Animal Torque Teno virus rapid detection kit and detection method using loop-mediated isothermal amplification technology
A ring-mediated isothermal and detection kit technology, applied in the direction of microorganism-based methods, biochemical equipment and methods, microorganism measurement/testing, etc., can solve the problem of thermal amplification gene technology detection animal TorqueTenovirus kit and detection method, No problems such as animal TorqueTeno virus have been seen yet, achieving the effect of simple identification, high sensitivity and high sensitivity
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Embodiment 2
[0057] Embodiment 2, design and screening of primers of the present invention
[0058] According to the genome full-length sequence of known TTV1 (AY823990.1) and TTV2 (AY823991.1) nucleotide sequence, utilize ClustW software to carry out multiple alignment, design specific primers with LAMP primer design software Primer Explorer V4.0 software, Marked respectively as: SEQ ID NO1...SEQ ID NO8. All primers were synthesized by Bao Biological Engineering (Dalian) Co., Ltd. The TTV virus DNA was extracted with a commercially available virus nucleic acid extraction kit, amplified, and primers with non-specific amplification were excluded. Get the primers as follows:
[0059]
Embodiment 3
[0060] Embodiment 3, the preparation of positive control substance
[0061] The viral DNA of positive porcine TTV1 and TTV2 was extracted with a commercially available nucleic acid extraction kit, and then amplified by PCR. The amplified lengths were 449 bp for TTV1 and 468 bp for TTV2, respectively. The amplified target band was recovered, ligated with the pMD19-T vector, ligated overnight at 4°C, transformed into JM109 competent cells, and the recombinant plasmid was extracted from those positive for resistance screening, shaking bacteria, and PCR. Sequence verification, obtain the clone containing the target fragment, mix the positive plasmids of the two serotypes in equal proportions, aliquot each 50 μL, and control the concentration at 80-100 ng / μL.
Embodiment 4
[0062] Embodiment 4, the preparation of negative control substance
[0063] Commercially available commercial nucleic acid extraction kits were used to extract the DNA of the negative sera not containing porcine TTV1 and TTV2, respectively. Dilute with sterilized deionized water, control the concentration at 80-100ng / μL, and pack into 50μL each.
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