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Production and Characterization of the Ectodomain of E2 Envelope Glycoprotein of Hepatitis C Virus Folded in the Presence of Full-length E1 glycoprotein

机译:全长E1糖蛋白折叠的丙型肝炎病毒E2信封糖蛋白Ectodomain的生产和表征

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摘要

Hepatitis C virus (HCV) envelope glycoproteins, E1 and E2, are involved in the first steps of virus infection. The E2 ectodomain can be produced as an isolated form (E2661). However, there is some concern about its proper conformation and the role that E1 can play as a chaperone for the folding of E2. In order to verify this fact we have expressed a chimeric protein (E1tmbE2) based on the full-length E1 sequence followed by the E2 ectodomain using the baculovirus-insect cells system. The E2 ectodomain is folded in the presence of the E1, proteolytically processed by cellular proteases and secreted to cell culture media (E2661p), while the E1 protein is retained into the cell due to its transmembrane sequence. The purification of E2661p from culture media was facilitated by a His tag introduced in its amino terminus. Both E2661 and E2661p glycoproteins shared very similar structural features, monitored by spectroscopic and antigenic studies. Moreover, their functional properties, tested by means of CD81 binding, were almost indistinguishable, indicating that the E2 ectodomain constitutes an independent folding unit.
机译:丙型肝炎病毒(HCV)包膜糖蛋白E1和E2参与病毒感染的第一步。 E2胞外域可以作为分离形式产生(E2661)。但是,对于其适当的构象以及E1作为E2折叠伴侣的作用,存在一些担忧。为了验证这一事实,我们使用杆状病毒-昆虫细胞系统基于全长E1序列和其后的E2胞外域表达了一种嵌合蛋白(E1tmbE2)。 E2胞外域在E1存在时折叠,通过细胞蛋白酶进行蛋白水解处理并分泌到细胞培养基(E2661p)中,而E1蛋白由于其跨膜序列而保留在细胞中。从培养基中纯化E2661p的方法是在其氨基末端引入一个His标签。 E2661和E2661p糖蛋白均具有非常相似的结构特征,并通过光谱和抗原研究进行了监测。此外,通过CD81结合测试的功能特性几乎无法区分,表明E2胞外域构成了一个独立的折叠单元。

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