PCR-RFLP (Polymerase Chain Reaction-Restricted Fragment Length Polymorphisms) method for distinguishing clade2.3.2.1 from clade2.3.4 H5 AIVs (Avian Influenza Virus)
A technology of RT-PCR and amplification products, applied in the field of rapid diagnosis of veterinary infectious diseases, can solve problems such as difficult identification by molecular biology methods, and achieve the effects of rapid and accurate rapid differential diagnosis and detection, high accuracy, and simple identification methods.
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[0026] 1. Extract the nucleic acid RNA of the virus;
[0027] (1) Virus source:
[0028] H5 subtype influenza virus clade 2.3.4 branch (CX1 strain) and clade 2.3.2.1 branch (DY1 strain) were both preserved by the Institute of Animal Husbandry and Veterinary Medicine, Fujian Academy of Agricultural Sciences.
[0029] (2) Extract viral RNA:
[0030] The nucleic acid RNAs of clade 2.3.4 branch (CX1 strain) and clade 2.3.2.1 branch (DY1 strain) H5AIV were extracted by conventional methods for RT-PCR amplification.
[0031] 2. RT-PCR amplification
[0032] (1) Design and selection of amplification primers:
[0033] According to the HA gene characteristics of clade 2.3.4 H5 AIV and clade 2.3.2.1 H5 AIV, the upstream primer P1 and downstream primer P2 were designed, wherein the sequences of the primers are as follows:
[0034] Upstream primer P1: 5'-ATGCAAACAACTCGACAG-3',
[0035] Downstream primer P2: 5'-ATCTCTGGTTTAGTGTTGATGT-3'.
[0036] Such as figure 1Shown: there are nuc...
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