CA2009708A1 - Nucleic acid probe for the detection of salmonella human pathogens - Google Patents
Nucleic acid probe for the detection of salmonella human pathogensInfo
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- CA2009708A1 CA2009708A1 CA002009708A CA2009708A CA2009708A1 CA 2009708 A1 CA2009708 A1 CA 2009708A1 CA 002009708 A CA002009708 A CA 002009708A CA 2009708 A CA2009708 A CA 2009708A CA 2009708 A1 CA2009708 A1 CA 2009708A1
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- Prior art keywords
- probe
- subgroup
- nucleic acid
- salmonella
- protein
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- C—CHEMISTRY; METALLURGY
- C12—BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
- C12Q—MEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
- C12Q1/00—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
- C12Q1/68—Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
- C12Q1/6876—Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes
- C12Q1/6888—Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes for detection or identification of organisms
- C12Q1/689—Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes for detection or identification of organisms for bacteria
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- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y02—TECHNOLOGIES OR APPLICATIONS FOR MITIGATION OR ADAPTATION AGAINST CLIMATE CHANGE
- Y02A—TECHNOLOGIES FOR ADAPTATION TO CLIMATE CHANGE
- Y02A50/00—TECHNOLOGIES FOR ADAPTATION TO CLIMATE CHANGE in human health protection, e.g. against extreme weather
- Y02A50/30—Against vector-borne diseases, e.g. mosquito-borne, fly-borne, tick-borne or waterborne diseases whose impact is exacerbated by climate change
Abstract
Abstract of the Invention Described herein are nucleic acid probes that can detect Salmonella human pathogens. The probes are generated from the nucleotide sequences of a gene encoding a virulence factor involved in the pathogenesis of Salmonella, especially the Type 1 fimbriae protein. The most preferred lengths of the probes range from about 20 to about 100 nucleotide bases in length. The probes are highly specific and sensitive for detecting Salmonella organisms pathogenic to humans. They are thus clinically useful in the detection of infection in diarrhea specimens. Additionally, they may be used in the detection of food-borne Salmonella, the causative agent of most salmonellosis in humans.
Description
~0~'7l)8 NUCLEIC AÇID PROBE FOR THE DETECTION OF SALMONE A HUMAN
PATHOGENS
_eld of ~he Invention:
Described herein are nucleic acid probes that can detect Salmonella human pathogens. The probes are generated fro~ the nucleotide sequence of a gene encoding a protein factor involved in the pathogenesis of Salmon~ll~, especially the Type 1 fimbrial protein.
Backqround of the Invention:
Microorganisms from the genus Salmonella are responsible for the majority of cases of bacterial diarrhea occurring in humans. Typically, screening and identification of a Salmonella infection is accomplished by microbial culturing techniques followed by biochemical testing. This takes from one to three days, sometimes ending in equivocal results. Identification of Salmonella spp. by use of an assay using DNA probes would be less labor intensive for the clinician, provide unequivocal results, and would enable quicker diagnosis of salmonellosis.
Nucleic acid hybridization technology is a new approach in the diagnostic industry. This methodology e~ploits the property that sequences unique to an organism comprise its genome. In a hybridization test, a po~itiYe signal is generated when these unique genomic sequences in the bacterial or the viral target hybridize with nucleic acid probes, which are tagged with a detection label.
U.S. Patent No. 4,689,295 to Taber, et al. describes Salmonella DNA probes which are Salmonella DNA fragments - 35 common to more than 80% of the known Salmonella species.
~RD-77 q~8 The fragments do not code for any protein or any other material known to contribute to pathogenicity. Thus, the probes are constructed ~rom a library of fragments without regard to ~enetic function, and are principally ùsed to detect the presence of SalmQ~Lella in a food sample.
U.S. Patent Mo. 4,358,535 to Falkow, et al. describes a method for detecting microorganisms using a DNA probe by affixing the genetic material from a sample containing the microorganism to an inert support and treating the sample to render the genetic material in a single-stranded form.
The fixed material is then contacted with a labeled nucleotide sequence that is substantially complementary to a nucleotide sequence of a structural gene encoding for toxins produced by the microorganisms. E. coli is the only organism exemplified in the patent, although Salmonell~ is mentioned in a laundry list of toxin-producing microorganisms.
PATHOGENS
_eld of ~he Invention:
Described herein are nucleic acid probes that can detect Salmonella human pathogens. The probes are generated fro~ the nucleotide sequence of a gene encoding a protein factor involved in the pathogenesis of Salmon~ll~, especially the Type 1 fimbrial protein.
Backqround of the Invention:
Microorganisms from the genus Salmonella are responsible for the majority of cases of bacterial diarrhea occurring in humans. Typically, screening and identification of a Salmonella infection is accomplished by microbial culturing techniques followed by biochemical testing. This takes from one to three days, sometimes ending in equivocal results. Identification of Salmonella spp. by use of an assay using DNA probes would be less labor intensive for the clinician, provide unequivocal results, and would enable quicker diagnosis of salmonellosis.
Nucleic acid hybridization technology is a new approach in the diagnostic industry. This methodology e~ploits the property that sequences unique to an organism comprise its genome. In a hybridization test, a po~itiYe signal is generated when these unique genomic sequences in the bacterial or the viral target hybridize with nucleic acid probes, which are tagged with a detection label.
U.S. Patent No. 4,689,295 to Taber, et al. describes Salmonella DNA probes which are Salmonella DNA fragments - 35 common to more than 80% of the known Salmonella species.
~RD-77 q~8 The fragments do not code for any protein or any other material known to contribute to pathogenicity. Thus, the probes are constructed ~rom a library of fragments without regard to ~enetic function, and are principally ùsed to detect the presence of SalmQ~Lella in a food sample.
U.S. Patent Mo. 4,358,535 to Falkow, et al. describes a method for detecting microorganisms using a DNA probe by affixing the genetic material from a sample containing the microorganism to an inert support and treating the sample to render the genetic material in a single-stranded form.
The fixed material is then contacted with a labeled nucleotide sequence that is substantially complementary to a nucleotide sequence of a structural gene encoding for toxins produced by the microorganisms. E. coli is the only organism exemplified in the patent, although Salmonell~ is mentioned in a laundry list of toxin-producing microorganisms.
2() U.S. Patent ~os. 4,486,539 and 4,563,419 to Ranki, et al. describe a one-step sandwich hybridization technique employing reagents having distinct single-stranded nucleic acid fragments isolated from the genome of a microbe to be identified. These fragments have no extensive seguence homology but are situated closely together in the qenome.
There is no mention of specific genes encoding or a proteinaceous virulence factor that may be involved in human pathogenicity from infection with a microbe from the genus Salmonell~.
Nichols and Yanofsky, Proc. Natl. Acad. Sci., Vol. 76, No. 10, pp. 5244-5248 (Oct. 1979) describe th~ nucleotide sequences of ~ of SalmQnella ty~himu ium and Es~herichia coli and make an evolutionary comparison of the two. There is no mention of using these sequences as ~RD-77 7~)~
DN~ probes.
Stoleru, et al., Chem. Abstracts, 85:90053b (1976) describe polynucleotide divergence among strains of ~i Salmonella sub-genus IV and other closely related organisms. Here again, there is no mention of using sequences for DNA probes.
Detailed Descrip~ion Qf the Invention lCI
The nucleic acid probes of the invention are believed to be unique to nucleic acid from microorganisms of the genus Salmonella causing human pathogenicity, especially those helonging to Subgroups l, 2, 3a, and 3b, 4, and 6 of that genus, as that classification is reported by the Center for Disease Control in Atlanta, ~eorgia (see Clinical MicrobioloRy Newsletter, Vol. 6, No. 9, pp.
63-66, for a discussion of Salmonella Classification).
Importantly, the probPs are unique to nucleic acid from those microorganisms belonging to Subgroups l, 3a, and 3b, which encompass almost all the Salmonella human pathogens. The~ are thus capable o f hybridizing by way of complementary base pair binding to a nucleic acid sequence from Salmonella that contains at least some complementarity, termed a "target sequence". The sequences can be either RNA or DNA. It should be understood that this binding of the probe of the invention to the target sequence does not have to be p~rfectly matched. Thexe may, in fact, be unpaired regions resulting in interior loops, bulge loops, hairpin loops, cruciform binding or any other mismatched regions. The key point is that hybridization must occur to the e~tent necessary to allow detectisn of the target sequence.
The nucleic acid probes of the invention are also believed to correspond to certain nucleic acid sequences that encode proteins, which proteins may be referred to as virulence factors, involved in the pathogenesis of human disease caused by Salmonella microorganisms, especially the fimbrial-type proteins, otherwise known as the pili.
Of these proteins that may be involved in one way or another with the pathogenesis of ~almonqlla infection may be mentioned Type 1 fimbriae proteins, Type II fimbriae proteins, Type III fimbriae proteins, and the like, with the Type 1 fimbriae proteins being the most notable.
Fimbriae are straight and rigid appendages extending from a bacterial cell. In the case of enteric microorganisms, they have been implicated in the life cycle of the organism (Clegg, S. and G.F. Gerbach, J.
8acteriol. 169:934-938 (1987). Although for most microorganisms the role of fimbriae has not yet been clearly elucidated, for E. coli, fimbriae aid in bacterial E, coli colonization of the human or animal host, a phenomenon necessary for infection. Clegg and co-workers (supra at 934) report that only bacteria identified as E.
ÇQ~ or belonging to the genus Shiqella demonstrate genetic sequences involved in fimbrial e~pression.
However, other workers have suggested that Type 1 fimbriae may be involved in the adherence and pathogenosis of Salmonella entçritidi~ (Jaber Anslanzedah and Leo J.
Paulissan, Jewish Hospital of St. Louis, Missouri, Abstracts of the Annual Meeting of the American Society for Microbiology, Abs. #Bll9, 87th Annual Meeting, Atlanta, Ga., March 1987).
The length of the nucleic acid sequences in the probes of the invention is a length which is sufficient to allow hybridization to occur to at least a portion of the DNA
from Salmonella, whether chromosomal or plasmid borne, but ~RD-77 )8 preferably chromosomal DNA, to allow detection of said DNA. Surprisingly, however, relatively shorter lengths have demonstrated a specific, high afinity binding, enabling easy detection of target nucleic acid.
