ITS rDNA regions. A minimum of one base pair difference between sequences can permit design of a discriminatory primer. Primers designed to a specific fungal DNA sequence can be used in combination with a primer made to a conserved sequence region flanking the region containing divergences to amplify species-specific PCR fragments. In general, primers should have a theoretical melting temperature between about 60 to about 70 degree ° C. to achieve good sensitivity and should be void of significant secondary structure and 3′ overlaps between primer combinations. In preferred embodiments, primers are anywhere from approximately 5-30 nucleotide bases long.


[0056] The present invention provides, a method for the detection of a fungal pathogen, comprising the steps of:


[0057] (a) isolating DNA from a plant tissue infected with a pathogen;


[0058] (b) subjecting said DNA to polymerase chain reaction amplification using at least one primer according to SEQ ID NO: 1-4 and 7-30; and


[0059] (c) detecting said fungal pathogen by visualizing the product or products of said polymerase chain reaction amplification.


[0060] In a preferred embodiment, the primer is at least one according to SEQ ID NO: 10-30.


[0061] In another embodiment, the method for detection is used when the fungal pathogen is Colletotrichum acutatum, Alternaria spp., and Cladosporium carpophilum.


[0062] In another embodiment, the invention provides a method for the detection of a fungal pathogen, comprising the steps of:


[0063] (a) isolating DNA from a plant tissue infected with said fungal pathogen;


[0064] (b) amplifying a part of the Internal Transcribed Spacer sequence of said fungal pathogen using said DNA as a template in a polymerase chain reaction with a pair of primers wherein the pair comprises or consists of at least one primer of SEQ ID NO: 1-4 or 7-10. In a preferred embodiment, the pair consists of at least one primer of SEQ ID NO:10-30; and


[0065] (c) detecting said fungal pathogen by visualizing the amplified part of the Internal Transcribed Spacer sequence.


[0066] In a preferred embodiment, the method detects a fungal pathogen, wherein said fungal pathogen is Colletotrichum acutatum, Alternaria spp., and Cladosporium carpophilum.


[0067] In yet other embodiments, the method of detection uses a pair of primers, wherein said pair of primers is selected from the group consisting of: SEQ ID NO: 30 and SEQ ID NO:4; SEQ ID NO:27 and SEQ ID NO:4; SEQ ID NO:16 and SEQ ID NO:12; SEQ ID NO:16 and SEQ ID NO:18; SEQ ID NO:17 and SEQ ID NO:12; SEQ ID NO:1 and SEQ ID NO:27; SEQ ID NO:24 and SEQ ID NO:25; and SEQ ID NO:21 and SEQ ID NO:4.


[0068] In preferred embodiments, the pair of oligonucleotide primers consists of SEQ ID NO:16 and SEQ ID NO:12; or SEQ ID NO:16 and 18; or SEQ ID NO:17 and SEQ ID NO:12; or SEQ ID NO:24 and SEQ ID NO:25.


[0069] The present invention also provides a method for performing PCR analysis on DNA extracted from tissue, comprising the steps of:


[0070] (a) taking a plurality of random tissue samples from an organism population;


[0071] (b) adding the extraction buffer described in Example 2, to the tissue samples;


[0072] (c) macerating the tissue samples and extraction buffer to form an extract;


[0073] (d) removing the extract from the macerated tissue and buffer; and


[0074] (e) performing PCR analysis on the extract.


[0075] In another embodiment, the method further comprises the step of boiling the extract after removing it from the macerated tissue and buffer.


[0076] In yet another embodiment, the method further comprises the step of diluting the extract.


[0077] In a preferred embodiment, the method uses an organism population that is a plant population. In more preferred embodiments, the method uses tissue samples selected from leaves, stems, roots, blossoms, immature flowers, peduncles, hulls, fruits, immature fruits, or woody tissue.


[0078] In another preferred embodiment, the method uses the extraction buffer comprising: 100 mM Tris, pH 8.0; 1.4 M NaCl; 20 mM EDTA; 2% w/v CTAB; 2% w/v PVP and 0.1% w/v ascorbic acid.


[0079] The present invention lends itself readily to the preparation of “kits” containing the elements necessary to carry out the process. Such a kit may comprise a carrier being compartmentalized to receive in close confinement therein one or more container, such as tubes or vials. One of the containers may contain unlabeled or detectably labeled DNA primers. The labeled DNA primers may be present in lyophilized form or in an appropriate buffer as necessary. One or more containers may contain one or more enzymes or reagents to be utilized in PCR reactions. These enzymes may be present by themselves or in admixtures, in lyophilized form or in appropriate buffers.


[0080] Finally, the kit may contain all of the additional elements necessary to carry out the technique of the invention, such as buffers, extraction reagents, enzymes, pipettes, plates, nucleic acids, nucleoside triphosphates, filter paper, gel materials, transfer materials, autoradiography supplies, and the like.


[0081] In an embodiment of the invention, the diagnostic kit used in detecting a fungal pathogen, comprises a primer of the present invention as described above.


[0082] In yet another embodiment, the diagnostic kit used in detecting a fungal pathogen, comprises a pair of primers of the present invention as described above. The primers, methods and kits of the present invention are useful for detecting the presence of fungal pathogens in any plants or plant parts that are infected by fungal pathogens. In particular, the present invention is useful for detection of Colletotrichum acutatum, Alternaria spp., and Cladosporium carpophilum. Examples of plants or plant tissues or plant parts infected by these pathogens include, but are not limited to, stone fruits, nuts, solanaceous plants such as tomato and potato, peanuts, corn, sorghum, peas, papaya, avacado, apples, and sugarbeets. Examples of stone fruits include, but are not limited to peaches, nectarines, cherries, apricots and plums. Examples of nut crops include, but are not limited to peanuts, almonds, walnuts, cashews, hazelnuts, brazil nuts, etc.


[0083] The examples below show typical experimental protocols that can be used in the selection of suitable primer sequences, the testing of primers for selective and diagnostic efficacy, and the use of such primers for disease and fungal isolate detection. Such examples are provided by way of illustration and not by way of limitation.







