Method for synchronously detecting three kinds of viruses on tobacco through triple one-step method RT-PCR (Reverse Transcription Polymerase Chain Reaction)
A RT-PCR and virus technology, applied in the direction of microorganism-based methods, biochemical equipment and methods, recombinant DNA technology, etc., can solve the problems of increasing test pollution, manual misoperation, and many influencing factors, and reduce sample crossover Pollution, reduction of influencing factors, reliable results
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Embodiment 1
[0030] (1) Using DNAMAN6.0 software, compare the whole genome sequences of TMV, PVY, and CMV virus strains and isolates from various regions included in GenBank, and determine the relatively conserved regions in the virus sequences. Within the selected conserved regions Primers were designed using Oligo 6.0 software, and primer specificity was ensured by BLAST analysis. Since multiplex PCR requires the annealing temperature of each primer and primer pair to be as close as possible, and the size of the amplicon should be as similar as possible under the condition that agarose gel electrophoresis can be clearly distinguished, so a pair of TMV, PVY, and CMV were finally selected. Primers were artificially synthesized and dissolved in RNase-free water to a working concentration of 10 μM.
[0031] TMV: Upstream primer (TF1) 5'-TGTGTGCAAAACTTACTTCCC-3';
[0032]Downstream primer (TR1) 5'-AGGACAAAACATTTGCGTATG-3';
[0033] PVY: upstream primer (PF1) 5'-ACTGTGATGAATGGGCTTATG-3';
...
Embodiment 2
[0043] (1) Using DNAMAN6.0 software, compare the whole genome sequences of TMV, PVY, and CMV virus strains and isolates from various regions included in GenBank, and determine the relatively conserved regions in the virus sequences. Within the selected conserved regions Primers were designed using Oligo 6.0 software, and primer specificity was ensured by BLAST analysis. Since multiplex PCR requires the annealing temperature of each primer and primer pair to be as close as possible, and the size of the amplicon should be as similar as possible under the condition that agarose gel electrophoresis can be clearly distinguished, so a pair of TMV, PVY, and CMV were finally selected. Primers (primers are the same as in Example 1), artificially synthesized and dissolved in RNase-free water to a working concentration of 10 μM.
[0044] (2) Use the TMV, PVY, and CMV virus pathogens preserved in our laboratory to inoculate tobacco at the 6-8 leaf stage (not from the same plant) separatel...
Embodiment 3
[0049] (1) Using DNAMAN6.0 software, compare the whole genome sequences of TMV, PVY, and CMV virus strains and isolates from various regions included in GenBank, and determine the relatively conserved regions in the virus sequences. Within the selected conserved regions Primers were designed using Oligo 6.0 software, and primer specificity was ensured by BLAST analysis. Since multiplex PCR requires the annealing temperature of each primer and primer pair to be as close as possible, and the size of the amplicon should be as similar as possible under the condition that agarose gel electrophoresis can be clearly distinguished, so a pair of TMV, PVY, and CMV were finally selected. Primers (primers are the same as in Example 1), artificially synthesized and dissolved in RNase-free water to a working concentration of 10 μM.
[0050] (2) Use the TMV, PVY, and CMV virus pathogens preserved in our laboratory to inoculate tobacco at the 8-10 leaf stage (tobacco of the same plant) succes...
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