PCR primer for identifying codling moth cell line and identifying method of codling moth cell line
A technology of codling moth and cell line, applied in the field of agricultural biology, can solve the problems of poor repeatability, low sensitivity and the like, and achieve the effect of stabilizing the enzyme cleavage identification method
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Embodiment 1
[0028] Example 1: Amplification and sequence analysis of COI gene fragments in codling moth cell lines and several other insect cell lines
[0029] The applicant analyzed the COI gene partial sequence (SEQIDNo: 5) of the amplified codling moth cell line and the COI gene partial sequence (SEQIDNo: 6) amplified from the codling moth egg genome; Blast comparison was carried out in the NCBI database, Using DNASTAR software to compare and analyze the COI gene fragments of codling moth and several other insects, it was found that the nucleotide identity of COI gene of codling moth and black beetle was 81.6%, and that of COI gene nucleotide of beet armyworm The nucleotide sequence of COI gene of codling moth is 87.9%, and the nucleotide sequence of COI gene of Trichoplusia spp. is 83.9%. difference.
[0030] According to the sequence analysis results, the applicant designed the following primers:
[0031] Forward primer LCO1490: 5'-GGTCAACAAATCATAAAGATATTGG-3' (SEQ ID NO: 1),
[0...
Embodiment 2
[0049] The PCR-RFLP pattern of embodiment 2 several codling moth cell lines
[0050] (1) Extraction of genomic DNA from several codling moth cell lines
[0051] Seven codling moth cell lines Cp-E-4, Cp-E-6, Cp-E-9, Cp-E-10, Cp-E-11, Cp-E-12 and Cp - Genomic DNA was extracted from the cell suspension of E-13 with a MagExtractor-Genome kit to obtain genomic DNA solutions of each cell line of codling moth.
[0052] (2) PCR amplification of COI gene fragments in several codling moth cell lines
[0053] The genomic DNA solutions of several codling moth cell lines were respectively used as templates for PCR amplification to obtain PCR amplification products;
[0054] The PCR amplification system is:
[0055] Genomic DNA solution of codling moth cell line: 1 μL, 10 μmol / L forward primer: solution 1 μL, 10 μmol / L reverse primer solution: 1 μL, 5 U / μL Taq enzyme: 0.5 μL, 10×Taq buffer: 5 μL, 2.5mmol / LdNTP: 4μL, sterilized pure water: 37.5μL.
[0056] The primer sequences are as fo...
Embodiment 3
[0066] Example 3 The difference between codling moth cell lines and other several insect cell lines PCR-RFLP patterns
[0067] (1) Extraction of genomic DNA of codling moth, black gill beetle, beet armyworm and Trichoplusia spp.
[0068] MagExtractor-Genome Reagent for Cell Suspensions of Codling Moth Cell Line Cp-E-10, Black Beetle Cell Line Hp-E-1, Beet Spodoptera Cell Line Se-1, and Trichoplusia Tn9-4s Genomic DNA was extracted using the cassette, and the genomic DNA solutions of the codling moth, black beetle, beet armyworm and Trichoplusiae cell lines were obtained.
[0069] (2) PCR amplification of COI gene fragments of codling moth, black gill beetle, beet armyworm and Trichoplusia spp.
[0070] The genomic DNA solution of codling moth and the genomic DNA solution of cell lines of beetle moth, beet armyworm and Trichoplusia spp. were respectively used as templates for PCR amplification to obtain PCR amplification products.
[0071] The PCR amplification system is:
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