EXAMPLES

[0084] Standard recombinant DNA and molecular cloning techniques used here are well known in the art and are described by J. Sambrook, E. F. Fritsch and T. Maniatis, Molecular Cloning: A Laboratory manual, Cold Spring Harbor laboratory, Cold Spring Harbor, N.Y. (1989) and by T. J. Silhavy, M. L. Berman, and L. W. Enquist, Experiments with Gene Fusions, Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y. (1984) and by Ausubel, F. M. et al., Current Protocols in Molecular Biology, pub. by Greene Publishing Assoc. and Wiley-Interscience (1987).



Example 1


Fungal Isolates and Genomic Fungal DNA Extraction

[0085] See Table 1 for a listing of the fungal isolates used and their source. Fungi are grown on PDA (Potato Dextrose Agar) plates. Cultures are incubated for up to 10 days at 28° C. Mycelia are ground in liquid nitrogen, and total genomic DNA is extracted using the protocol of Lee and Taylor (1990; In: PCR Protocols: A Guide to Methods and Applications; Eds.: Innes et al.; pages 282-287).
1TABLE 1Source of Test IsolatesIsolateSourceIsolationGeographic OriginColletotrichum acutatum26255ATCC1TomatoNew ZealandColletotrichum acutatum42373ATCC1MangoAustraliaColletotrichum acutatum60468ATCC1VacciniumNew ZealandcorymbosumColletotrichum acutatum66367ATCC1StrawberryIndiana, USAColletotrichum acutatum38689ATCC1Pinusf.sp. pinearadiataColletotrichum44228ATCC1StylosanthesAustraliagiceosporicideshamata cv.VeranoColletotrichum38237ATCC1MangogloeosporioidesCladosporium carpophilum52935ATCC1PeachGeorgia, USACladosporium carpophilumBS-1Jones2PeachMichigan, USACladosporium carpophilumBS-2Jones2PeachMichigan, USACladosporium carpophilumBS-3Jones2PeachMichigan, USACladosporium carpophilumBS-4Jones2PeachMichigan, USACladosporium carpophilumBS-5Jones2PeachMichigan, USACladosporium carpophilumBS-6Jones2PeachMichigan, USAAlternaria alternata56835ATCC1Wheat grainEnglandAlternaria alternata34509ATCC1AppleJapanAlternaria alternata26294ATCC1TobaccoMaryland, USAAlternaria alternata60647ATCC1TomatoGreecef.sp. lycopersiciAlternaria alternata sensuAa001Pryor3AlmondlatoAlternaria alternata sensuAa002Pryor3AlmondlatoAlternaria alternata sensuAa003Pryor3AlmondlatoAlternaria alternata sensuAa004Pryor3AlmondlatoAlternaria alternata sensuAa005Pryor3AlmondlatoAlternaria alternata sensuAa006Pryor3AlmondlatoAlternaria sp.2000#47Novartis4AlmondCalifornia, USAAlternaria brassicae21-61-02Pryor3Alternaria brassicola2232Pryor3Alternaria radicina96831Pryor3Alternaria petroselini06-196Pryor3Alternaria dauci36613Pryor3Alternaria porri58175Pryor3Alternaria alternataP154Pryor3PistachioAlternaria tenuissimaP59Pryor3PistachioAlternaria arborescensP67Pryor3PistachioAlternaria infectoriaP60Pryor3PistachioAlternaria tenuissima34-015Pryor3Alternaria arborescens39-128Pryor3Alternaria infectoria27-193Pryor3Colletotrichum fragariae26010ATCC1BeanFlorida, USAColletotrichum fragariae58718ATCC1StrawberryFlorida, USAMonilinia laxa32671ATCC1NectarineCalifornia, USAMonilinia fructicola32670ATCC1PeachCalifornia, USAWhetzelinia sclerotiorum46762ATCC1CauliflowerAustraliaUnknown2000#69A1Novartis4AlmondCalifornia, USAUnknown2000#105CNovartis4AlmondCalifornia, USAUnknown2000#106A(2P)Novartis4AlmondCalifornia, USA1American Type Culture Collection; Rockville, MD, USA 2Jones, A.L.; Michigan State University, East Lansing, MI, USA (Strains documented in Phytopathology (1999) 89: 100-108) 3Pryor, B.; University of California, Davis, CA, USA 4Novartis Agribusiness Biotechnology Research, Inc.; Research Triangle Park, NC, USA



Example 2


DNA Extraction from Almond tissues

[0086] DNA was extracted from almond leaves by using a bulk maceration method with a modified version of the CTAB extraction buffer (Wang et al., 1993, “PCR amplification from single seeds, facilitating DNA marker-assisted breeding,” Nucleic Acids Res. 21:2527). The bulk maceration method was used to isolate DNA from several naturally infected tissues from the field. The potential concentration ranges of the buffer ingredients of the modified CTAB extraction buffer are as follows:


[0087] approximately 100 mM Tris, pH 8.0;


[0088] 0.2-2.0 M NaCl;


[0089] 1-200 mM ethylenediaminetetraacetic acid (EDTA);


[0090] 0. 1-5% w/v hexadecyltrimethylammonium (CTAB);


[0091] 0. 1-5% w/v polyvinylpyrolidine (PVP); and


[0092] 0.01-2% w/v ascorbic acid.


[0093] In other embodiments of the invention, the DNA extraction buffer comprises 100 mM Tris, pH 8.0; or comprises 1.4 M NaCl; or comprises 20 mM EDTA; or comprises 2% w/v CTAB; or comprises 2% w/v PVP; or comprises 0. 1% w/v ascorbic acid.


[0094] However, in the preferred embodiment of the bulk maceration method, the following concentrations are used: 100 mM Tris, pH 8.0; 1.4 M NaCl; 20 mM EDTA; 2% w/v CTAB; 2% w/v PVP and 0.1% w/v ascorbic acid.


[0095] The present invention provides a method for preparing an extract of DNA from tissue, comprising the steps of:


[0096] (a) taking a plurality of random tissue samples from an organism population;


[0097] (b) adding the DNA extraction buffer described above, to the tissue samples;


[0098] (c) macerating the tissue samples and extraction buffer to form an extract; and


[0099] (d) removing the extract from the macerated tissue and buffer.


[0100] In another embodiment, the method of extraction takes tissue samples from a plant population. In yet another embodiment, the tissue samples are selected from leaves, stems, roots, blossoms, immature flowers, peduncles, hulls, fruits, immature fruits, or woody tissue.


