IPC분류정보
국가/구분 |
United States(US) Patent
등록
|
국제특허분류(IPC7판) |
|
출원번호 |
US-0995707
(2011-12-21)
|
등록번호 |
US-9238843
(2016-01-19)
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국제출원번호 |
PCT/US2011/066392
(2011-12-21)
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§371/§102 date |
20130619
(20130619)
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국제공개번호 |
WO2012/092054
(2012-07-05)
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발명자
/ 주소 |
- Weise, Dale Wade
- Harris, James Robert
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출원인 / 주소 |
|
대리인 / 주소 |
|
인용정보 |
피인용 횟수 :
0 인용 특허 :
18 |
초록
▼
Disclosed are methods and compositions for identifying viral-specific polynucleotide sequences in a biological sample, and particularly in samples of veterinary origin. Also disclosed are oligonucleotide primer pairs, as well as labeled oligonucleotide detection probes useful in detecting the presen
Disclosed are methods and compositions for identifying viral-specific polynucleotide sequences in a biological sample, and particularly in samples of veterinary origin. Also disclosed are oligonucleotide primer pairs, as well as labeled oligonucleotide detection probes useful in detecting the presence of one or more particular species, strains, types, or subtypes of one or more mammalian pathogens of viral origin, as well as systems, diagnostic kits and articles of manufacture comprising virus-specific primers and labeled detection probes, including those useful in identifying viral components of a multivalent vaccine, and quantitating the potency of particular attenuated, live viruses that comprise a livestock vaccine. In certain embodiments, real-time, quantitative PCR methods have been utilized to identify and distinguish between the three known genetic subtypes of bovine viral diarrhea viruses (BVDV-1a, BVDV-1b, and BVDV-2) in a multivalent bovid shipping fever vaccine.
대표청구항
▼
1. A method for detecting the presence of a BVDV-1b live virus, the method comprising: diluting a sample in (i) an assay plate containing cultured bovine cells in which live virus particles are capable of replicating and (ii) a corresponding reference plate without cells;contacting nucleic acids fro
1. A method for detecting the presence of a BVDV-1b live virus, the method comprising: diluting a sample in (i) an assay plate containing cultured bovine cells in which live virus particles are capable of replicating and (ii) a corresponding reference plate without cells;contacting nucleic acids from at least one sample dilution with a BVDV-1b virus-specific primer/probe set, said virus-specific primer/probe set comprising a forward BVDV-1b virus-specific oligonucleotide amplification primer, a reverse BVDV-1b virus-specific oligonucleotide amplification primer, and a BVDV-1b virus-specific oligonucleotide detection probe; andperforming at least one cycling step, wherein the at least one cycling step is performed using quantitative real-time polymerase chain reaction (qPCR);wherein said BVDV-1b virus-specific primer/probe set is useful in detecting the presence of a BVDV-1b viral-specific polynucleotide in a population of polynucleotides obtained from a plurality of bovine virus particles;wherein said plurality of bovine virus particles comprises at least one BVDV Type 1b virus particle; andwherein a higher level of a signal from a virus-specific oligonucleotide detection probe in the presence of nucleic acids from the assay plate compared to a signal from the virus-specific oligonucleotide detection probe in the presence of nucleic acids from the reference plate indicates the presence of a live bovine virus in the sample. 2. The method in accordance with claim 1, wherein the sample comprises modified, live bovine virus particles contained within a mammalian vaccine. 3. The method in accordance with claim 2, wherein the mammalian vaccine is a Bovine Respiratory Disease Complex (BRDC) or shipping fever vaccine. 4. The method in accordance with claim 1, wherein said plurality of bovine virus particles comprises a plurality of modified, live bovine virus particles; and wherein the plurality of bovine virus particles comprises at least one modified, live BVDV Type 1 b virus particle. 5. The method in accordance with claim 4, wherein the plurality of modified, live bovine virus particles further comprises at least one modified, live bovine virus particle selected from the group of a BVDV-1a, BVDV-2, BHV-1, PI3, or an BRSV virus particle. 6. The method in accordance with claim 4, wherein the plurality of modified, live bovine virus particles further comprises at least two different modified, live bovine virus particles selected from the group of a BVDV-1a, BVDV-2, BHV-1, PI3, or an BRSV virus particle. 7. The method according to claim 1, wherein the BVDV-1b virus-specific primer/probe set comprises: a forward virus-specific oligonucleotide amplification primer of less than, or about, 50 nucleotides in length comprising a nucleotide sequence of SEQ ID NO: 1;a reverse virus-specific oligonucleotide amplification primer of less than, or about, 50 nucleotides in length comprising a nucleotide sequence of SEQ ID NO: 2 ; anda virus-specific oligonucleotide detection probe of less than, or about, 50 nucleotides in length comprising a nucleotide sequence of SEQ ID NO: 3. 8. The method according to claim 1, wherein the at least one virus-specific primer/probe set consists of the nucleotide sequences of SEQ ID NO: 1, SEQ ID NO: 2, and SEQ ID NO: 3. 9. The method in accordance with claim 1, wherein the plurality of bovine virus particles further comprises at least one bovine virus particle selected from the group of a BVDV-1a, BVDV-2, BHV-1, PI3, or BRSV virus particle. 10. The method in accordance with claim 9, wherein the plurality of bovine virus particles further comprises at least two different bovine virus particles selected from the group of a BVDV-1a, BVDV-2, BHV-1, PI3, or an BRSV virus particle.
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