Accordingly, preferred for use herein, are probes having a nucleic acid sequence of about 20 to about 400 nucleotide bases long. It is more preferred that said sequences be about 20 to 200 bases long, most preferably about 20 to about 100 bases long.
In the preferred embodiments, the probe comprises a nucleic acid sequence having at least about 20 nucleotide bases comprising in whole or in part the following sequence:
5'-ATGAGACATAAATTAATGACCTCTACTATTGCGAGTCTGATGTTTGTCGCTGCCGCA
GCGGTTGCGGCTGATCCTACTCCGGTGAGCGTGGTGGGCGGGACTATTCATTTCGAAGGT
AAACTGGTTAATGCAGCCTGTGCCGTCAGCACTAAATCCGCCGATCAAACGGTGACGCTG
GGTCAATACCGTACCGCCAGCTTTACGGCGATTGGTAATACGACTGCGCAGGTGCCTTTC
~O TCCATCGTCCTGAATGACTGCGATCCGAhAGTGGCGGCCACCGCTGCCGTGGCTTTCTCT
GGTCAGGCAGATAACACCACCCCTAATTTGCTGGCTGTGTCCTCTCCGGACAATAGCACT
ACCGCAACCGGCGTCGGGATTGAGATTCTTGATAATACCTCTTCACCGTTGAAGCCGGAC
GGCGCGACCTTCTCGGCGAAGCAGTCCCTGGTTGAAGGCACCAATACGCTGCGTTTTACC
GCACGCTATAAGGCAACCGCCGCCGCCACGACGCCAGGCCAGGCTAATGCCGACGCCACC
TTTATCATGAAATACGAATAA-3' In more preferred embodiments, the nucleotide probe comprises all or a portion of at least one of the following sequenc~s, or all or a portion of a sequence complementary thereto, said sequences selected from the group consisting essentially of:
5'...CAGGCCAGGCTAATGCCGACGCCACCTTTATCATGAAATACGAATAAT...3', 5'...CCTACTCCGGTGAGCGTGAGTGGCGGTACTATTCATTTCGAAGGTAAACT..3', )RD-77 5~ GCG TGC GGT AAA ACG CAG CGT ATT GGT GCC TTC AAC -3', 5~ TAG TGC TAT TGT CCG CAG AGG AGA CAG CCA -3', 5' GCC GGT TGC GGT AGT GCT ATT GTC CGC AGA -3', 5' ACC CAG CGT CAC CGT TTG ATC GGC GGA TTT -3', 5' GTA TTG GTG CCT TCA ACC AGC GAC TGC TTC -3', :10 5'- ATT GCG AGT CTG ATG TTT G -3', 5'- TGC AGC CTG TGC CGT CAG C -3', 5'- TCT GCG GAC AAT AGC ACT A -3~, 5~- GTT GAA GGC ACC AAT AC -3', 5'- TGC CGT TCC CTG ACG GGA -3', 5'- GCG TGC GGT ~AA ACG CAG -3', 5'- CCC GAC GCC GGT TGC GG -3', 5'- GGC CGC CAC TTT CGG AT -3', 5'- GTT TGA TCG GC5 GAT TT -3', a~d 5 '- GCT CAC CGG AGT AGG ATC -3'.
In the most preferred embodiments, the nucleic acid probes comprise all or a portion of at least one of the following sequences, or all or a portion of sequences complementary thereto:
-7- ~J~
5' GCCG~TTGCGGTAGTGCTATTGTCCGCAGA 3~, and 5' GTATTGGTGCCTTCAACCAGCGACTGCTTC 3'.
It should be appreciated that any part of the sequences detailed above, having a length of at least about 20 nucleotide bases, and being capable of hybridizing to the nucleic acid of Salmonella, especially chromosomal DNA, is within the contemplation of the present invention. For example, a sequence of nucleic acid which begins in the middle of one of above-described sequences and extends further than the end of that sequence, and which detects Salmonella without appreciable cross-hybridization with other species, is suitable for use in the invention. Overlapping sequences, combinations of smaller subsequences found within the sequences described above, and the like, are also included.
Additional sequences that do not interfere with the hybridization abilities of the probe are also included, such as primer sequences, cloning site sequences, and any other type of flan~ing sequence.
As alluded to, DNA sequences complementary to those specifically depicted above are also suitable for use in the invention. In vivo, DNA e~ists as a double helix with complementary strands. DNA hybridization methods which utilize the probes of the invention hreak apart the double strands to provide single-stranded chromosomal DN~ ~hich is then available to bind with the probe. The probes of the invention bind to one strand of the denatured double-stranded target DNA, whereas the complementary sequence of the probe would bind to the other strand.
Subsets, derivatives, subclones and mutation~ of the nucleotide sequences as detailed above, which do not detract from the ability of the nucleotide sequences to - ~ -detect ~almonella, are also suitable for use in the invention. As used herein, the terms "subsetsN means nucleotide sequences having fewer than the entire number of nucleotides in a discrete nucleotide sequence. As used herein, the term ~derivatives" means discrete nucleotide sequences of the invention having additional oligonucleotides not derived from Salmonella. These may be purposely attached, such as polynucleotide sequence that may be termed a tail, or other sequences interspersed throughout the sequences taught herein which are not completely complementary to specific portions of the nucleic acid from Salmonell~, but do not interfere with the overall ability of the probe to hybridize to the nucleic acid of $almonella.
1~
As used herein, the term ~subclones" means fragments of the original nucleic acid sequences as taught herein, which have been inserted into a vector. It is well known in the art that subsets, derivatives, subclones and mutations of nucleotide sequences may function in the same way as the original nucleotide sequence.
The nucleic acid probes of the invention are labeled to signal hybridization to target nucleic acid from a microorganism belonging to the genus Salmonella. The labeling may take on many forms, including conventional radioisotopic labeling, chemical labeli~g, immunogenic labeling, or a label with light scattering effect, and the like. Suitable methods to detect such labels are scintillation counting, autoradiography, fluorescence measurement, colorimetric measurement, or light emission measurement.
Thus, the labeling may comprise a radiolabel (e.g.
~5 14c, 32p, 3H, and the like), an enzyme (e.g., horseradish peroxidase, alkaline or acid phosphatase, and the like), a bacterial label, a fluorescent label, an antibody (which may be used in a double antibody system), an antigen (to be used with a labeled antibody), a small molecule such as biotin (to be used with an avidin, streptavidin, or antibiotin system), a late~ particle (to be used in a buoyancy or latex agglutination system), an electron dense compound such as ferritin) to be used with electron microscopy), or a light scattering particle such as colloidal gold, or any combinations or permutations of the foregoing.
For e~ample, if the labeling portion of the probe is an antigen, a signal can be generated by complexing said antigen with an antibody/enzyme conjugate, followed by an addition of an enæyme substrate. If this portion were an antibody, signal can be generated by complexing anti-antibody or an FC binding protein such as Protein A
therewith, when such second antibody or Protein A have been conjugated to an enzyme.
For reasons of ease and safety in the handling of the probe, it is preferred that it be chemically labeled, especially enzymatically or immunologically. In more Z5 preferred embodiments, the chemical label of choice is a hapten such as biotin, iminobiotin, fluorescein, and the like.
Among the preferred labeling systems that may be mentioned are those based on the biotin/streptavidin system. Thi~ system can be incorporated into the probe by a variety of means. For e~ample, the probe can be covalently attach~d to biotin via a cytochrome c bridge (Manninq, et al., Biochemistry, 16: 1364-1370 (1977), Manninq, et al., Chromosoma, 53: 107-117 (1975), Sodia 1 o - ~ 8 A., Nucleic Acids Research, 5: 385-401 (1978)), or the biotin can be covalently incorporated into specific nucleotide residues (~.anaer P.~., Proceedings of one National Academy of Sciences, USA, 7~: 6633-6637 (1981), or the biotin can be attached to a polynucleotide by means of a diamine (e.g., pentane diamine) bridge (Broker, T.R~.
, Nucleic Acids Research 5: 363-384 (1978)).
Interaction oE the biotin molecules is accomplished with avidin, streptavidin or antibiotin antibodies that are conjugated to such signalling components as latex particles ~Sodja,_A,. et al ~ or Manninq, et al.
Chromosoma, supra,) ferritin (Broker, supra, a fluorogen such as fluorescein, an enzyme, secondary antibodies, magnetic particles, or the like.
In some preferred embodiments, however, the chemical label is attached to a "tail seyuence~ which is affixed to the 3' terminal end of the probe~ The tail sequence of the rlucleic acid probes of the in~ention are preferably composed of nucleotide bases. In more preferred embodiments of the invention, the nucleotides are adenosine and uridine. In the most preferred embodiments of the invention the tail sequence has a composition of appro~imately 30% adenosine and 10% uridine. The nucleotide sequence of the tail is preferably approsimately 200 to 400 bases long. The tail sequence may be added to the probe by enzymatic reaction using terminal deoxynucleotidyl transferase (Pharmacia), or by any other conventional method.
The nucleic acid sequences useful in the nucleic acid probes of the invention are readily prepared by any conventional method such as organic synthesis, recombinant DNA techniques or isolation from genomic DNA, especially that DNA that carries a fim gene, which encodes for a ~RD-77 ~imbrial protein. ~owever, the se~uences as described herein are particularly amenable to organic synthesis using techniques known in the art, such as techniques utiliziny a nucleic acid synthesizer and commercially 5 available reagents.
Accordingly, then, the probes of the present invention are preferably made synthetically rather than being derived from genomic DNA or RNA. Methods of chemically synthesizing the oligonucleotide probes of the present invention are well known in the art. One such method is the phosphoramidite method described in U.S. Patent No.
4,4S8,066 (Caruthers, et al.~. Other methods are described in ~. Amarnath et al. (1977), Chem. Rev~ 77:
183-217. Since the preferred probes of the present invention are relatively short, they therefore can be efficiently made by an automated DNA synthesizer. The probes may also conveniently be tailed with additional nu~leotides, for e~ample, biotin labeled nucleotides, preferably less than about 1000 bases, more preferably about 150 to about 500 bases, most preferably about 200-400 bases. Chemical synthesis of the probes makes it possible to easily produce large numbers of purified probes with specific nucleotide sequences rather than relying on the difficult recombinant procedures of isolating and purifying the genetic information from a natural source.
