Infectivity scrapie resistance gene rapid typing detection reagent, preparation method and application thereof
A technology for detecting reagents and disease resistance is applied in the field of animal disease detection. The effect of closing the technology gap
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Embodiment 1
[0103] Example 1 Extraction of Goat Genomic DNA
[0104] The goat genomic DNA template of each genotype used in the invention is a gift from the Italian Institut zooprofilatticsperimen DELLA SARDEGNA, and the virus DNA is extracted according to the instructions of the Roche spinning column DNA extraction kit. Example 2 Design and synthesis of primers and probes for detecting codons 136, 154 and 171 of PRNP alleles
Embodiment 2
[0104] The goat genomic DNA template of each genotype used in the invention is a gift from the Italian Institut zooprofilatticsperimen DELLA SARDEGNA, and the virus DNA is extracted according to the instructions of the Roche spinning column DNA extraction kit. Example 2 Design and synthesis of primers and probes for detecting codons 136, 154 and 171 of PRNP alleles
[0105] According to (GenBank accession number: AY907689) PRNP gene sequence design the PRNP coding region 136 (A) codon MGB probe and primer; according to (GenBank accession number: AY907685) PRNP coding region 136 (V) ) MGB probes and primers for codons; according to (GenBank accession number: AY907685) PRNP gene sequence design MGB probes and primers for the 154th (R) codon of the PRNP coding region; according to (GenBank accession number: AY822666.1) PRNP gene sequence design PRNP coding region 154 (H) codon MGB probe and primer; according to (GenBank accession number: AB373795.1) PRNP gene sequence design PRNP co...
Embodiment 3
[0123] Example 3 Real-time PCR amplification of target gene
[0124] The gene amplification master mix Taqman Universal PCR MasterMix was purchased from Applied Biosystems Reagent Company, the real-time fluorescent quantitative PCR instrument was Roche LightCycler 480, and the fluorescent PCR tube (plate) and tube cap (sealing membrane) were purchased from Roche Company.
[0125] 1 Preparation of PCR reaction mixture
[0126] Take the DNA extracted in Example 1 as a template, and use the various fluorescent primers and probes designed in Example 2 to perform a fluorescent quantitative PCR reaction, and select 20 μL of the following PCR reaction system:
[0127] Template DNA: 2μL; Upstream primer (10μmol / L): 2μL; Downstream primer (10μmol / L): 2μL; FAM-labeled probe (10μmol / L): 0.5μL; VIC-labeled probe (10μmol / L): 0.5μL; 2×mastermix: 10μL; double distilled water to make up.
[0128] 136 upstream and downstream primers and 136A and 136V probes are a detection system used to identify 136 a...
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