[0101] In a preferred embodiment the method of extraction uses the extraction buffer comprising: 100 mM Tris, pH 8.0; 1.4 M NaCl; 20 mM EDTA; 2% w/v CTAB; 2% w/v PVP and 0.1% w/v ascorbic acid.


[0102] DNA is extracted from almond tissues as follows:


[0103] Bulk Maceration Method:


[0104] (1) A sample consists of almond tissue taken from trees suspected of disease within a given orchard.


[0105] (2) Samples are handled individually using a different pair of gloves for each. Any implements used in preparing the samples are washed with water and then with 70% EtOH between each sample.


[0106] (3) Samples are separated into subsamples for testing according to tissue:


[0107] A. Blossoms, immature flowers, and peduncles.


[0108] B. Hulls from last season's almonds (mummies) and old crescents (immature fruit). Only the outer part of the almond fruit that was once fleshy and can now be separated from the shell of the nut is to be tested.


[0109] C. Hulls from fresh almonds and crescents from this season. Again, only the outer, fleshy part of the fruit is tested.


[0110] D. Woody tissue.


[0111] (4) The sample is placed in a Bioreba (Reinach, Switzerland) heavy duty plastic bag (cat#490100). The plant tissue is weighed, plastic bag with leaves minus the tare (weight of the plastic bag).


[0112] (5) A volume (mL) of well-mixed CTAB extraction buffer is added per gram fresh weight of sample according to the following:
2TissueVolume/WeightA. Blossoms, peduncles3 XB. Hulls, old almond fruit4 XC. Hulls, fresh almond fruit2 XD. Woody tissue2 X


[0113] CTAB extraction buffer: (100 mM Tris, pH 8.0; 1.4 M NaCl; 20 mM ethylenediaminetetraacetic acid (EDTA); 2% w/v hexadecyltrimethylammonium bromide (CTAB); 2% w/v polyvinylpyrolidine (PVP); and 0.1% w/v ascorbic acid.The tissue is macerated using a Bioreba Homex 6 homogenizer (Reinach, Switzerland, cat #400005) set at 90. The sample is ground until tissues appear as broken as possible to liberate fungal DNA.


[0114] (6) Once maceration is complete, the extraction is pressed into the bottom of the extraction bag. Using clean scissors cut the bag at a length to allow a 10 or 25 mL transfer pipet to reach the extraction without contaminating the pipettor.


[0115] (7) By pipetting up and down several times, the extraction juice is homogenized.


[0116] (8) One milliliter of extraction juice is transferred into each of two eppendorf tubes. One of these tubes is immediately frozen in storage for reference. The other is further processed.


[0117] (9) The test aliquot is boiled for five minutes. A centrifuge cap sleeve is used to ensure that the tube will not pop open.


[0118] (10) The boiled extracted is allowed to cool on ice for 2 minutes.


[0119] (11) The extraction is centrifuged at 15,000×G for 5 minutes.


[0120] (12) Extracts are either diluted and tested directly (13A) or nucleic acids are purified from them prior to testing (13B).


[0121] (13A). Extracts are diluted for testing. Extraction supernatant is added to ice-cold water according to the following scheme:
3TissuemL CTAB/g tissueDilution TestedE. Blossoms, peduncles3 X1:67 F. Hulls, old almond fruit4 X1:50 G. Hulls, fresh almond fruit2 X1:100H. Woody tissue2 X1:100


[0122] (13B) Nucleic acids are purified from almond extracts by performing an equal volume 25:24:1 phenol:chloroform:isoamyl alcohol extraction on 1 mL of homogenized extraction juice. The aqueous phase of this extraction is transferred to a fresh microcentrifuge tube and 0.5 volumes of ice-cold isopropanol are added. After incubation for 20 minutes at −20° C., the precipitate is spun down at 15,000 rpm for 10 minutes. The supernatant is discarded and the pellet is washed with 0.7 mL of 70% ethanol. The wash is discarded and the pellet allowed to dry. The pellet is resuspended in Tris EDTA buffer (10 mM Tris base, I mM EDTA, pH 8.0) with RNase added at a concentration of 10 mg/mL. The DNA concentration can be read on a spectrophotometer and adjusted to 100 ng/μL by addition of TE buffer.
4TABLE 2Source of almond tissues usedSample IdentificationTissue typeOrigin (City, California, USA)1999#3Almond hullsEscalon1999#5Almond hulls1999#11Almond hullsModesto1999#41Almond hullsChico1999#42Almond hullsChico1999#104Almond hullsSalida1999#109BAlmond hullsModesto1999#118DAlmond hullsTurlock2000#8Almond hullsRipon2000#11Almond hullsTurlock2000#19Almond hullsHughson2000#31AMummified fruitRipon2000#JA-1AFlower blossoms2000#59BFlower blossoms and crescentsGridley



Example 3


Polymerase Chain Reaction Amplification

[0123] Polymerase chain reactions are performed with the GeneAmp Kit from Perkin-Elmer (Foster City, Calif.; part no. N808-0009) using 50 mM KCl, 2.5 mM MgCl2, 10 mM Tris-HCl, pH8.3, containing 200 μM of each dTTP, dATP, dCTP, and dGTP in either 25 or 50 μL reactions containing 50 μM each primer, 0.25 U/μL of Taq polymerase and 0.2ng/μL of genomic DNA. Reactions are run for 30-40 cycles of 15 s at 94° C., 15 s at 50° C.-70° C., and 45 s at 72° C. in a Perkin-Elmer Model 9600 or 9700 thermal cycler. The products are analyzed by loading 10 μl of each PCR sample on a 1.0% agarose gel and electrophoresing.



Example 4


Synthesis and Purification of Oligonucleotides

[0124] Oligonucleotides (primers) are synthesized by, for example, either Integrated DNA Technologies (Coralville, Iowa) or Midland Certified Reagent Company (Midland, Tex.).