The probes may be provided in a lyophilized form, to be reconstituted in a buffer appropriat~ for conducting - hybridization r~actions. Alternatively, the probes may already be present in such a buffer or reagent solution, providing a reagent for detection of human pathogenic Salmonella. Such a reagent solution comprises agents that, in general, enhance the ability of the probe to bind ~3~
to the ta~get nucleic acid. For e~ample, the reagent solution may contain any suitable hybridi~ation enhancer, detergent, carrier DNA, and a compound to increase the specificity, such as formamide. Such a reagent solution may comprise one or more nucleotide sequences as described herein, in any combination, as the probe portion of the reagent. In the preferred embodiments, the reagent solution comprises formamide, especially in the amounts of about 40% to about 60% of buffer volume, more preferably about 47~ to about 55%. In the particularly preferred embodiments, the reagent solution also contains a carrier DNA.
The use of the probes as described herein is not limited to any specific method or technique of conducting hybridization to the nucleic acid in a biological specimen, to detect the target sequence. Several hybridization assay techniques are known to the art and include, for e~ample, dot blot hybridization, Southern blotting; sandwich hybridization assays such as those described by Ranki, et al., in U.S. Patent Nos. 4,563,415 and 4,486,539; sandwich hybridization on beads as described by Hansen, et al. in European Patent Application 84306513.7; displacement hybridization techniques such as those described in WO 87/03911; capture techniques wherein the nucleic acid probes as described herein are first immobili~ed onto a solid support and then contacted with sample; n situ hybridization such as those cited or described by Ploeg, Folia Histochemica et Cytobiologica, Vol. 24 (1986) No. 3~ pp 189-199; and the like.
The target analyte polynllcleotide of a microorganism belonging to the genus Salmonella, may be present in various media, most often in a biological, physiological, or environmental specimen. It is preferred in some cases ~RD-77 -13- ~3~ 8 to subject the specimen containing the target polynucleotide to a variety of e~traction, purification, and isolation protocols before conducting analysis according to the methods of this invention. Measures such as these are desirable to rid the sample of substances that might interfere with binding of the analyte to the hybridization probe. Examples of such protocols may be found in the second chapter of NucleiG Acid Hybridization, ed. B. Hames & S. Hiqgins, IRL Press, Washington, D.C.
(1985), and in standard textbooks.
It is also within the contemplation of the present invention that synthetic homo- or hetero- poly-nucleotides can be prepared in the laboratory to serve as the target analyte despite their abiological origins, as such synthetic polynucleotides might be desirable for research in the area of the pathogenesis of Salmonçlla infection, and the like.
Additionally, sample containing target analyte nucleotide sequences must often be treated to convert any target analyte to sin~le-stranded form. This conversion to single-stranded form may be accomplished by a variety of ways conventional to ths art. For example, the denaturation of duplex nucleic acids can be accomplished thermally, chemically or in other conventional ways. The denaturation process will depend upon the pH, ionic strength, temperature, and other properties of the ambient medium (e.g., presence of urea, formamide, glyo~al, methyl mercury hydro~ide or other agents), as well as upon the base composition (i.e., the GC/AT ratio), sequence, and length o the duple~ nucleic acid. Reviews of various methods of denaturation may be found in standard te~tbooks, and in J. Marmur, C. Schildkraut and P. Doty in Molecular Basis of Neoplasia, Univ. of Te~as Press~
oRD-77 -14- ~ ~3~
Austin, Te~as, 1962; and T. Maniatis, E.F. Fritsch, and J.
Sarnbrook, in Molecular Cl~nina, Cold Spring Harbor Laboratory, 1982.
Exemplary of a hybridization reaction are situations wherein the target analyte nucleotide is provided in a liquid medium. This medium may take many forms, most illustrative of which is unprocessed biological fluid, or solid biological samples dispersed in water or other compati~le liquid medium. The unprocessed biological fluid c~n be mixed with a ~second solution~ in some embodiments so as to produce a medium known to support rehybridization of complementary single-stranded nucleic acids.
The second solution may be aqueous or nonaqueous or a mixture of both. Certain inorganic or organic additives known to affect rehybridization of complementary single-stranded nucleic acids may be added to enhance the rate of hybridization and~or to increase the equilibrium e~tent of rehybridization (i.e., stability of the rehybridized form). Of the inorganic additives may be mentioned sodium citrate and sodium chloride; of the organic compounds may be mentioned such compounds as formamide. Other useful additives are polyethyl~ne glycol, de~tran sulfate, sodium dodecyl sulfate and casein.
The probe may be contact~d with a liquid sample under conditions in which the analyte target nucleotide sequence, if present, can hybridize in whole or in part to a complementary region contained in the target recognition moiety of the probe nucleotide. This contacting stPp may be effectuated in a variety vf ways, and under varying conditions of rstringency". A review of factors which ~3~
affect rehybridization ~reassociation) processes is available in NuSleic Acid Hybridization, ed. B. Hames and S. Higgins, IRL Press, Washington, D.C. (1985). The factors include conditions of temperature, pH, salt concentration and solvent medium, in addition to factors which reflect the length, complexity, and degree of complementarity of the probe and analyte target polynucleotides. The contact period may vary depending on the length of time necessary to effect hybridization to the desired e~tent, which is dependent in part on the length of the binding region in the target recognition moiety as well as the reaction conditions.
The nucleotide probe, with any bound complementary target analyte, is separated from the biological sample after the desired hybridization has taken place. This separation may be accomplished by any suitable procedure including, but not limited to chromatography (column, gel, etc.~, filtration, electrophoresis ~including electroelution) and the like. It may be further desirable to incorporate a rinsing step to ensure that unbound material is fully separated from rehybridized material which has bound to the probe.
Once the hybridization event has taken place and the bound material is separated from unbound, detection of the label on the probe is undertaken by assaying the bound material, unbound matsrial, or both. If the label is a radioactive one, direct detection an be accomplished through conventional radioisotopic quantitation techniques. If the label is a chemical one, as for example, biotin, indirect detection takes place.
The following are more specif;c examples of certain embodiments of the presPnt invention, but are not to be ~RD-77 -16~ 3~ 3~
considered limitative thereof.
EXAMPLES
E~ample 1 - Testin~ a Double-Stran~e~ ~fim" Probe A double stranded DNA probe was derived from the chimeric plasmid pISC137 (Purcell, B., et al., Journal of Bacteriology, Volume 169, pp. 5831-5834 (1987)) A 1.6 Rb iO EcoRI-HpaI fragment carrying the ~m gene from S.
typhimurium was 32P-labeled and us~d in hybridization experiments to test specificity and sensitivity of the fim probe. Both ATCC strains and clinical isolates were examined for reactivity with the probe in dot blot experiments (Table 1). It appeare~ that the fim gene could act as a novel probe for Salmonella.
20Hybridization Pattern of fim Probe Tarqet Oraanism Hybridization Sianal S. choleraesuis ATCC#13312 S. enteriditis ATCC~13076 S. typhi ATCC#6539 +
S. typhimuruim ATCC#14028 +
S. typhimuruim ATCC#19585 t S. typhimuruim Clinical isolate 30 Shigella boydiae ATCC#9207 S. dysenteriae ATCC#29026 S. sonnei ATCC#lln60 ~. fle~neri ATCC#12022 E. coli ATCC#9339 E. coli ATcc#25922 ~D-77 ~ 3~
T~E~et Orqani~m HybridizatiQn Siqnal E. coli ATCC#9546 Campylobacter jejuni ATCC~29^128 5 C. jejuni ATCC#33560 C. fecalis ATCC#33709 C. coli ATCC#33559 Pseudomonas aeruginosa ATCC#27853 Klebsiella pneumoniae ATCC#135~3 Bacillus A positive hy~ridization signal was seen after autoradiography if the 32P-labeled probe reacted with target DNA.
1~
Example 2 - Use of SYnthetic Oliqonucleotides as Probes Starting with the DNA sequence of the entire fim gene, 5' to 3':
5'-ATGAGACATAAATTAATGACCTCTACTATTGCGAGTCTGATGTTTGTCGCTGCCGCA
GCGGTTGCGGCTG~TCCTACTGCGGT&AGCGTG~TGGGCGGGACTATTCATTTCGAAGGT
AAACTGGTTAATGCAGCCTGTGCCGTCAGCACTAAATCCGCCGATCAAACGGTGACGCTG
GGTCAATACCGTACCGCCAGCTTTACGGCGATTGGTAATACGACTGCGCAGGTGCCTTTC
TCCATCGTCCTGAATGACTGCGATCCGAAAGTGGCGGCCACCGCTGCCGTGGGTTTCTCT
GGTCAGGCAGATAACACCACCCCTAATTTGCTGGCTGTGTCCTCTGCGGACAATAGCACT
ACCGCAACCGGCGTCGGGATTGAGATTCTTGATAATACCTCTTCACCGTTGAAGCCGGAC
GGCGCGACCTTCTCGGCCAAGCAGTCGCTGGTTGAAGGCACCAATACGCTGCGTTTTACC
GCACGCTATAAGGCAACCGCC~CCGCCACGACGCCAGGCCAGGGTAATGCCGACGCCACC
TTTATCATGAAATACGAATAA-3' two oligomers were chemically synthesized. They were chosen on the basis of (a) location outside o~ the invertible repeats that are 5' proximal and, (b~ a G plus C content of approximately 50% (~hich relates to lysine )RD-77 content, ~almonella spp. having a high content o this amino acid versus Klebsiella, E. coli, etc.~. Otherwise, sequences to be synthesized were arbitrarily selected and were approximately 50 bases long.
The discrete nucleotide sequsnces below were synthesized for testing:
5'...CAGGCCAGGCTAAT~CCGACGCCACCTTTATCATGAAATACGAATAAT...3' 10 (this sequence was designated ODS0098).
5'...CCTACTCCGGTGAGCGTGAGTGGC~GTACTATTCATTTCGAAGGTAAACT..3' (this sequence was designated ODS0100) The synthetic oligomers were tested in colony hybridization experiments. Both probes were 32P-labelled and tested in combination, against a panel of 142 Salmonella strains obtained from the Center for Disease Control and representing all species' subgroups (1,2,3a,3b,4,5 and 6). Other organisms tested for reactivity with the probe are indicated in Table II.
