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机构地区:[1]中国预防医学科学院病毒学研究所
出 处:《中华实验和临床病毒学杂志》1999年第2期117-120,共4页Chinese Journal of Experimental and Clinical Virology
基 金:国家"九五"攻关课题
摘 要:目的研究HGVNS3区基因产物的抗原性,并探讨NS3蛋白在血清学检测中的应用。方法将中国株HGVNE3区的3个基因片段分别克隆到pRSETB和pRSETC质粒载体中,构建成原核表达载体。IPTG诱导下,在大肠杆菌BL21中高效表达,获得3个重组蛋白,用Westernblot和ELISA法分别对表达产物进行分析。结果所构建的表达载体均得到高效表达,得到的重组蛋白PA、P3和P4的分子量分别为42000,30000和24000,在Westernblot和ELISA反应中均可被HGV阳性血清识别,其中HGVNS3区N端的基因产物抗原性较强。结论中国株HGVNS3区的N端存在优势的抗原决定簇,其基因产物有较好的抗原性。Objective This study is to analyze the antigenicity of the NS3 proteins of Chinese HGV and their potential use in the serological diagnosis. Methods All three gene fragments of NS3 region of Chinese HGV were cloned into the pRSET vectors to construct recombinant plasmids. In E.coli BL21, all three recombinant plasmids achieved a high expression level with induction of IPTG. The expressed products were analyzed with Western blot and ELISA. Results The recombinant protein PA, P3 and P4 have a molecular weight of 42 000, 30 000 and 24 000, respectively. They all could react with HGV positive sera in Western blot and ELISA. Among them, the protein that covers the N terminal of NS3 region of HGV had a stronger reaction with HGV positive sera than the other two proteinsdid. Conclusion The N terminal in the NS3 region of Chinese HGV includes an dominant antigenic determinant, and its gene product has relatively strong antigenicity.
关 键 词:GBV-C/HGV 大肠杆菌 基因表达 抗原性分析
分 类 号:R378.21[医药卫生—病原生物学]
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