Example 5


Cloning and sequencing of ITS region rDNA

[0125] ITS region sequences are PCR-amplified using conserved primers ITS1 and ITS4 (SEQ-ID-NO: 1 and 4) as described in Example 3. Products cloned into the pCR®2.1-TOPO TA-cloning vector using the TOPO-TA Cloning Kit (Invitrogen, Carlsbad, Calif.; part no. K4550-40) according to manufacturer's directions. Clones containing the ITS fragment inserts are sequenced using the TA cloning vector's FORWARD (5′-gtaaaacgacggccagt-3′; SEQ ID NO:5) and REVERSE (5′-caggaaacagctatgac-3′; SEQ ID NO:6) primers. Sequencing is performed on an ABI PRISM 377™ DNA sequencer (Perkin Elmer Applied Biosystems, Foster City, Calif.).



Example 6


Design of species-specific PCR primers

[0126] Example 6 is broken down into three subsections describing details of the design of specific primers for Colletotrichum acutatum, Alternaria spp., and Cladosporium carpophilum. A few common steps are involved in the design of primers for the three target species. In the design of each assay, Internal Transcribed Spacer region DNA sequences are obtained either from the GenBank database of the National Center for Biotechnology Information (www.ncbi.nlm.nih.gov) or from PCR-amplified and sequenced DNA from isolates in Example 1 according to the protocol in Example 5. A multiple sequence alignment is made of these sequences. The alignment is analyzed for divergences among the target sequences and among sequences for other fungal DNAs. The divergences permit the development of primers that will specifically amplify target sequences in PCR reactions. Oligonucleotide primers are designed to target regions that contain the greatest differences in sequence among the species analyzed (See individual tables 4-7). These primers are synthesized according to Example 4. In addition, the published ribosomal gene-specific primers ITS1, ITS2, ITS3 and ITS4 (White et al., 1990;.In: PCR Protocols; Eds.: Innes et al. pages 315-322) are synthesized for testing in combination with the primers specific for the ITS regions. The conserved fungal ITS region primers are shown in Table 3.
5TABLE 3Conserved primers designed for amplification of fungal ITS region DNANameOligo Sequence (5′→3′)TargetIdentifierITS1TCCGTAGGTGAACCTGCGGFungal Nuclear rDNA ITS regionSEQ-ID-NO:1ITS2GCTGCGTTCTTCATCGATGCFungal Nuclear rDNA ITS regionSEQ-ID-NO:2ITS3GCATCGATGAAGAACGCAGCFungal Nuclear rDNA ITS regionSEQ-ID-NO:3ITS4TCCTCCGCTTATTGATATGCFungal Nuclear rDNA ITS regionSEQ-ID-NO:4



Example 6A


Design of Colletotrichum acutatum -specific PCR primers

[0127] Primers are designed for the specific detection of Colletotrichum acutatum. Internal Transcribed Spacer region I DNA sequences for C. acutatumare obtained from the GenBank database. Those sequences include accession numbers Z32907, Z32913, Z32915, Z32916, Z32917, Z32918, Z32921, Z32922, Z32924, Z32925, Z32926, and Z32928. A multiple sequence alignment is made of these sequences along with ITS I region sequences for other almond pathogens (Z32930 for Colletotrichum coccodes; Z32938, C.dematium; Z32943, C.fragariae; Z32961, C.gloeosporioides; Z32981, C.graminicola; Z32984, C.linicola; Z33000, C.trichellum). The alignment is analyzed for divergences between the target sequences and sequences for other fungal DNAs. The divergences permit the development of primers that will specifically amplify C. acutatum ITS region DNA when used in PCR reactions. Oligonucleotide primers JB677, JB677. 1, JB677.2, JB677.3 and JB678 (SEQ-ID-NO: 10, 28, 29, 30 and 11, respectively) are designed to target the ITS region 1 DNA of C. acutatum. Primers JB677, JB677.1, JB677.2, and JB677.3 are targeted to the same region of ITS1 and demonstrate how adding or removing bases to a primer that contains a target-specific sequence can produce a diverse number of oligonucleotides for use in the detection of the same target.


[0128] SEQ-ID-NO: 7 Oligonucleotide Primer CaINT-1


[0129] SEQ-ID-NO: 8 Oligonucleotide Primer CaINT-2


[0130] SEQ-ID-NO: 9 Oligonucleotide Primer CaInt2


[0131] In a similar alignment obtained from the literature (Bailey et al., Phytopathology 86: 1076-1083), ITS region 2 DNA sequences of several Colletotrichum species are compared. The alignment in this report is used to find divergences among the species compared for the design of a C. acutatum ITS region 2 primer. Oligonucleotide primer JB679 (SEQ-ID-NO: 12) is designed to target ITS region 2 DNA of C. acutatum. The C. acutatum specific primers are shown in Table 4. These primers may be used in combination with one another, with one of the conserved primers in Table 3, or with one of the C. acutatum specific primers from the literature (Primers CaINT-1, 5′-GGCGCCGGCCCCCACCACGGGGA-3′and CaINT-2, 5′- GGCGCCGGCCCCGTCACGGGGG-3′ referenced in Adaskaveg and Hartin, Phytopathology 87:979-987, or primer CaInt2, 5′ - GGGGAAGCCTCTCGCGG-3′ referenced in Sreenivasaprasad et al. Plant Pathology (1996) 45, 650-655) to target C. acutatum DNA.
6TABLE 4Primers designed for detection ofColletotrichum acutatumOligonucleotideNamesequence (5′→3′)IdentifierJB677CGGGCAGGGGAAGCCTCSEQ-ID-NO:10JB678GGAAGCCTCTCGCGGGCSEQ-ID-NO:11JB679ATCCCAGTGCGAGACGTTAGSEQ-ID-NO:12JB677.1GCGGGCAGGGGAAGCCTCTSEQ-ID-NO:28JB677.2CGGCGGGCAGGGGAAGCCTCTSEQ-ID-NO:29JB677.3GTTGCTTCGGCGGGCAGGGGAASEQ-ID-NO:30



Example 6B


Design of Alternaria spp. -specific PCR primers

[0132] Primers are designed for the specific detection of Alternaria-spp. ITS region DNA sequences for A. alternata were obtained as described in Example 5 for four ATCC isolates (56835, 34509, 26294, and 60647) as well as plate isolates obtained from almond sample 2000#47 (See Table 1 for more information on isolates). Additionally, GenBank sequences for the A. alternata ITS region were obtained (Accession # AF229461, AF229460, AF229459, AF218791, AJ276059, AJ276055, and AF071346). These sequences were aligned in SeqMan II ver 3.6.0 (DNAStar, Madison, Wis., U.S.A.). A consensus sequence of these sequences was generated and labeled “Alternaria ITS sequence”.