TABLE II
Target Organism* Number tested ~b~ ti~n ~.~5~ 1 Su~roup l S. adelaide 30 S. agona 3 +
S. alachua 1 +
S. albany S. anatum 3 +
S. bareilly 2 35 S~ bere ~RD-77 ( ( --lg--Target Orqan sm* Number tes~~d Hybridization Signal S. berta 1 +
S. hlockley 1 +
5 S. bovis morbificans S. braenderup S. brandenburg 1 +
S. bredeney 1 +
S. cerro 1 +
10 S. chester 1 +
S. choleraesuis 4 +
S. decatur S. derby S. drypool 1 +
15 S. dublin 3 +
S. enteritidis 5 +
S. give 1 +
S. haardt 1 +
S. hadar 3 +
20 S. hartford 1 +
S. havana S. heidelberg 3 S. indiana 1 +
S. infantis 3 +
25 S. invern~ss 1 +
S. java S. javiana S. johannesburg 1 +
S. kentucky 30 S. kottbus S. krefeld 1 +
S. livingstone 1 +
S. london S. madelia 1 +
35 S. manhattan 1 +
~RD-77 -20~ &
Target Orqanism~ Numb~r te~d HYbridization Siqnal S. mbandaka 1 +
S. meleagridis 1 +
5 S. miami S. minnesota 1 +
S. mississippi 1 +
S. montevideo 2 +
S. muenchen 3 +
10 S. muenster 1 +
S. new brunswick 1 +
S. newington 1 +
S. newport 3 +
S. norwich :15 S. ohio 1 +
S. oranienburg 1 +
S. panama 1 +
S. paratyphi A 2 +
S. paratyphi B 1 +
20 S. paratyphi C 2 S. poona 1 f S. reading 1 +
5. rubislau S. san diego 2 25 S. saphra 1 +
S. senftenburg 4 +
S. st. paul 1 +
S. stanley S. sundsvall 1 +
30 S. tennessee 1 +
S. typhimurium 9 S. typhi 2 +
S. virchow S. welterredon 1 +
35 S. worthington 1 +
~u~qrouP 2 Salmonella:
58:dz 6 1 +
There is no mention of specific genes encoding or a proteinaceous virulence factor that may be involved in human pathogenicity from infection with a microbe from the genus Salmonell~.
Nichols and Yanofsky, Proc. Natl. Acad. Sci., Vol. 76, No. 10, pp. 5244-5248 (Oct. 1979) describe th~ nucleotide sequences of ~ of SalmQnella ty~himu ium and Es~herichia coli and make an evolutionary comparison of the two. There is no mention of using these sequences as ~RD-77 7~)~
DN~ probes.
Stoleru, et al., Chem. Abstracts, 85:90053b (1976) describe polynucleotide divergence among strains of ~i Salmonella sub-genus IV and other closely related organisms. Here again, there is no mention of using sequences for DNA probes.
Detailed Descrip~ion Qf the Invention lCI
The nucleic acid probes of the invention are believed to be unique to nucleic acid from microorganisms of the genus Salmonella causing human pathogenicity, especially those helonging to Subgroups l, 2, 3a, and 3b, 4, and 6 of that genus, as that classification is reported by the Center for Disease Control in Atlanta, ~eorgia (see Clinical MicrobioloRy Newsletter, Vol. 6, No. 9, pp.
63-66, for a discussion of Salmonella Classification).
Importantly, the probPs are unique to nucleic acid from those microorganisms belonging to Subgroups l, 3a, and 3b, which encompass almost all the Salmonella human pathogens. The~ are thus capable o f hybridizing by way of complementary base pair binding to a nucleic acid sequence from Salmonella that contains at least some complementarity, termed a "target sequence". The sequences can be either RNA or DNA. It should be understood that this binding of the probe of the invention to the target sequence does not have to be p~rfectly matched. Thexe may, in fact, be unpaired regions resulting in interior loops, bulge loops, hairpin loops, cruciform binding or any other mismatched regions. The key point is that hybridization must occur to the e~tent necessary to allow detectisn of the target sequence.
The nucleic acid probes of the invention are also believed to correspond to certain nucleic acid sequences that encode proteins, which proteins may be referred to as virulence factors, involved in the pathogenesis of human disease caused by Salmonella microorganisms, especially the fimbrial-type proteins, otherwise known as the pili.
Of these proteins that may be involved in one way or another with the pathogenesis of ~almonqlla infection may be mentioned Type 1 fimbriae proteins, Type II fimbriae proteins, Type III fimbriae proteins, and the like, with the Type 1 fimbriae proteins being the most notable.
Fimbriae are straight and rigid appendages extending from a bacterial cell. In the case of enteric microorganisms, they have been implicated in the life cycle of the organism (Clegg, S. and G.F. Gerbach, J.
8acteriol. 169:934-938 (1987). Although for most microorganisms the role of fimbriae has not yet been clearly elucidated, for E. coli, fimbriae aid in bacterial E, coli colonization of the human or animal host, a phenomenon necessary for infection. Clegg and co-workers (supra at 934) report that only bacteria identified as E.
ÇQ~ or belonging to the genus Shiqella demonstrate genetic sequences involved in fimbrial e~pression.
However, other workers have suggested that Type 1 fimbriae may be involved in the adherence and pathogenosis of Salmonella entçritidi~ (Jaber Anslanzedah and Leo J.
Paulissan, Jewish Hospital of St. Louis, Missouri, Abstracts of the Annual Meeting of the American Society for Microbiology, Abs. #Bll9, 87th Annual Meeting, Atlanta, Ga., March 1987).
The length of the nucleic acid sequences in the probes of the invention is a length which is sufficient to allow hybridization to occur to at least a portion of the DNA
from Salmonella, whether chromosomal or plasmid borne, but ~RD-77 )8 preferably chromosomal DNA, to allow detection of said DNA. Surprisingly, however, relatively shorter lengths have demonstrated a specific, high afinity binding, enabling easy detection of target nucleic acid.
Accordingly, preferred for use herein, are probes having a nucleic acid sequence of about 20 to about 400 nucleotide bases long. It is more preferred that said sequences be about 20 to 200 bases long, most preferably about 20 to about 100 bases long.
In the preferred embodiments, the probe comprises a nucleic acid sequence having at least about 20 nucleotide bases comprising in whole or in part the following sequence:
5'-ATGAGACATAAATTAATGACCTCTACTATTGCGAGTCTGATGTTTGTCGCTGCCGCA
GCGGTTGCGGCTGATCCTACTCCGGTGAGCGTGGTGGGCGGGACTATTCATTTCGAAGGT
AAACTGGTTAATGCAGCCTGTGCCGTCAGCACTAAATCCGCCGATCAAACGGTGACGCTG
GGTCAATACCGTACCGCCAGCTTTACGGCGATTGGTAATACGACTGCGCAGGTGCCTTTC
~O TCCATCGTCCTGAATGACTGCGATCCGAhAGTGGCGGCCACCGCTGCCGTGGCTTTCTCT
GGTCAGGCAGATAACACCACCCCTAATTTGCTGGCTGTGTCCTCTCCGGACAATAGCACT
ACCGCAACCGGCGTCGGGATTGAGATTCTTGATAATACCTCTTCACCGTTGAAGCCGGAC
GGCGCGACCTTCTCGGCGAAGCAGTCCCTGGTTGAAGGCACCAATACGCTGCGTTTTACC
GCACGCTATAAGGCAACCGCCGCCGCCACGACGCCAGGCCAGGCTAATGCCGACGCCACC
TTTATCATGAAATACGAATAA-3' In more preferred embodiments, the nucleotide probe comprises all or a portion of at least one of the following sequenc~s, or all or a portion of a sequence complementary thereto, said sequences selected from the group consisting essentially of:
5'...CAGGCCAGGCTAATGCCGACGCCACCTTTATCATGAAATACGAATAAT...3', 5'...CCTACTCCGGTGAGCGTGAGTGGCGGTACTATTCATTTCGAAGGTAAACT..3', )RD-77 5~ GCG TGC GGT AAA ACG CAG CGT ATT GGT GCC TTC AAC -3', 5~ TAG TGC TAT TGT CCG CAG AGG AGA CAG CCA -3', 5' GCC GGT TGC GGT AGT GCT ATT GTC CGC AGA -3', 5' ACC CAG CGT CAC CGT TTG ATC GGC GGA TTT -3', 5' GTA TTG GTG CCT TCA ACC AGC GAC TGC TTC -3', :10 5'- ATT GCG AGT CTG ATG TTT G -3', 5'- TGC AGC CTG TGC CGT CAG C -3', 5'- TCT GCG GAC AAT AGC ACT A -3~, 5~- GTT GAA GGC ACC AAT AC -3', 5'- TGC CGT TCC CTG ACG GGA -3', 5'- GCG TGC GGT ~AA ACG CAG -3', 5'- CCC GAC GCC GGT TGC GG -3', 5'- GGC CGC CAC TTT CGG AT -3', 5'- GTT TGA TCG GC5 GAT TT -3', a~d 5 '- GCT CAC CGG AGT AGG ATC -3'.
In the most preferred embodiments, the nucleic acid probes comprise all or a portion of at least one of the following sequences, or all or a portion of sequences complementary thereto:
-7- ~J~
5' GCCG~TTGCGGTAGTGCTATTGTCCGCAGA 3~, and 5' GTATTGGTGCCTTCAACCAGCGACTGCTTC 3'.
It should be appreciated that any part of the sequences detailed above, having a length of at least about 20 nucleotide bases, and being capable of hybridizing to the nucleic acid of Salmonella, especially chromosomal DNA, is within the contemplation of the present invention. For example, a sequence of nucleic acid which begins in the middle of one of above-described sequences and extends further than the end of that sequence, and which detects Salmonella without appreciable cross-hybridization with other species, is suitable for use in the invention. Overlapping sequences, combinations of smaller subsequences found within the sequences described above, and the like, are also included.
Additional sequences that do not interfere with the hybridization abilities of the probe are also included, such as primer sequences, cloning site sequences, and any other type of flan~ing sequence.
As alluded to, DNA sequences complementary to those specifically depicted above are also suitable for use in the invention. In vivo, DNA e~ists as a double helix with complementary strands. DNA hybridization methods which utilize the probes of the invention hreak apart the double strands to provide single-stranded chromosomal DN~ ~hich is then available to bind with the probe. The probes of the invention bind to one strand of the denatured double-stranded target DNA, whereas the complementary sequence of the probe would bind to the other strand.
