A real-time fluorescent quantitative PCR detection kit for aphthous ulcer virus
A real-time fluorescence quantitative, aphthous virus technology, applied in the field of virus molecular biology detection
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Embodiment 1
[0036] Example 1 Design of primers and Taqman probes for real-time fluorescent quantitative PCR detection of aphthous ulcer virus
[0037] Referring to the full genome sequence of the ORFV NZ2 strain of oropharyngeal virus (GenBank accession No.DQ184476.1) collected by GenBank, select the conserved region of the ORFV 024 gene, which is [ORFV NZ2 strain genome (GenBank accession No.DQ184476.1) 23758bp-23844bp fragment , using ABI Primer Express 3.0 and Primer 5.0 primer design software to design and synthesize real-time fluorescent quantitative PCR primers and probes. At the 5' end of the probe, FAM was selected as the fluorescent labeling reporter luminescent group, and at the 3' end Tamara was used as the quenching group.
[0038] The sequence is as follows:
[0039] Upstream primer (ORFV-Forward primer): 5'-TCTGTGCATGCTCAAGATCCT -3' (SEQ ID NO: 1 in the sequence listing);
[0040] Downstream primer (ORFV-Reverse primer): 5'-GCCAAGTTGCAGGTTTTTCTT -3' (SEQ ID NO: 2 in the se...
Embodiment 2
[0042] Example 2 Real-time fluorescent quantitative PCR detection of aphthous ulcer virus
[0043] 1. Establishment of standard curve
[0044] 1. Construction of pET21b-ORFV024 recombinant plasmid
[0045] (1) Clone the target gene ORFV024 gene of sheep oral disease virus
[0046] Strictly follow the requirements in the P2 laboratory negative pressure biosafety cabinet for the extraction of aphthus virus genomic DNA. The specific steps are as follows: collect the lip scabs of sheep infected with aphthous ulcer virus under aseptic conditions, grind them with a mortar, resuspend the powder in normal saline, take 200 μL of the suspension containing the virus, and use Roche High Pure Viral Nucleic Acid Kit ( Purchased from Roche Company, USA) According to the instructions, viral genomic DNA was extracted.
[0047] The PCR reaction system was 50 μL, and the following components were added in sequence: 5 μL 10×PCR buffer (purchased from Promega, USA), 2.0 mM MgCl 2 , 0.2mM dNTP...
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