Construction method of PRV gE/gI dual-gene deletion strains for expressing ASFV P30 protein
The invention discloses a construction method of PRV gE/gI dual-gene deletion strains for expressing ASFV P30 protein and belongs to the biopharmaceutical field. The construction method specially comprises the following steps of S1, preparing a reagent; S2, preparing cloned plasmids; S3, constructin...
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Language | Chinese English |
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31.07.2020
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Abstract | The invention discloses a construction method of PRV gE/gI dual-gene deletion strains for expressing ASFV P30 protein and belongs to the biopharmaceutical field. The construction method specially comprises the following steps of S1, preparing a reagent; S2, preparing cloned plasmids; S3, constructing a PRV eukaryon transfer plasmid pEGFP-CP204L; S4, performing cotransfection on DNA of PRV and pEGFP-CP204L plasmids. P30 protein gene (CP204L) fragments are synthesized, the transfer plasmid pEGFP-CP204L is constructed, a classical homologous recombination manner is adopted for inserting an ASFV CP204L gene into a PRV genome to replace gI and gE virulence genes, and recombinant pseudorabies virus strains rXJgE/gI-CP204L for constructing co-expression P30 protein can be used for preventing ASFVand PRV infection, and the cloned plasmids are simple to prepare, low in cost and suitable for industrial production.
本发明公开了生物医药领域的一种表达ASFV P30蛋白的PRV gE/gI双基因缺失株的构建方法,具体包括以下步骤,S1:试剂准备;S2:克隆质粒的制备;S3:构建PRV真核转移质粒pEGFP-CP204L;S4 |
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AbstractList | The invention discloses a construction method of PRV gE/gI dual-gene deletion strains for expressing ASFV P30 protein and belongs to the biopharmaceutical field. The construction method specially comprises the following steps of S1, preparing a reagent; S2, preparing cloned plasmids; S3, constructing a PRV eukaryon transfer plasmid pEGFP-CP204L; S4, performing cotransfection on DNA of PRV and pEGFP-CP204L plasmids. P30 protein gene (CP204L) fragments are synthesized, the transfer plasmid pEGFP-CP204L is constructed, a classical homologous recombination manner is adopted for inserting an ASFV CP204L gene into a PRV genome to replace gI and gE virulence genes, and recombinant pseudorabies virus strains rXJgE/gI-CP204L for constructing co-expression P30 protein can be used for preventing ASFVand PRV infection, and the cloned plasmids are simple to prepare, low in cost and suitable for industrial production.
本发明公开了生物医药领域的一种表达ASFV P30蛋白的PRV gE/gI双基因缺失株的构建方法,具体包括以下步骤,S1:试剂准备;S2:克隆质粒的制备;S3:构建PRV真核转移质粒pEGFP-CP204L;S4 |
Author | ZHU LING XU ZHIWEN ZENG YUBING |
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DocumentTitleAlternate | 一种表达ASFV P30蛋白的PRV gE/gI双基因缺失株的构建方法 |
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Snippet | The invention discloses a construction method of PRV gE/gI dual-gene deletion strains for expressing ASFV P30 protein and belongs to the biopharmaceutical... |
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Title | Construction method of PRV gE/gI dual-gene deletion strains for expressing ASFV P30 protein |
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