Subsets, derivatives, subclones and mutation~ of the nucleotide sequences as detailed above, which do not detract from the ability of the nucleotide sequences to - ~ -detect ~almonella, are also suitable for use in the invention. As used herein, the terms "subsetsN means nucleotide sequences having fewer than the entire number of nucleotides in a discrete nucleotide sequence. As used herein, the term ~derivatives" means discrete nucleotide sequences of the invention having additional oligonucleotides not derived from Salmonella. These may be purposely attached, such as polynucleotide sequence that may be termed a tail, or other sequences interspersed throughout the sequences taught herein which are not completely complementary to specific portions of the nucleic acid from Salmonell~, but do not interfere with the overall ability of the probe to hybridize to the nucleic acid of $almonella.
1~
As used herein, the term ~subclones" means fragments of the original nucleic acid sequences as taught herein, which have been inserted into a vector. It is well known in the art that subsets, derivatives, subclones and mutations of nucleotide sequences may function in the same way as the original nucleotide sequence.
The nucleic acid probes of the invention are labeled to signal hybridization to target nucleic acid from a microorganism belonging to the genus Salmonella. The labeling may take on many forms, including conventional radioisotopic labeling, chemical labeli~g, immunogenic labeling, or a label with light scattering effect, and the like. Suitable methods to detect such labels are scintillation counting, autoradiography, fluorescence measurement, colorimetric measurement, or light emission measurement.
Thus, the labeling may comprise a radiolabel (e.g.
~5 14c, 32p, 3H, and the like), an enzyme (e.g., horseradish peroxidase, alkaline or acid phosphatase, and the like), a bacterial label, a fluorescent label, an antibody (which may be used in a double antibody system), an antigen (to be used with a labeled antibody), a small molecule such as biotin (to be used with an avidin, streptavidin, or antibiotin system), a late~ particle (to be used in a buoyancy or latex agglutination system), an electron dense compound such as ferritin) to be used with electron microscopy), or a light scattering particle such as colloidal gold, or any combinations or permutations of the foregoing.
For e~ample, if the labeling portion of the probe is an antigen, a signal can be generated by complexing said antigen with an antibody/enzyme conjugate, followed by an addition of an enæyme substrate. If this portion were an antibody, signal can be generated by complexing anti-antibody or an FC binding protein such as Protein A
therewith, when such second antibody or Protein A have been conjugated to an enzyme.
For reasons of ease and safety in the handling of the probe, it is preferred that it be chemically labeled, especially enzymatically or immunologically. In more Z5 preferred embodiments, the chemical label of choice is a hapten such as biotin, iminobiotin, fluorescein, and the like.
Among the preferred labeling systems that may be mentioned are those based on the biotin/streptavidin system. Thi~ system can be incorporated into the probe by a variety of means. For e~ample, the probe can be covalently attach~d to biotin via a cytochrome c bridge (Manninq, et al., Biochemistry, 16: 1364-1370 (1977), Manninq, et al., Chromosoma, 53: 107-117 (1975), Sodia 1 o - ~ 8 A., Nucleic Acids Research, 5: 385-401 (1978)), or the biotin can be covalently incorporated into specific nucleotide residues (~.anaer P.~., Proceedings of one National Academy of Sciences, USA, 7~: 6633-6637 (1981), or the biotin can be attached to a polynucleotide by means of a diamine (e.g., pentane diamine) bridge (Broker, T.R~.
, Nucleic Acids Research 5: 363-384 (1978)).
Interaction oE the biotin molecules is accomplished with avidin, streptavidin or antibiotin antibodies that are conjugated to such signalling components as latex particles ~Sodja,_A,. et al ~ or Manninq, et al.
Chromosoma, supra,) ferritin (Broker, supra, a fluorogen such as fluorescein, an enzyme, secondary antibodies, magnetic particles, or the like.
In some preferred embodiments, however, the chemical label is attached to a "tail seyuence~ which is affixed to the 3' terminal end of the probe~ The tail sequence of the rlucleic acid probes of the in~ention are preferably composed of nucleotide bases. In more preferred embodiments of the invention, the nucleotides are adenosine and uridine. In the most preferred embodiments of the invention the tail sequence has a composition of appro~imately 30% adenosine and 10% uridine. The nucleotide sequence of the tail is preferably approsimately 200 to 400 bases long. The tail sequence may be added to the probe by enzymatic reaction using terminal deoxynucleotidyl transferase (Pharmacia), or by any other conventional method.
The nucleic acid sequences useful in the nucleic acid probes of the invention are readily prepared by any conventional method such as organic synthesis, recombinant DNA techniques or isolation from genomic DNA, especially that DNA that carries a fim gene, which encodes for a ~RD-77 ~imbrial protein. ~owever, the se~uences as described herein are particularly amenable to organic synthesis using techniques known in the art, such as techniques utiliziny a nucleic acid synthesizer and commercially 5 available reagents.
Accordingly, then, the probes of the present invention are preferably made synthetically rather than being derived from genomic DNA or RNA. Methods of chemically synthesizing the oligonucleotide probes of the present invention are well known in the art. One such method is the phosphoramidite method described in U.S. Patent No.
4,4S8,066 (Caruthers, et al.~. Other methods are described in ~. Amarnath et al. (1977), Chem. Rev~ 77:
183-217. Since the preferred probes of the present invention are relatively short, they therefore can be efficiently made by an automated DNA synthesizer. The probes may also conveniently be tailed with additional nu~leotides, for e~ample, biotin labeled nucleotides, preferably less than about 1000 bases, more preferably about 150 to about 500 bases, most preferably about 200-400 bases. Chemical synthesis of the probes makes it possible to easily produce large numbers of purified probes with specific nucleotide sequences rather than relying on the difficult recombinant procedures of isolating and purifying the genetic information from a natural source.
The probes may be provided in a lyophilized form, to be reconstituted in a buffer appropriat~ for conducting - hybridization r~actions. Alternatively, the probes may already be present in such a buffer or reagent solution, providing a reagent for detection of human pathogenic Salmonella. Such a reagent solution comprises agents that, in general, enhance the ability of the probe to bind ~3~
to the ta~get nucleic acid. For e~ample, the reagent solution may contain any suitable hybridi~ation enhancer, detergent, carrier DNA, and a compound to increase the specificity, such as formamide. Such a reagent solution may comprise one or more nucleotide sequences as described herein, in any combination, as the probe portion of the reagent. In the preferred embodiments, the reagent solution comprises formamide, especially in the amounts of about 40% to about 60% of buffer volume, more preferably about 47~ to about 55%. In the particularly preferred embodiments, the reagent solution also contains a carrier DNA.
The use of the probes as described herein is not limited to any specific method or technique of conducting hybridization to the nucleic acid in a biological specimen, to detect the target sequence. Several hybridization assay techniques are known to the art and include, for e~ample, dot blot hybridization, Southern blotting; sandwich hybridization assays such as those described by Ranki, et al., in U.S. Patent Nos. 4,563,415 and 4,486,539; sandwich hybridization on beads as described by Hansen, et al. in European Patent Application 84306513.7; displacement hybridization techniques such as those described in WO 87/03911; capture techniques wherein the nucleic acid probes as described herein are first immobili~ed onto a solid support and then contacted with sample; n situ hybridization such as those cited or described by Ploeg, Folia Histochemica et Cytobiologica, Vol. 24 (1986) No. 3~ pp 189-199; and the like.
The target analyte polynllcleotide of a microorganism belonging to the genus Salmonella, may be present in various media, most often in a biological, physiological, or environmental specimen. It is preferred in some cases ~RD-77 -13- ~3~ 8 to subject the specimen containing the target polynucleotide to a variety of e~traction, purification, and isolation protocols before conducting analysis according to the methods of this invention. Measures such as these are desirable to rid the sample of substances that might interfere with binding of the analyte to the hybridization probe. Examples of such protocols may be found in the second chapter of NucleiG Acid Hybridization, ed. B. Hames & S. Hiqgins, IRL Press, Washington, D.C.
(1985), and in standard textbooks.
It is also within the contemplation of the present invention that synthetic homo- or hetero- poly-nucleotides can be prepared in the laboratory to serve as the target analyte despite their abiological origins, as such synthetic polynucleotides might be desirable for research in the area of the pathogenesis of Salmonçlla infection, and the like.
Additionally, sample containing target analyte nucleotide sequences must often be treated to convert any target analyte to sin~le-stranded form. This conversion to single-stranded form may be accomplished by a variety of ways conventional to ths art. For example, the denaturation of duplex nucleic acids can be accomplished thermally, chemically or in other conventional ways. The denaturation process will depend upon the pH, ionic strength, temperature, and other properties of the ambient medium (e.g., presence of urea, formamide, glyo~al, methyl mercury hydro~ide or other agents), as well as upon the base composition (i.e., the GC/AT ratio), sequence, and length o the duple~ nucleic acid. Reviews of various methods of denaturation may be found in standard te~tbooks, and in J. Marmur, C. Schildkraut and P. Doty in Molecular Basis of Neoplasia, Univ. of Te~as Press~
oRD-77 -14- ~ ~3~
Austin, Te~as, 1962; and T. Maniatis, E.F. Fritsch, and J.
Sarnbrook, in Molecular Cl~nina, Cold Spring Harbor Laboratory, 1982.
Exemplary of a hybridization reaction are situations wherein the target analyte nucleotide is provided in a liquid medium. This medium may take many forms, most illustrative of which is unprocessed biological fluid, or solid biological samples dispersed in water or other compati~le liquid medium. The unprocessed biological fluid c~n be mixed with a ~second solution~ in some embodiments so as to produce a medium known to support rehybridization of complementary single-stranded nucleic acids.
The second solution may be aqueous or nonaqueous or a mixture of both. Certain inorganic or organic additives known to affect rehybridization of complementary single-stranded nucleic acids may be added to enhance the rate of hybridization and~or to increase the equilibrium e~tent of rehybridization (i.e., stability of the rehybridized form). Of the inorganic additives may be mentioned sodium citrate and sodium chloride; of the organic compounds may be mentioned such compounds as formamide. Other useful additives are polyethyl~ne glycol, de~tran sulfate, sodium dodecyl sulfate and casein.
