Primer group, reagent and method for detecting feline parvovirus based on polymerase spiral reaction
A feline parvovirus and polymerase technology, which is applied in the field of reagents and primer sets for detection of feline parvovirus based on the polymerase helical reaction, can solve the problems of complex temperature-changing instruments, long detection time, and high detection cost, achieving good repeatability and low cost. Effect of Assay Cost, Strong Strand Displacement Activity
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Embodiment 1
[0041] 1. Primer Design
[0042] Use Oligo 6.0 software to design a pair of PCR primers for the conserved region of the FPV NS1 gene: FPV-F and FPV-R, the size of the amplified fragment is about 403bp, and design a pair of PSR-specific primers in the amplified fragment based on the PSR principle: PSR-FPVF, PSR-FPVR, and 1 pair of PSR accelerating primers: PSR-FPV-FJ, PSR-FPV-RJ. The PSR amplification product is a series of ladder-shaped bands. All primers were synthesized by Xi'an Branch of Beijing Qingke Biotechnology Co., Ltd. The specific primer names and sequences are listed in Table 1.
[0043] Table 1 PCR and PSR primers for detecting FPV
[0044]
[0045] 2. Nucleic acid extraction and copy number calculation
[0046] Use the viral nucleic acid extraction kit to extract viral nucleic acid from FPV positive samples, feline coronavirus (FCoV) positive samples, and feline norovirus (FNV) positive samples, respectively, use an ultramicro spectrophotometer to measure ...
Embodiment 2
[0055] In order to verify the influence of accelerating primers PSR-FPVF FJ and PSR-FPVF RJ on the experimental results, four sets of reaction systems were set up, the first group did not add any accelerating primers, the second group only added PSR-FPVF FJ, and the third group only added PSR -FPVF RJ, the fourth group joined both PSR-FPVF FJ and PSR-FPVF RJ. The detection method adopts the optimized result of Example 1.
[0056] see results figure 2 In the first group, a clear ladder-like band could be observed when the accelerated primer group was not introduced for 75 minutes; when the accelerated primer group was introduced, there was a PSR amplification product when the accelerated primer group was introduced for 45 minutes, but the fourth The electrophoretic bands of the first group were brighter than those of the second and third groups introduced with a single accelerated primer set at 45 minutes of reaction, indicating that the introduction of two accelerated primer...
Embodiment 3
[0058] With the FPV, FCoV and FNV genome nucleic acid that embodiment extracts as template, utilize the detection method of embodiment 1 and add acceleration primer PSR-FPVF FJ and PSR-FPVF RJ, carry out specificity test, set up simultaneously with sterilized water as template negative control.
[0059] see results image 3 , the results showed that no gene amplification occurred in the sterile water, FCoV and FNV groups, but gene amplification occurred in the FPV, FPV+FCoV, FPV+FNV, FPV+FCoV+FNV groups, see image 3 A. After the reaction, add a nucleic acid dye with a final concentration of 20×SYBRGreen I. Observe with the naked eye under visible light, and find that the three groups of sterilized water, FCoV and FNV are orange, FPV, FPV+FCoV, FPV+FNV, FPV+FCoV+FNV The color of the four groups changed from orange to green, which shows that the SYBR Green I staining results are consistent with the electrophoresis results, see image 3 B (Since the drawings in the description...
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