A specific detection target of Phytophthora syringae psyri_s00018g00015.1 and its application
A Phytophthora syringae, specific technology, applied in the application, microbial determination/inspection, resistance to vector-borne diseases, etc., can solve the problems of long cycle, poor specificity and low sensitivity of detection methods, and achieve fast and accurate detection. high sex effect
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Embodiment 1
[0040] More than 1,100 Phytophthora syringae-specific genes were obtained by whole-genome sequence alignment, and some genes were randomly selected from more than 1,000 Phytophthora syringae specific genes as candidate genes ( Psyri_s00018g00015.1, Psyri_ s00001g00003.1, Psyri_s00001g00023.1Psyri_s00016g00009.1, Psyri_ s00024g00013.1 ), designed and screened specific primers, and Table 1 lists the five target genes and upstream and downstream detection primers (Table 1).
[0041] Table 1 Sequences and primers of five specific genes of Phytophthora syringae
[0042]
[0043] Select different species from Phytophthora syringae (Phytophthora cedar; .
[0044] Sample detection: To a 0.2 mL TwistAmp reaction unit tube (TwistAmp Basickits, Twist) containing lyophilized enzyme powder, add Buffer 29.5 μL, 10 μM upstream primer 2.1 μL, 10 μM downstream primer 2.1 μL, probe 0.6 μL, Add 2.0 μL of DNA and 2.5 μL of MgAc to the inside of the PCR tube lid, and make up to 50 μL of ...
Embodiment 2
[0050] To further verify the specificity of the RPA lateral flow chromatography test strip detection method, Phytophthora syringae strains and other Phytophthora and pathogenic bacteria were used as test materials (Table 2). The results of the RPA lateral flow chromatography test strip detection method showed that the The test strips for Phytophthora show two brown bands, one in the Control Line and the other in the Test Line, then the result is positive, while the test strips for other Phytophthora and pathogenic bacteria only have quality control A brown band appears in the test area, and there is no band in the test area (TestLine), the result is negative, indicating that the sample does not contain Phytophthora syringae.
[0051] Select different species from Phytophthora syringae (Phytophthora cedar; Fusarium; anthracnose flathead; Verticillium dahliae; Rhizoctonia solani; M. oryzae, etc.) DNA was used as a template for RPA-LFD (lateral flow chromatography test strip dete...
Embodiment 3
[0057]The genomic DNA of the standard strain of Phytophthora syringae with the same concentration was used as the amplification template, and the upstream and downstream primers Psyri015.1F / Psyri015.1R were used for PCR amplification reaction to compare the sensitivity of the two methods; repeat the experiment 3 times to determine the PCR Sensitivity of Phytophthora syringae genomic DNA detection by the method; the results of three repeated experiments were consistent. The genomic DNA concentration is 1 ng μL -1 , PCR detection can detect specific bands, and the results are as follows Figure 5 As shown, it was proved that specific amplification occurred, and the test result was judged to be positive. After utilizing the RPA amplification reaction of the present invention, the detection result of the LFD lateral flow chromatography test strip is as follows: Image 6 The indicated target bands are resolved. It can be seen that based on the same new excavation target Psyri_...
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