The probe may be contact~d with a liquid sample under conditions in which the analyte target nucleotide sequence, if present, can hybridize in whole or in part to a complementary region contained in the target recognition moiety of the probe nucleotide. This contacting stPp may be effectuated in a variety vf ways, and under varying conditions of rstringency". A review of factors which ~3~
affect rehybridization ~reassociation) processes is available in NuSleic Acid Hybridization, ed. B. Hames and S. Higgins, IRL Press, Washington, D.C. (1985). The factors include conditions of temperature, pH, salt concentration and solvent medium, in addition to factors which reflect the length, complexity, and degree of complementarity of the probe and analyte target polynucleotides. The contact period may vary depending on the length of time necessary to effect hybridization to the desired e~tent, which is dependent in part on the length of the binding region in the target recognition moiety as well as the reaction conditions.
The nucleotide probe, with any bound complementary target analyte, is separated from the biological sample after the desired hybridization has taken place. This separation may be accomplished by any suitable procedure including, but not limited to chromatography (column, gel, etc.~, filtration, electrophoresis ~including electroelution) and the like. It may be further desirable to incorporate a rinsing step to ensure that unbound material is fully separated from rehybridized material which has bound to the probe.
Once the hybridization event has taken place and the bound material is separated from unbound, detection of the label on the probe is undertaken by assaying the bound material, unbound matsrial, or both. If the label is a radioactive one, direct detection an be accomplished through conventional radioisotopic quantitation techniques. If the label is a chemical one, as for example, biotin, indirect detection takes place.
The following are more specif;c examples of certain embodiments of the presPnt invention, but are not to be ~RD-77 -16~ 3~ 3~
considered limitative thereof.
EXAMPLES
E~ample 1 - Testin~ a Double-Stran~e~ ~fim" Probe A double stranded DNA probe was derived from the chimeric plasmid pISC137 (Purcell, B., et al., Journal of Bacteriology, Volume 169, pp. 5831-5834 (1987)) A 1.6 Rb iO EcoRI-HpaI fragment carrying the ~m gene from S.
typhimurium was 32P-labeled and us~d in hybridization experiments to test specificity and sensitivity of the fim probe. Both ATCC strains and clinical isolates were examined for reactivity with the probe in dot blot experiments (Table 1). It appeare~ that the fim gene could act as a novel probe for Salmonella.
20Hybridization Pattern of fim Probe Tarqet Oraanism Hybridization Sianal S. choleraesuis ATCC#13312 S. enteriditis ATCC~13076 S. typhi ATCC#6539 +
S. typhimuruim ATCC#14028 +
S. typhimuruim ATCC#19585 t S. typhimuruim Clinical isolate 30 Shigella boydiae ATCC#9207 S. dysenteriae ATCC#29026 S. sonnei ATCC#lln60 ~. fle~neri ATCC#12022 E. coli ATCC#9339 E. coli ATcc#25922 ~D-77 ~ 3~
T~E~et Orqani~m HybridizatiQn Siqnal E. coli ATCC#9546 Campylobacter jejuni ATCC~29^128 5 C. jejuni ATCC#33560 C. fecalis ATCC#33709 C. coli ATCC#33559 Pseudomonas aeruginosa ATCC#27853 Klebsiella pneumoniae ATCC#135~3 Bacillus A positive hy~ridization signal was seen after autoradiography if the 32P-labeled probe reacted with target DNA.
1~
Example 2 - Use of SYnthetic Oliqonucleotides as Probes Starting with the DNA sequence of the entire fim gene, 5' to 3':
5'-ATGAGACATAAATTAATGACCTCTACTATTGCGAGTCTGATGTTTGTCGCTGCCGCA
GCGGTTGCGGCTG~TCCTACTGCGGT&AGCGTG~TGGGCGGGACTATTCATTTCGAAGGT
AAACTGGTTAATGCAGCCTGTGCCGTCAGCACTAAATCCGCCGATCAAACGGTGACGCTG
GGTCAATACCGTACCGCCAGCTTTACGGCGATTGGTAATACGACTGCGCAGGTGCCTTTC
TCCATCGTCCTGAATGACTGCGATCCGAAAGTGGCGGCCACCGCTGCCGTGGGTTTCTCT
GGTCAGGCAGATAACACCACCCCTAATTTGCTGGCTGTGTCCTCTGCGGACAATAGCACT
ACCGCAACCGGCGTCGGGATTGAGATTCTTGATAATACCTCTTCACCGTTGAAGCCGGAC
GGCGCGACCTTCTCGGCCAAGCAGTCGCTGGTTGAAGGCACCAATACGCTGCGTTTTACC
GCACGCTATAAGGCAACCGCC~CCGCCACGACGCCAGGCCAGGGTAATGCCGACGCCACC
TTTATCATGAAATACGAATAA-3' two oligomers were chemically synthesized. They were chosen on the basis of (a) location outside o~ the invertible repeats that are 5' proximal and, (b~ a G plus C content of approximately 50% (~hich relates to lysine )RD-77 content, ~almonella spp. having a high content o this amino acid versus Klebsiella, E. coli, etc.~. Otherwise, sequences to be synthesized were arbitrarily selected and were approximately 50 bases long.
The discrete nucleotide sequsnces below were synthesized for testing:
5'...CAGGCCAGGCTAAT~CCGACGCCACCTTTATCATGAAATACGAATAAT...3' 10 (this sequence was designated ODS0098).
5'...CCTACTCCGGTGAGCGTGAGTGGC~GTACTATTCATTTCGAAGGTAAACT..3' (this sequence was designated ODS0100) The synthetic oligomers were tested in colony hybridization experiments. Both probes were 32P-labelled and tested in combination, against a panel of 142 Salmonella strains obtained from the Center for Disease Control and representing all species' subgroups (1,2,3a,3b,4,5 and 6). Other organisms tested for reactivity with the probe are indicated in Table II.
TABLE II
Target Organism* Number tested ~b~ ti~n ~.~5~ 1 Su~roup l S. adelaide 30 S. agona 3 +
S. alachua 1 +
S. albany S. anatum 3 +
S. bareilly 2 35 S~ bere ~RD-77 ( ( --lg--Target Orqan sm* Number tes~~d Hybridization Signal S. berta 1 +
S. hlockley 1 +
5 S. bovis morbificans S. braenderup S. brandenburg 1 +
S. bredeney 1 +
S. cerro 1 +
10 S. chester 1 +
S. choleraesuis 4 +
S. decatur S. derby S. drypool 1 +
15 S. dublin 3 +
S. enteritidis 5 +
S. give 1 +
S. haardt 1 +
S. hadar 3 +
20 S. hartford 1 +
S. havana S. heidelberg 3 S. indiana 1 +
S. infantis 3 +
25 S. invern~ss 1 +
S. java S. javiana S. johannesburg 1 +
S. kentucky 30 S. kottbus S. krefeld 1 +
S. livingstone 1 +
S. london S. madelia 1 +
35 S. manhattan 1 +
~RD-77 -20~ &
Target Orqanism~ Numb~r te~d HYbridization Siqnal S. mbandaka 1 +
S. meleagridis 1 +
5 S. miami S. minnesota 1 +
S. mississippi 1 +
S. montevideo 2 +
S. muenchen 3 +
10 S. muenster 1 +
S. new brunswick 1 +
S. newington 1 +
S. newport 3 +
S. norwich :15 S. ohio 1 +
S. oranienburg 1 +
S. panama 1 +
S. paratyphi A 2 +
S. paratyphi B 1 +
20 S. paratyphi C 2 S. poona 1 f S. reading 1 +
5. rubislau S. san diego 2 25 S. saphra 1 +
S. senftenburg 4 +
S. st. paul 1 +
S. stanley S. sundsvall 1 +
30 S. tennessee 1 +
S. typhimurium 9 S. typhi 2 +
S. virchow S. welterredon 1 +
35 S. worthington 1 +
~u~qrouP 2 Salmonella:
58:dz 6 1 +
3 1'Z28 Z6 1 +
S. setubal 1 +
S. phoenix 1 +
Subaroup 3a Salmonella:
62:z4, Z23 - 1 +
431 3 4 Z4'z23 - 1 +
18:Z~,Z32:-62:Z36: 1 +
481,482:z4,z24:- 1 +
Su~qroup 3b Salmonella:
65:(k):z 1 +
61:k:1,S,(7) 1 +
1,3,4 1 +
1,2,3 ~ 1 +
38:(k3:Z35 1 +
Salmonella:
431,3,4 Z29 1 +
44:z :-S. wassenaar S. fl;nt 1 +
$~bqroup 5 Salmonella:
48, 4827 482:2:- 1 _ 5 S. brookfield S. marogrosso S. malawi Sub~rou~ 6 :LO
Salmonella-ll:b:1,7 41:b:1,7 1 +
S. ferlac 1 +
:L5 S. vrindaban 1 +
Other q~nera E. coli 6 ,'0 Enteric Group 90 2 Citrobacter freundii 2 ~ and -Enterobacter hafniae The above strains were obtained from the CDC, ~tlanta, GA, complements of Dr. J.J. Farmer III and Alma C. McWhorter.
With some exceptions, the two probes ODS0098 and ODS0100 (a 48mer and a 50mer, respectively) showed esc~llent specificity and sensitivity. The probes reacted specifically with all Salmonella subgroups related to human pathogenesis (Subgroup 5 is a reptilean pathogen;
the probes do not react with organisms from this subgroup). Of khe non-Salmonellae biochemically or serologically-related organisms e~amined, only one of two Citrobacter freundii cross-reacted with the probes.
