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An improved system for constructing marker-free recombinant goatpox viruses to express foreign proteins

机译:一种改进的构建无组重建山羊毒病毒以表达外来蛋白质的改进系统

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摘要

Goatpox virus (GTPV), belonging to the genus Capripoxvirus in the family Poxviridae, causes a contagious disease affecting goats and sheep. Homologous recombination as a conventional method is commonly used to construct recombinant GTPVs but generally with genetic markers, such as enhanced green fluorescent protein (eGFP) and guanine phosphoribosyl transferase (gpt). We have previously constructed a recombinant GTPV, which can efficiently express the EG95 antigen of Echinococcus granulosus, but contains eGFP and gpt markers in viral genome. In this study, our previous GTPV-generating system was modified by reconstruction of a Loxp-containing transfer plasmid for deleting markers using the Cre/Loxp system. Meanwhile, the previous method was significantly improved by introduction of an immortalized goat testis cell line as a substitute for primary cells. Based on the latest system, a marker-free recombinant GTPV was reconstructed for expressing the EG95 antigen, and showed neither a significant difference in replication kinetics from its parental virus nor mutations in the foreign sequence during serial 10 passages in vitro.
机译:Goatpox病毒(GTPV)属于痘病毒族藻类属藻毒素,导致影响山羊和绵羊的传染病。作为常规方法的同源重组通常用于构建重组GTPV,但通常具有遗传标记,例如增强的绿色荧光蛋白(EGFP)和鸟嘌呤磷酰基转移酶(GPT)。我们以前构建了一种重组GTPV,其可以有效地表达Echinococcus颗粒的EG95抗原,但含有病毒基因组中的EGFP和GPT标记物。在该研究中,通过使用CRE / LOXP系统重建含LOXP的转移质粒来修饰我们之前的GTPV生成系统。同时,通过将永生化的山羊睾丸细胞系作为原代细胞的替代方法,先前的方法显着改善。基于最新的系统,重建了一种无标准的GTPV以表达EG95抗原,并且在体外连续10次通道期间,在其亲本病毒中的复制动力学中的复制动力学的突变既没有显着差异。

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