PCR (Polymerase Chain Reaction) detection primer for phytophthora capsici leonian, kit containing primer and application thereof
A technology for Phytophthora capsicum and detection primers, which is applied in the field of PCR detection primers for Phytophthora capsicum, can solve the problems of small sequence differences, no specific Phytophthora capsicum detection primers related reports, low resolution, etc. Good specificity and high sensitivity
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Embodiment 1
[0037] Embodiment 1 is used to detect the synthesis of the PCR primer of Phytophthora capsici
[0038] Select the Enl and Ypt gene sequences of Phytophthora capsici and other Phytophthora from the GenBank database, and the involved sequences are shown in Table 2:
[0039] Table 2 Enl and Ypt gene sequences involved in the present invention
[0040]
[0041] Using DNAMAN and other biological software to compare and analyze the above-mentioned Enl and Ypt gene sequences, design Phytophthora capsici-specific primers located on Enl and Ypt genes, and obtain four pairs of specific primers, the sequences of which are shown in Table 1:
[0042] Table 1 Phytophthora capsici specific primer sequence involved in the present invention
[0043]
[0044]
[0045] *W is A or T.
[0046] The primers were synthesized by Shanghai Yingjun Biotechnology Co., Ltd.
Embodiment 2
[0047] Example 2 Utilize PCR primers Enl4s / Enl1a to detect the specificity and sensitivity analysis of Phytophthora capsici
[0048] 1.1 Sample source:
[0049] The six strains of Phytophthora capsici used in this example, Phytophthora infestans, Phytophthora cucumber, Phytophthora sojae, Phytophthora falciparum, Phytophthora lychee, Pythium ultima, Pythium maloestrogens, Phytophthora spinosa, Pythium solani, Fusarium, etc. (Table 3) are preserved in the State Key Laboratory of Mycology, Institute of Microbiology, Chinese Academy of Sciences and the laboratory of Professor Liu Xili, China Agricultural University, and some pathogens were donated by the laboratory of Professor Zhang Xiuguo, Shandong Agricultural University.
[0050] Table 3 Sources of samples used for PCR testing
[0051]
[0052]
[0053] 1.2 DNA extraction:
[0054] Refer to the NaOH method described in Wang et al. (Nucleic Acids Research, 1993, 21:4153-4154), slightly modified to extract DNA from plan...
Embodiment 3
[0065] Example 3 Utilize PCR primers Enl2s / Enl3a to detect the specificity and sensitivity analysis of Phytophthora capsici
[0066] The primers used in the PCR reaction are Enl2s and Enl3a, the PCR amplification procedure and the detection method of the amplified product are the same as in Example 2, and the specificity and sensitivity analysis methods of the primers are the same as in Example 2.
[0067] After the amplification reaction, the amplified products were detected by electrophoresis on a 1% agarose gel. If a band of about 300bp appears, it proves that the detected pathogen is Phytophthora capsici. The results of electrophoresis were as image 3 As shown, lanes 1-6 are samples of Phytophthora capsici, and DNA bands of about 300 bp can be amplified, while no bands appear in other species, Pythium species and Fusarium species. The above results indicated that the primers Enl2s and Enl3a had strong specificity.
[0068] The PCR amplification reaction was carried out...
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