-~3-7~
To attain greater specificity, a series of shorter oligometric probes, 17-l9 bases long were examined. The discr~te nucleotide sequences below were synthesized for testing:
5'- ATT GCG AGT CTG ATG TTT G -3' (this sequence was designated ODS0111) 5'- TGC AGC CTG TGC CGT CAG C -3' (this sequence was designated ODS0112) 5'- TCT GCG GAC AAT AGC ACT A -3' (this sequence was designated ODS0113) 5'- GTT GAA GGC ACC AAT AC -3' (this sequence was designated ODS0114) 5'- TGC CGT TCC CTG ACG GGA -3' (this sequence was designated ODS0115) 5'- GCG TGC GGT AAA ACG CAG -3' (this sequence was designated ODS0116) 5'- CCC GAC GCC GGT TGC GG -3' (this sequence was designated ODS0117 5'- GGC CGC CAC TTT CGG AT -3' (this sequence was designated ODS0118) 5'- GTT TGA TCG GCG GAT TT -3' (this sequence was designated ODS0119) 5'- GCT CAC CGG AGT AGG ATC -3' ~this sequence was designated ODS0120) ~(3~
Each of these probes ~ere 32P-labelled and tested in colony hybridization experiments against 34 Salmonella strains, 5 ~itrobac~qr strains, a Ent Qob cter hafniae and an E. coli strain. Five of the 10 probes elicited non-crossreactive hybridization patterns. However, the shorter probes sacrifice sensitivity with the concomitant gain in specificity, i.e., a small number of Salrnonella~
(other than subgroup 5) were non-reactive, resultant of the use of short probes.
:LO
Probes of about 30 bases in length were also tested.
These probes were synthesized as 5' or 3' extensions of ODS0111, ODS0113, ODS0114, ODS0116 and ODS0119. The discrete nucleotide sequences below were tested:
5' ATT GCG AGT CTG ATG TTT GTC GCT GGC GCA -3' (this sequence was designated ODS0137) 5' GCG TGC GGT AAA ACG CAG CGT ATT GGT GCC TTC AAC -3' (this sequence was designated ODS0139) 5' TAG TGC TAT TGT CCG CAG AGG AGA CAG CCA -3' (this sequence was designated ODS0143) 5' GCC GGT TGC GGT AGT GCT ATT GTC CGC AGA -3' (this sequence was designated ODS0144) 5' ACC CAG CGT CAC CGT TTG ATC GGC GGA TTT -3' (this sequence was designated ODS0145) 5' GT~ TTG GTG CCT TCA ACC AGC GAC TGC TTC -3' (this sequence was designated ODS0146) Results of dot blot experiments employing P-labelled probe and pure chromosomal DNA preparations ~RD-77 ~9~
from 3 variety of organisms indicated that excellent specificity~sensitivity was obtained in the case of ODS0144 and ODS0146. Of the 8 Salmonella DNA preparations (representing all subgroups), only subgroup 5, the reptilean pathogen, was not detected. No cross-reactivity was seen with any DNA's from other organisms, i.e. 8 Citro~ ~Q~ strains, a Serratia marc~s~ens, M Qqanella moraanii, E. coli, En~erQbacter cloac~ Proteus mirabilis Yersinia ent~Qs~ icus, VibriQ
arahemolyticus. n-terob~ct-er-a-eroqenes~ as well as 4 Shi~ella species, were tested and were not probe reactive.
All of the probes as described herein are highly specific probes for detecting Salmonella organisms which are pathogenic in humans. They are clinically significant in the detection of Salmonella in diarrhea specimens.
Additionally, they would be useful in the detection of food-borne Salmonella, the causative agent of salmonellosis in humans.
3~
S. setubal 1 +
S. phoenix 1 +
Subaroup 3a Salmonella:
62:z4, Z23 - 1 +
431 3 4 Z4'z23 - 1 +
18:Z~,Z32:-62:Z36: 1 +
481,482:z4,z24:- 1 +
Su~qroup 3b Salmonella:
65:(k):z 1 +
61:k:1,S,(7) 1 +
1,3,4 1 +
1,2,3 ~ 1 +
38:(k3:Z35 1 +
Salmonella:
431,3,4 Z29 1 +
44:z :-S. wassenaar S. fl;nt 1 +
$~bqroup 5 Salmonella:
48, 4827 482:2:- 1 _ 5 S. brookfield S. marogrosso S. malawi Sub~rou~ 6 :LO
Salmonella-ll:b:1,7 41:b:1,7 1 +
S. ferlac 1 +
:L5 S. vrindaban 1 +
Other q~nera E. coli 6 ,'0 Enteric Group 90 2 Citrobacter freundii 2 ~ and -Enterobacter hafniae The above strains were obtained from the CDC, ~tlanta, GA, complements of Dr. J.J. Farmer III and Alma C. McWhorter.
With some exceptions, the two probes ODS0098 and ODS0100 (a 48mer and a 50mer, respectively) showed esc~llent specificity and sensitivity. The probes reacted specifically with all Salmonella subgroups related to human pathogenesis (Subgroup 5 is a reptilean pathogen;
the probes do not react with organisms from this subgroup). Of khe non-Salmonellae biochemically or serologically-related organisms e~amined, only one of two Citrobacter freundii cross-reacted with the probes.
-~3-7~
To attain greater specificity, a series of shorter oligometric probes, 17-l9 bases long were examined. The discr~te nucleotide sequences below were synthesized for testing:
5'- ATT GCG AGT CTG ATG TTT G -3' (this sequence was designated ODS0111) 5'- TGC AGC CTG TGC CGT CAG C -3' (this sequence was designated ODS0112) 5'- TCT GCG GAC AAT AGC ACT A -3' (this sequence was designated ODS0113) 5'- GTT GAA GGC ACC AAT AC -3' (this sequence was designated ODS0114) 5'- TGC CGT TCC CTG ACG GGA -3' (this sequence was designated ODS0115) 5'- GCG TGC GGT AAA ACG CAG -3' (this sequence was designated ODS0116) 5'- CCC GAC GCC GGT TGC GG -3' (this sequence was designated ODS0117 5'- GGC CGC CAC TTT CGG AT -3' (this sequence was designated ODS0118) 5'- GTT TGA TCG GCG GAT TT -3' (this sequence was designated ODS0119) 5'- GCT CAC CGG AGT AGG ATC -3' ~this sequence was designated ODS0120) ~(3~
Each of these probes ~ere 32P-labelled and tested in colony hybridization experiments against 34 Salmonella strains, 5 ~itrobac~qr strains, a Ent Qob cter hafniae and an E. coli strain. Five of the 10 probes elicited non-crossreactive hybridization patterns. However, the shorter probes sacrifice sensitivity with the concomitant gain in specificity, i.e., a small number of Salrnonella~
(other than subgroup 5) were non-reactive, resultant of the use of short probes.
:LO
Probes of about 30 bases in length were also tested.
These probes were synthesized as 5' or 3' extensions of ODS0111, ODS0113, ODS0114, ODS0116 and ODS0119. The discrete nucleotide sequences below were tested:
5' ATT GCG AGT CTG ATG TTT GTC GCT GGC GCA -3' (this sequence was designated ODS0137) 5' GCG TGC GGT AAA ACG CAG CGT ATT GGT GCC TTC AAC -3' (this sequence was designated ODS0139) 5' TAG TGC TAT TGT CCG CAG AGG AGA CAG CCA -3' (this sequence was designated ODS0143) 5' GCC GGT TGC GGT AGT GCT ATT GTC CGC AGA -3' (this sequence was designated ODS0144) 5' ACC CAG CGT CAC CGT TTG ATC GGC GGA TTT -3' (this sequence was designated ODS0145) 5' GT~ TTG GTG CCT TCA ACC AGC GAC TGC TTC -3' (this sequence was designated ODS0146) Results of dot blot experiments employing P-labelled probe and pure chromosomal DNA preparations ~RD-77 ~9~
from 3 variety of organisms indicated that excellent specificity~sensitivity was obtained in the case of ODS0144 and ODS0146. Of the 8 Salmonella DNA preparations (representing all subgroups), only subgroup 5, the reptilean pathogen, was not detected. No cross-reactivity was seen with any DNA's from other organisms, i.e. 8 Citro~ ~Q~ strains, a Serratia marc~s~ens, M Qqanella moraanii, E. coli, En~erQbacter cloac~ Proteus mirabilis Yersinia ent~Qs~ icus, VibriQ
arahemolyticus. n-terob~ct-er-a-eroqenes~ as well as 4 Shi~ella species, were tested and were not probe reactive.
All of the probes as described herein are highly specific probes for detecting Salmonella organisms which are pathogenic in humans. They are clinically significant in the detection of Salmonella in diarrhea specimens.
Additionally, they would be useful in the detection of food-borne Salmonella, the causative agent of salmonellosis in humans.
3~
Claims (30)
1. A nucleotide probe comprising at least a part of a nucleotide sequence encoding a virulence factor involved in the human pathogenesis of Salmonella infection, said probe capable of hybridizing to complementary target nucleic acid of Salmonella and signalling such hybridization through a detectable label.
2. The probe of Claim 1 wherein said virulence factor is a protein produced by microorganisms from the genus Salmonella, wherein said microorganisms belong to a Subgroup selected from the group consisting essentially of Subgroup 1, Subgroup 2, Subgroup 3a, Subgroup 3b, Subgroup 4, and Subgroup 6.
3. The probe of Claim 2 wherein said virulence factor is produced by a microorganism from the genus Salmonella, wherein said microorganism belongs to a Subgroup selected from the group consisting essentially of Subgroup 1, Subgroup 3a and Subgroup 3b.
4. The probe of Claim 2 wherein said virulence factor is a fimbrial-type protein.
5. The probe of claim 4 wherein said protein is selected from the group consisting of Type 1 fimbriae, Type 2 fimbriae and Type 3 fimbriae.
6. The probe of Claim 5 wherein said protein is Type 1 fimbriae protein.
7. The probe of Claim 1, capable of hybridizing to complementary target nucleic acid derived from a microorganism belonging to at least one Salmonella Subgroup selected from the group consisting of Subgroup 1, Subgroup 2, Subgroup 3a, Subgroup 3b, Subgroup 4, and Subgroup 6.
8. A probe according to Claim 7 which does cross hybridize with DNA from organisms selected from the group consisting of:
Salmonella subgroup 5 (reptile pathogen), Citrobacter freundii, Serratia marcescens, Morganella morganii, Escherichia coli, the genus Enterobacter, Vibrio cholerae, Proteus mirabilis, the genus Shigella, and the genus Campylobacter.
Salmonella subgroup 5 (reptile pathogen), Citrobacter freundii, Serratia marcescens, Morganella morganii, Escherichia coli, the genus Enterobacter, Vibrio cholerae, Proteus mirabilis, the genus Shigella, and the genus Campylobacter.