[0133] A multiple sequence alignment is made of this sequence along with ITS region sequences for other almond pathogens. These include sequences obtained from GenBank for Colletotrichum gloeosporioides (Accession #AF090855), C. acutatum (AF090853), C. fragariae (AF090854), Venturia carpophila (syn. Fusicladium carpophilum, Cladosporium carpophilum) (AF065849), Monilinia fructigena (Z73781), M laxa (Z73786), Sclerotinia sclerotiorum (Z73799), and Botrytis cinerea (Z73765). An ITS region sequence generated as in Example 5 for ATCC Fusicladium carpophilum isolate 52935 is also included in the multiple sequence alignment.


[0134] The alignment is analyzed for divergences between the A. alternata consensus sequence target and other fungal sequences. The divergences found allow for the development of primers that will specifically amplify Alternaria spp. ITS region DNA when used in PCR reactions. Oligonucleotide primers Alal-1, Alal-2, Alal-3, Alal-4, alal-5, and Alal-6 (SEQ-ID-NOs: 13-18) are designed to target the ITS region DNA of Alternaria spp. (Table 5).


[0135] Additionally, these primers can be used with conserved ITS region primers in Table 3 as well as other ITS derived Alternaria spp. primers found in the literature (primers altl, 5′-ATTGCAATCAGCGTCAGTAAC-3′ and alt2, 5-CAAGCAAAGCTTGAGGGTACA-3′Zur et al. 1999. J. Food Protection 62(10) p 1191-1197) (SEQ-ID-NOs: 19 and 20, respectively).
7TABLE 5Primers designed for detection of Alternaria spp.Oligonucleotide sequenceName(5′->3′)IdentifierAlal-1AAATATGAAGGCGGGCTGGASEQ-ID-NO:13Alal-2AGACCTTTGCTGATAGAGAGTGCGASEQ-ID-NO:14Alal-3CCTTTGCTGATAGAGAGTGCGACTTSEQ-ID-NO:15Alal-4CTCGGGGTTACAGCCTTGCTSEQ-ID-NO:16Alal-5AACCTCTCGGGGTTACAGCCTTGCTSEQ-ID-NO:17Alal-6TGATAGAGAGTGCGACTTGTSEQ-ID-NO:18



Example 6C


Design of Cladosporium carpophilum-specific PCR Primers

[0136] Primers are designed for the specific detection of Cladosporium carpophilum. ITS region DNA sequences for C. carpophilum were obtained as described in Example 5 for six isolates (BS-1, BS-2, BS-3, BS-4, BS-6, and ATCC isolate 52935). One additional sequence for C. carpophilum ITS region DNA was obtained from GenBank (Accession # AF065489). These sequences were aligned in SeqMan II ver 3.6.0 (DNAStar, Madison, Wis., U.S.A.). A consensus sequence of these sequences was generated and labeled “Vcarpophila consensus”.


[0137] A multiple sequence alignment is made of this sequence along with ITS region sequences for other almond pathogens. These include sequences obtained from GenBank for Colletotrichum gloeosporioides (Accession #AF090855), C. acutatum (AF090853), C. fragariae (AF090854), Monilinia fructigena (Z73781), M. laxa (Z73786), Sclerotinia sclerotiorum (Z73799), and Botrytis cinerea (Z73765). The consensus sequence generated in Example 6B for multiple Alternaria alternata sequences is also included in the multiple sequence alignment.


[0138] The alignment is analyzed for divergences between the C. carpophilum consensus sequence target and other fungal sequences. The divergences found allow for the development of primers that will specifically amplify C. carpophilum ITS region DNA when used in PCR reactions. Oligonucleotide primers Vcarp1, Vcarp2, Vcarp3, Vcarp4, Vcarp5, Vcarp6, and Vcarp7 (SEQ-ID-NOs: 21-27) are designed to target the ITS region of C. carpophilum (Table 6). These primers can be used with conserved ITS region primers in Table 3.
8TABLE 6Primers designed for detection ofCladosporium carpophilumOligonucleotideNamesequence (5′->3′)IdentifierVcarp1TGCCGGAATCAGCAAGCCCTSEQ-ID-NO:21Vcarp2CAACCGCGGCCCGGATSEQ-ID-NO:22Vcarp3TCAGCAAGCCCTGCCTAGAASEQ-ID-NO:23Vcarp4GTCTGAGGAGAAAGCCAAACGASEQ-ID-NO:24Vcarp5GCTCCGGGCGAGGGATSEQ-ID-NO:25Vcarp6GCGACGGCGCCTACGGGTTTSEQ-ID-NO:26Vcarp7CCGGGCGAGGGATTTCTCTTSEQ-ID-NO:27



Example 7


Determination of Primer Specificity to Purified Fungal Genomic DNA

[0139] PCRs are performed according to Example 3 using different primer combinations (Table 7) in an attempt to amplify single specific fragments. Specific PCR amplification products are produced from primers designed from the nuclear rDNA ITS regions of each fungal species of interest.


