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标签化 p7 衣壳蛋白在丙型肝炎病毒生产细胞中的亚细胞定位和功能。

Subcellular localization and function of an epitope-tagged p7 viroporin in hepatitis C virus-producing cells.

机构信息

Institute of Experimental Virology, Twincore, Centre for Experimental and Clinical Infection Research, Hannover, Germany.

出版信息

J Virol. 2013 Feb;87(3):1664-78. doi: 10.1128/JVI.02782-12. Epub 2012 Nov 21.

Abstract

The hepatitis C virus (HCV) viroporin p7 is crucial for production of infectious viral progeny. However, its role in the viral replication cycle remains incompletely understood, in part due to the poor availability of p7-specific antibodies. To circumvent this obstacle, we inserted two consecutive hemagglutinin (HA) epitope tags at its N terminus. HA-tagged p7 reduced peak virus titers ca. 10-fold and decreased kinetics of virus production compared to the wild-type virus. However, HA-tagged p7 rescued virus production of a mutant virus lacking p7, thus providing formal proof that the tag does not disrupt p7 function. In HCV-producing cells, p7 displayed a reticular staining pattern which colocalized with the HCV envelope glycoprotein 2 (E2) but also partially with viral nonstructural proteins 2, 3, and 5A. Using coimmunoprecipitation, we confirmed a specific interaction between p7 and NS2, whereas we did not detect a stable interaction with core, E2, or NS5A. Moreover, we did not observe p7 incorporation into affinity-purified virus particles. Consistently, there was no evidence supporting a role of p7 in viral entry, as an anti-HA antibody was not able to neutralize Jc1 virus produced from an HA-p7-tagged genome. Collectively, these findings highlight a stable interaction between p7 and NS2 which is likely crucial for production of infectious HCV particles. Use of this functional epitope-tagged p7 variant should facilitate the analysis of the final steps of the HCV replication cycle.

摘要

丙型肝炎病毒 (HCV) 卷曲螺旋蛋白 p7 对于产生感染性病毒颗粒至关重要。然而,其在病毒复制周期中的作用仍不完全清楚,部分原因是缺乏 p7 特异性抗体。为了克服这一障碍,我们在其 N 端插入了两个连续的血凝素 (HA) 表位标签。与野生型病毒相比,HA 标记的 p7 降低了峰值病毒滴度约 10 倍,并降低了病毒产生的动力学。然而,HA 标记的 p7 拯救了缺乏 p7 的突变病毒的病毒产生,从而提供了正式的证据表明该标签不会破坏 p7 的功能。在产生 HCV 的细胞中,p7 显示出网状染色模式,与 HCV 包膜糖蛋白 2 (E2) 共定位,但也与病毒非结构蛋白 2、3 和 5A 部分共定位。通过共免疫沉淀,我们证实了 p7 与 NS2 之间存在特异性相互作用,而我们没有检测到与核心、E2 或 NS5A 之间的稳定相互作用。此外,我们没有观察到 p7 掺入亲和纯化的病毒颗粒中。一致地,没有证据支持 p7 在病毒进入中的作用,因为抗 HA 抗体不能中和从 HA-p7 标记基因组产生的 Jc1 病毒。总之,这些发现强调了 p7 与 NS2 之间的稳定相互作用,这对于产生感染性 HCV 颗粒可能至关重要。使用这种功能性表位标记的 p7 变体应有助于分析 HCV 复制周期的最后步骤。

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