9. A probe according to Claim 8 having at least about 18 nucleotide bases.
10. A probe according to Claim 9 having at least about 25 nucleotide bases.
11. A probe according to Claim 8 having about 25 to about 150 nucleotide bases.
12. A probe according to Claim 11 having about 25 to about 50 nucleotide bases.
13. A probe according to Claim 12 that is complementary to a nucleic acid sequence that encodes a protein involved in the human pathogenesis of Salmonella infection.
14. A probe according to Claim 13 having a sequence of at least about 30 nucleotide bases that is complementary to a nucleic acid sequence that encodes 2 protein involved in said human pathogenesis.
15. A probe according to Claim 14 wherein said protein is a fimbrial-type protein.
16. A probe according to Claim 15 wherein said protein is a type 1 fimbriae protein.
17. A probe according to Claim 16 comprising a part of the following sequence:
18. A probe according to Claim 17 comprising all or a part of at least one sequence selected from the group consisting essentially of:
, , , , , , , , , , , , , , , , and .
, , , , , , , , , , , , , , , , and .
19. A probe according to Claim 18 comprising at least one nucleotide sequence selected from the group consisting of:
, ; and a nucleotide sequence complementary to either one or both.
, ; and a nucleotide sequence complementary to either one or both.
20. A nucleic acid probe comprising a subset, derivative, subclone or mutation of all or part of said at least one nucleotide sequence of Claim 19, said probe capable of hybridizing to target analyte from a microorganism belonging to the genus Salmonella, said microorganism causing human pathogenicity.
21. The nucleic acid probe of Claim 19 further comprising a 3' tail nucleotide sequence having a detectable label bound thereon.
22. The nucleic acid probe of Claim 21 wherein said detectable label is biotin.
23. A probe according to Claim 1 wherein said complementary target nucleic acid from a microorganism in the genus Salmonella is chromosomal DNA.
24. A probe according to Claim 1 wherein said complementary target nucleic acid is RNA.
25. The nucleic acid probe of Claim 1 wherein said detectable label is bound to a 3' tail nucleotide sequence.
26. The probe of Claim 22 wherein said detectable label is a hapten.
27. The probe of Claim 23 wherein said hapten is selected from the group consisting of biotin, iminobiotin, and fluorescein.
28. A reagent for use in detecting nucleic acid from human pathogenic microorganisms from the genus Salmonella comprising at least one nucleic acid probe of Claim 15 dispersed in a buffer solution.
29. A reagent according to Claim 28 comprising at least one nucleic acid probe having at least one nucleotide sequence selected from the group consisting of , and ; and a complementary sequence to one or both.
30. The reagent of Claim 29 further comprising a hybridization enhancer;
a detergent; and carrier DNA.
a detergent; and carrier DNA.
Applications Claiming Priority (2)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US30944189A | 1989-02-13 | 1989-02-13 | |
| US309,441 | 1989-02-13 |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CA2009708A1 true CA2009708A1 (en) | 1990-08-13 |
Family
ID=23198249
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CA002009708A Abandoned CA2009708A1 (en) | 1989-02-13 | 1990-02-09 | Nucleic acid probe for the detection of salmonella human pathogens |
Country Status (8)
| Country | Link |
|---|---|
| US (1) | US5486454A (en) |
| EP (1) | EP0383509B1 (en) |
| JP (1) | JPH02295498A (en) |
| AT (1) | ATE122728T1 (en) |
| CA (1) | CA2009708A1 (en) |
| DE (1) | DE69019393T2 (en) |
| ES (1) | ES2074533T3 (en) |
| GR (1) | GR1000695B (en) |
Families Citing this family (16)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| FR2664614B1 (en) * | 1990-07-11 | 1992-10-16 | Pasteur Institut | NUCLEIC SEQUENCES FROM THE GENOME OF SALMONELLA TYPHI, AND THEIR USES IN PARTICULAR FOR THE IN VITRO DIAGNOSIS OF THE PRESENCE OF BACTERIA OF THE GENUS SALMONELLA IN FOOD PRODUCTS. |
| IE913456A1 (en) * | 1990-10-01 | 1992-04-08 | Mini Agriculture & Fisheries | Salmonella polynucleotide sequence |
| NL9100510A (en) * | 1991-03-21 | 1992-10-16 | Centraal Diergeneeskundig Inst | DNA SEQUENCES CODING FOR CHARACTERISTICS OF VIRULENCE OF STREPTOCOCCUS SUIS AND PARTS THEREOF, DERIVATIVES OF POLYPEPTIDES AND ANTIBODIES, AND USE THEREOF IN THE DIAGNOSIS AND PROTECTION AGAINST INFECTION WITHOUT SUCH ANIMALS. |
| WO1993004202A1 (en) * | 1991-08-22 | 1993-03-04 | Washington University | Polynucleotide probes for salmonella |
| GB9207069D0 (en) * | 1992-03-31 | 1992-05-13 | Mini Agriculture & Fisheries | Method of testing for salmonella |
| CA2161404A1 (en) * | 1993-04-26 | 1994-11-10 | William W. Kay | Methods and compositions for salmonella-based vaccines |
| DE4337295A1 (en) * | 1993-11-02 | 1995-05-04 | Merck Patent Gmbh | Oligonucleotides for detecting Enterobacteriaceae |
| LT3828B (en) | 1993-11-10 | 1996-03-25 | Fermentas Biotech Inst | Process for detecting salmonella bacteries and probe for the same |
| US6290959B1 (en) * | 1996-10-24 | 2001-09-18 | New York University | Method for screening compounds for inhibiting bacterial attachment to host cell receptors |
| US6664045B1 (en) | 1998-06-18 | 2003-12-16 | Boston Probes, Inc. | PNA probes, probe sets, methods and kits pertaining to the detection of microorganisms |
| NZ530343A (en) | 2001-06-22 | 2007-01-26 | Marshfield Clinic | Methods and oligonucleotides for the detection of E. coli 0157:H7 |
| WO2005017488A2 (en) * | 2003-01-23 | 2005-02-24 | Science Applications International Corporation | Method and system for identifying biological entities in biological and environmental samples |
| US20060240442A1 (en) * | 2005-04-20 | 2006-10-26 | Vevea Dirk N | Methods and oligonucleotides for the detection of Salmonella SP., E coli 0157:H7, and Listeria monocytogenes |
| US20060246463A1 (en) * | 2005-04-20 | 2006-11-02 | Vevea Dirk N | Methods and oligonucleotides for the detection of Salmonella SP., E coli 0157:H7, and Listeria monocytogenes |
| WO2007027936A2 (en) * | 2005-09-01 | 2007-03-08 | The General Hospital Corporation | Methods and compositions for the diagnosis of a salmonella spp. infection |
| CN101659992B (en) * | 2009-03-20 | 2011-11-16 | 曹际娟 | Detection kit and detection method for 5 new pathogens in foods |
Family Cites Families (12)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| US4458066A (en) * | 1980-02-29 | 1984-07-03 | University Patents, Inc. | Process for preparing polynucleotides |
| US4358535A (en) * | 1980-12-08 | 1982-11-09 | Board Of Regents Of The University Of Washington | Specific DNA probes in diagnostic microbiology |
| US4717653A (en) * | 1981-09-25 | 1988-01-05 | Webster John A Jr | Method for identifying and characterizing organisms |
| FI63596C (en) * | 1981-10-16 | 1983-07-11 | Orion Yhtymae Oy | MICROBIA DIAGNOSIS FOERFARANDE SOM GRUNDAR SIG PAO SKIKTSHYBRIDISERING AV NUCLEINSYROR OCH VID FOERFARANDET ANVAENDA KOMBINATIONER AV REAGENSER |
| US4556643A (en) * | 1982-07-26 | 1985-12-03 | Agracetus | Assay method and probe for polynucleotide sequences |
| JPS5984162A (en) * | 1982-11-05 | 1984-05-15 | Toshiba Corp | Immunological analysis method |
| US4689295A (en) * | 1983-01-20 | 1987-08-25 | Integrated Genetics, Inc. | Test for Salmonella |
| US4533628A (en) * | 1983-08-03 | 1985-08-06 | New York University | Colony hybridization method |
| FR2567541B1 (en) * | 1984-07-13 | 1987-02-06 | Pasteur Institut | DNA PROBE AND METHOD FOR THE DETECTION OF "SHIGELLES" AND ENTERO-INVASIVE STRAINS OF ESCHERICHIA COLI |
| GB8422650D0 (en) * | 1984-09-07 | 1984-10-10 | Technology Licence Co Ltd | Monoclonal antibodies |
| AU6834187A (en) * | 1985-12-17 | 1987-07-15 | Genetics Institute Inc. | Displacement polynucleotide method and reagent complex |
| US4851331A (en) * | 1986-05-16 | 1989-07-25 | Allied Corporation | Method and kit for polynucleotide assay including primer-dependant DNA polymerase |
-
1990
- 1990-02-09 CA CA002009708A patent/CA2009708A1/en not_active Abandoned
- 1990-02-12 DE DE69019393T patent/DE69019393T2/en not_active Expired - Fee Related
- 1990-02-12 AT AT90301440T patent/ATE122728T1/en not_active IP Right Cessation
- 1990-02-12 EP EP90301440A patent/EP0383509B1/en not_active Expired - Lifetime
- 1990-02-12 ES ES90301440T patent/ES2074533T3/en not_active Expired - Lifetime
- 1990-02-12 GR GR900100091A patent/GR1000695B/en unknown
- 1990-02-13 JP JP2032279A patent/JPH02295498A/en active Pending
-
1994
- 1994-05-17 US US08/243,749 patent/US5486454A/en not_active Expired - Lifetime
Also Published As
| Publication number | Publication date |
|---|---|
| GR1000695B (en) | 1992-10-08 |
| EP0383509B1 (en) | 1995-05-17 |
| JPH02295498A (en) | 1990-12-06 |
| GR900100091A (en) | 1991-06-28 |
| EP0383509A2 (en) | 1990-08-22 |
| ES2074533T3 (en) | 1995-09-16 |
| DE69019393D1 (en) | 1995-06-22 |
| EP0383509A3 (en) | 1991-04-03 |
| DE69019393T2 (en) | 1995-10-05 |
| US5486454A (en) | 1996-01-23 |
| ATE122728T1 (en) | 1995-06-15 |
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| FZDE | Discontinued |