[0140] In an initial screen for specificity, PCR reaction mixtures are made according to Example 3 for each of the primer combinations in Table 7. These are run against a negative control (no DNA added), a healthy almond tissue control (prepared as in Example 2) to test for background amplification, and 10 ng of fungal DNA for each of the known species listed in Table 1 prepared as described in example 1.
9TABLE 7Possible combinations of PCR primers for the specific amplification ofColletotrichum acutatum, Alternaria spp., and Cladosporium carpophilum.TargetPathogen5′ primer3′ primerC. acutatumCaINT-1 (SEQ-ID-NO: 7)JB679 (SEQ-ID-NO: 12)C. acutatumCaINT-2 (SEQ-ID-NO: 8)JB679 (SEQ-ID-NO: 12)C. acutatumCaInt2 (SEQ-ID-NO: 9)JB679 (SEQ-ID-NO: 12)C. acutatumJB677.1 (SEQ-ID-NO: 28)JB679 (SEQ-ID-NO: 12)C. acutatumJB677.1 (SEQ-ID-NO: 28)ITS4 (SEQ-ID-NO: 4)C. acutatumJB677.1 (SEQ-ID-NO: 28)ITS2 (SEQ-ID-NO: 2)C. acutatumJB677.2 (SEQ-ID-NO: 29)JB679 (SEQ-ID-NO: 12)C. acutatumJB677.2 (SEQ-ID-NO: 29)ITS4 (SEQ-ID-NO: 4)C. acutatumJB677.2 (SEQ-ID-NO: 29)ITS2 (SEQ-ID-NO: 2)C. acutatumJB677.3 (SEQ-ID-NO: 30)JB679 (SEQ-ID-NO: 12)C. acutatumJB677.3 (SEQ-ID-NO: 30)ITS4 (SEQ-ID-NO: 4)C. acutatumJB677.3 (SEQ-ID-NO: 30)ITS2 (SEQ-ID-NO: 2)C. acutatumJB677 (SEQ-ID-NO: 10)JB679 (SEQ-ID-NO: 12)C. acutatumJB677 (SEQ-ID-NO: 10)ITS4 (SEQ-ID-NO: 4)C. acutatumJB677 (SEQ-ID-NO: 10)ITS2 (SEQ-ID-NO: 2)C. acutatumJB678 (SEQ-ID-NO: 11)JB679 (SEQ-ID-NO: 12)C. acutatumJB678 (SEQ-ID-NO: 11)ITS4 (SEQ-ID-NO: 4)C. acutatumJB678 (SEQ-ID-NO: 11)ITS2 (SEQ-ID-NO: 2)C. acutatumITS1 (SEQ-ID-NO: 1)JB679 (SEQ-ID-NO: 12)C. acutatumITS3 (SEQ-ID-NO: 3)JB679 (SEQ-ID-NO: 12)Alternaria spp.Alal-4 (SEQ-ID-NO: 16)ITS2 (SEQ-ID-NO: 2)Alternaria spp.Alal-4 (SEQ-ID-NO: 16)Alt2 (SEQ-ID-NO: 20)Alternaria spp.Alal-4 (SEQ-ID-NO: 16)Alal-2 (SEQ-ID-NO: 14)Alternaria spp.Alal-4 (SEQ-ID-NO: 16)Alal-3 (SEQ-ID-NO: 15)Alternaria spp.Alal-4 (SEQ-ID-NO: 16)Alal-6 (SEQ-ID-NO: 18)Alternaria spp.Alal-5 (SEQ-ID-NO: 17)ITS4 (SEQ-ID-NO: 4)Alternaria spp.Alal-5 (SEQ-ID-NO: 17)ITS2 (SEQ-ID-NO: 2)Alternaria spp.Alal-5 (SEQ-ID-NO: 17)Alt2 (SEQ-ID-NO: 20)Alternaria spp.Alal-5 (SEQ-ID-NO: 17)Alal-2 (SEQ-ID-NO: 14)Alternaria spp.Alal-5 (SEQ-ID-NO: 17)Alal-3 (SEQ-ID-NO: 15)Alternaria spp.Alal-5 (SEQ-ID-NO: 17)Alal-6 (SEQ-ID-NO: 18)Alternaria spp.Alt1 (SEQ-ID-NO: 19)Alal-2 (SEQ-ID-NO: 14)Alternaria spp.Alt1 (SEQ-ID-NO: 19)Alal-3 (SEQ-ID-NO: 15)Alternaria spp.Alt1 (SEQ-ID-NO: 19)Alal-6 (SEQ-ID-NO: 18)Alternaria spp.ITS1 (SEQ-ID-NO: 1)Alal-2 (SEQ-ID-NO: 14)Alternaria spp.ITS1 (SEQ-ID-NO: 1)Alal-3 (SEQ-ID-NO: 15)Alternaria spp.ITS1 (SEQ-ID-NO: 1)Alal-6 (SEQ-ID-NO: 18)Alternaria spp.ITS3 (SEQ-ID-NO: 3)Alal-2 (SEQ-ID-NO: 14)Alternaria spp.ITS3 (SEQ-ID-NO: 3)Alal-3 (SEQ-ID-NO: 15)Alternaria spp.ITS3 (SEQ-ID-NO: 3)AlaI-6 (SEQ-ID-NO: 18)C. carpophilumVcarp1 (SEQ-ID-NO: 21)Vcarp5 (SEQ-ID-NO: 25)C. carpophilumVcarp1 (SEQ-ID-NO: 21)Vcarp6 (SEQ-ID-NO: 26)C. carpophilumVcarp1 (SEQ-ID-NO: 21)Vcarp7 (SEQ-ID-NO: 27)C. carpophilumVcarp1 (SEQ-ID-NO: 21)ITS4 (SEQ-ID-NO: 4)C. carpophilumVcarp1 (SEQ-ID-NO: 21)ITS2 (SEQ-ID-NO: 2)C. carpophilumVcarp2 (SEQ-ID-NO: 22)Vcarp5 (SEQ-ID-NO: 25)C. carpophilumVcarp2 (SEQ-ID-NO: 22)Vcarp6 (SEQ-ID-NO: 26)C. carpophilumVcarp2 (SEQ-ID-NO: 22)Vcarp7 (SEQ-ID-NO: 27)C. carpophilumVcarp2 (SEQ-ID-NO: 22)ITS4 (SEQ-ID-NO: 4)C. carpophilumVcarp2 (SEQ-ID-NO: 22)ITS2 (SEQ-ID-NO: 2)C. carpophilumVcarp3 (SEQ-ID-NO: 23)Vcarp5 (SEQ-ID-NO: 25)C. carpophilumVcarp3 (SEQ-ID-NO: 23)Vcarp6 (SEQ-ID-NO: 26)C. carpophilumVcarp3 (SEQ-ID-NO: 23)Vcarp7 (SEQ-ID-NO: 27)C. carpophilumVcarp3 (SEQ-ID-NO: 23)ITS4 (SEQ-ID-NO: 4)C. carpophilumVcarp3 (SEQ-ID-NO: 23)ITS2 (SEQ-ID-NO: 2)C. carpophilumVcarp4 (SEQ-ID-NO: 24)Vcarp5 (SEQ-ID-NO: 25)C. carpophilumVcarp4 (SEQ-ID-NO: 24)Vcarp6 (SEQ-ID-NO: 26)C. carpophilumVcarp4 (SEQ-ID-NO: 24)Vcarp7 (SEQ-ID-NO: 27)C. carpophilumVcarp4 (SEQ-ID-NO: 24)ITS4 (SEQ-ID-NO: 4)C. carpophilumVcarp4 (SEQ-ID-NO: 24)ITS2 (SEQ-ID-NO: 2)C. carpophilumITS1 (SEQ-ID-NO: 1)Vcarp5 (SEQ-ID-NO: 25)C. carpophilumITS1 (SEQ-ID-NO: 1)Vcarp6 (SEQ-ID-NO: 26)C. carpophilumITS1 (SEQ-ID-NO: 1)Vcarp7 (SEQ-ID-NO: 27)C. carpophilumITS3 (SEQ-ID-NO: 3)Vcarp5 (SEQ-ID-NO: 25)C. carpophilumITS3 (SEQ-ID-NO: 3)Vcarp6 (SEQ-ID-NO: 26)C. carpophilumITS3 (SEQ-ID-NO: 3)Vcarp7 (SEQ-ID-NO: 27)


[0141] When visualized on an ethidium bromide stained gel several primer pairs give satisfactory results: good amplification of target DNA from multiple isolates of the target species with all other reactions (negative control, almond background, and other fungal DNAs) free of both specific and nonspecific reaction products. Some give unsatisfactory results including nonspecific amplification, no amplification of target DNA, and amplification of DNAs from fungal species other that the target. The primer pairs that give the good amplification for their specific targets with no cross-amplification are summarized in Table 8.
10TABLE 8PCR primer pairs providing specific and sensitive amplificationof target DNA for Colletotrichum acutatum, Alternaria spp., andCladosporium carpophilum PCR assays.TargetPathogen5′ primer3′ primerC. acutatumJB677.3 (SEQ-ID-NO: 30)ITS4 (SEQ-ID-NO: 4)C. acutatumJB677 (SEQ-ID-NO: 27)ITS4 (SEQ-ID-NO: 4)Alternaria spp.Alal-4 (SEQ-ID-NO: 16)Alal-2 (SEQ-ID-NO: 12)Alternaria spp.Alal-4 (SEQ-ID-NO: 16)Alal-6 (SEQ-ID-NO: 18)Alternaria spp.Alal-5 (SEQ-ID-NO: 17)Alal-2 (SEQ-ID-NO: 12)C. carpophilumITS1 (SEQ-ID-NO: 1)Vcarp7 (SEQ-ID-NO: 27)C. carpophilumVcarp4 (SEQ-ID-NO: 24)Vcarp5 (SEQ-ID-NO: 25)C. carpophilumVcarp1 (SEQ-ID-NO: 21)ITS4 (SEQ-ID-NO: 4)



Example 7


Validation of Almond Pathogen PCR Assays Against a Panel of Almond Tissue DNA Extractions

[0142] For the primer pairs that give the best amplification of their given targets (JB677.3 with ITS4 for C. acutatum, Alal-4 with Alal-2 for Alternaria spp., and ITS1 with Vcarp7 for C. carpophilum), each is run in PCR reactions against a panel of almond tissue extractions prepared as in Example 2 on tissues listed in Table 2. In this experiment, extractions from sample designated as “1999” are diluted and tested directly. Nucleic acids are purified from extractions on samples designated as “2000” and then tested at a 100 ng per reaction concentration. Results are scored as either positive (+) or negative (−) with any product visible being considered a positive and with nonspecifics recorded if present. Results of these tests are shown in Table 9.
11TABLE 9Results of almond pathogen PCR assays against a panel ofAlmond tissue DNA extractions.SampleColletotrichumAlternariaCladosporiumIdentificationTissue Typeacutatumspp.carpophilum1999#3Almond hulls++1999#5Almond hulls++1999#11Almond hulls+1999#41Almond hulls1999#42Almond hulls+1999#104Almond hulls++1999#109BAlmond hulls++1999#118DAlmond hulls+2000#8Almond hulls++2000#19Almond hulls2000#31AMummified fruit+2000#JA-1AFlower blossoms+2000#59BFlower blossoms andcrescents


[0143] For the thirteen isolates tested, the assays detect and differentiate Colletotrichum acutatum, Alternaria spp., and Cladosporium carpophilum in almond extractions. This experiment demonstrates the utility of these primers in directly characterizing almond tissue extractions for the presence of disease.



Example 8


Validation of Almond Pathogen PCR Assays Against a Panel of Unknown Fungal Isolates Collected from Almond Tissues

[0144] DNAs are extracted from unknown fungal isolates (Table 1, bottom) collected from almond samples by the method in Example 1. These purified DNA extracts are tested using PCR reaction mixtures made according to Example 3 for each of the primer combinations in Table 8. Table 10 shows the utility of these assays in the characterization of purified fungal isolates grown from almond tissues.
12TABLE 10Results of almond pathogen PCR assays against a panel ofUnknown fungal isolates from field-grown almonds.SampleColletotrichumAlternariaCladosporiumIdentificationAcutatumspp.carpophilum2000#69A1+2000#105C+2000#106A(2P)+


[0145] All references cited herein are incorporated by reference in their entireties.


Claims
  • 1. An oligonucleotide primer selected from the group consisting of SEQ ID NOS: 10-30.
  • 2. A pair of oligonucleotide primers, wherein said pair consists of at least one primer of claim 1.
  • 3. A pair of oligonucleotide primers, selected from the group consisting of: a) SEQ ID NO: 30 and SEQ ID NO:4; b) SEQ ID NO:27 and SEQ ID NO:4; c) SEQ ID NO:16 and SEQ ID NO:12; d) SEQ ID NO:16 and SEQ ID NO:18; e) SEQ ID NO:17 and SEQ ID NO:12; f) SEQ ID NO:1 and SEQ ID NO:27; g) SEQ ID NO:24 and SEQ ID NO:25; and h) SEQ ID NO:21 and SEQ ID NO:4.
  • 4. A pair of oligonucleotide primers, wherein said pair consists of SEQ ID NO:16 and SEQ ID NO:12.
  • 5. A pair of oligonucleotide primers, wherein said pair consists of SEQ ID NO:16 and SEQ ID NO:18.
  • 6. A pair of oligonucleotide primers, wherein said pair consists of SEQ ID NO:17 and SEQ ID NO:12.
  • 7. A pair of oligonucleotide primers, wherein said pair consists of SEQ ID NO:24 and SEQ ID NO:25.
  • 8. A method for the detection of a fungal pathogen, comprising the steps of: (a) isolating DNA from a plant tissue infected with a pathogen; (b) subjecting said DNA to polymerase chain reaction amplification using at least one primer according to claim 1; and (c) detecting said fungal pathogen by visualizing the product or products of said polymerase chain reaction amplification.
  • 9. The method of claim 8, wherein said fungal pathogen is Colletotrichum acutatum, Alternaria spp., and Cladosporium carpophilum.
  • 10. A method for the detection of a fungal pathogen, comprising the steps of: (a) isolating DNA from a plant tissue infected with said fungal pathogen; (b) amplifying a part of the Internal Transcribed Spacer sequence of said fungal pathogen using said DNA as a template in a polymerase chain reaction with a pair of primers according to claim 2; and (c) detecting sad fungal pathogen by visualizing the amplified part of the Internal Transcribed Spacer sequence.
  • 11. The method of claim 10, wherein said fungal pathogen is Colletotrichum acutatum, Alternaria spp., and Cladosporium carpophilum.
  • 12. The method of claim 10, wherein said pair of primers is according to claim 3.
  • 13. The method of claim 10, wherein said pair of primers is according to claim 4.
  • 14. The method of claim 10, wherein said pair of primers is according to claim 5.
  • 15. The method of claim 10, wherein said pair of primers is according to claim 6.
  • 16. The method of claim 10, wherein said pair of primers is according to claim 7.
  • 19. A diagnostic kit used in detecting a fungal pathogen, comprising the primer of claim 1.
  • 20. A diagnostic kit used in detecting a fungal pathogen, comprising the pair of primers of claim 2.
  • 21. A diagnostic kit used in detecting a fungal pathogen, comprising the pair of primers of claim 3.
  • 22. A diagnostic kit used in detecting a fungal pathogen, comprising the pair of primers of claim 4.
  • 23. A diagnostic kit used in detecting a fungal pathogen, comprising the pair of primers of claim 5.
  • 24. A diagnostic kit used in detecting a fungal pathogen, comprising the pair of primers of claim 6.
  • 25. A diagnostic kit used in detecting a fungal pathogen, comprising the pair of primers of claim 7.
  • 26. A DNA extraction buffer, comprising: (a) approximately 100 mM Tris, pH 8.0; (b) 0.2-2.0 M NaCl; (c) 1-200 mM ethylenediaminetetraacetic acid (EDTA); (d) 0.1-5% w/v hexadecyltrimethylammonium (CTAB); (e) 0.1-5% w/v polyvinylpyrolidine (PVP); and (f) 0.01-2% w/v ascorbic acid.
  • 27. The DNA extraction buffer of claim 26, comprising: 100 mM Tris, pH 8.0; 1.4 M NaCl; 20 mM EDTA; 2% w/v CTAB; 2% w/v PVP and 0.1% w/v ascorbic acid.
  • 28. The DNA extraction buffer of claim 26, comprising 100 mM Tris, pH 8.0.
  • 29. The DNA extraction buffer of claim 26, comprising 1.4 M NaCl.
  • 30. The DNA extraction buffer of claim 26, comprising 20 mM EDTA.
  • 31. The DNA extraction buffer of claim 26, comprising 2% w/v CTAB.
  • 32. The DNA extraction buffer of claim 26, comprising 2% w/v PVP.
  • 33. The DNA extraction buffer of claim 26, comprising 0.1% w/v ascorbic acid.
  • 34. A method for preparing an extract of DNA from tissue, comprising the steps of: (a) taking a plurality of random tissue samples from an organism population; (b) adding the extraction buffer of claim 26, to the tissue samples; (c) macerating the tissue samples and extraction buffer to form an extract; and (d) removing the extract from the macerated tissue and buffer.
  • 35. The method of claim 34, wherein the organism population is a plant population.
  • 36. The method of claim 35, wherein the tissue samples are selected from leaves, stems, roots, blossoms, immature flowers, peduncles, hulls, fruits, immature fruits, or woody tissue.
  • 37. The method of claim 34, wherein the extraction buffer comprises: 100 mM Tris, pH 8.0; 1.4 M NaCl; 20 mM EDTA; 2% w/v CTAB; 2% w/v PVP and 0.1% w/v ascorbic acid.
  • 38. A method for performing PCR analysis on DNA extracted from tissue, comprising the steps of: (a) taking a plurality of random tissue samples from an organism population; (b) adding the extraction buffer of claim 26, to the tissue samples; (c) macerating the tissue samples and extraction buffer to form an extract; (d) removing the extract from the macerated tissue and buffer; and (e) performing PCR analysis on the extract.
  • 39. The method of claim 38, further comprising the step of boiling the extract after removing it from the macerated tissue and buffer.
  • 40. The method of claim 39, further comprising the step of diluting the extract.
  • 41. The method of claim 40, wherein the organism population is a plant population.
  • 42. The method of claim 41, wherein the tissue samples are selected from leaves, stems, roots, blossoms, immature flowers, peduncles, hulls, fruits, immature fruits, or woody tissue.
  • 43. The method of claim 38, wherein the extraction buffer comprises: 100 mM Tris, pH 8.0; 1.4 M NaCl; 20 mM EDTA; 2% w/v CTAB; 2% w/v PVP and 0.1% w/v ascorbic acid.
  • 44. The method of claim 41, wherein the plant tissue is from a stone fruit plant population.
  • 45. The method of claim 8, wherein the plant tissue is from a stone fruit plant.
  • 46. The method of claim 8, wherein the plant tissue is from an almond plant.
Provisional Applications (1)
Number Date Country
60274540 Mar 2001 US
Divisions (1)
Number Date Country
Parent 09939379 Aug 2001 US
Child 10623880 Jul 2003 US