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丙型肝炎病毒结构蛋白在高效复制该病毒的细胞培养系统中的亚细胞定位。

Subcellular localization of hepatitis C virus structural proteins in a cell culture system that efficiently replicates the virus.

作者信息

Rouillé Yves, Helle François, Delgrange David, Roingeard Philippe, Voisset Cécile, Blanchard Emmanuelle, Belouzard Sandrine, McKeating Jane, Patel Arvind H, Maertens Geert, Wakita Takaji, Wychowski Czeslaw, Dubuisson Jean

机构信息

CNRS-UPR2511, Institut de Biologie de Lille, 1 Rue Calmette, BP447, 59021 Lille Cedex, France.

出版信息

J Virol. 2006 Mar;80(6):2832-41. doi: 10.1128/JVI.80.6.2832-2841.2006.

Abstract

Due to the recent development of a cell culture model, hepatitis C virus (HCV) can be efficiently propagated in cell culture. This allowed us to reinvestigate the subcellular localization of HCV structural proteins in the context of an infectious cycle. In agreement with previous reports, confocal immunofluorescence analysis of the subcellular localization of HCV structural proteins indicated that, in infected cells, the glycoprotein heterodimer is retained in the endoplasmic reticulum. However, in contrast to other studies, the glycoprotein heterodimer did not accumulate in other intracellular compartments or at the plasma membrane. As previously reported, an association between the capsid protein and lipid droplets was also observed. In addition, a fraction of labeling was consistent with the capsid protein being localized in a membranous compartment that is associated with the lipid droplets. However, in contrast to previous reports, the capsid protein was not found in the nucleus or in association with mitochondria or other well-defined intracellular compartments. Surprisingly, no colocalization was observed between the glycoprotein heterodimer and the capsid protein in infected cells. Electron microscopy analyses allowed us to identify a membrane alteration similar to the previously reported "membranous web." However, no virus-like particles were found in this type of structure. In addition, dense elements compatible with the size and shape of a viral particle were seldom observed in infected cells. In conclusion, the cell culture system for HCV allowed us for the first time to characterize the subcellular localization of HCV structural proteins in the context an infectious cycle.

摘要

由于最近细胞培养模型的发展,丙型肝炎病毒(HCV)能够在细胞培养中高效繁殖。这使我们能够在感染周期的背景下重新研究HCV结构蛋白的亚细胞定位。与之前的报道一致,对HCV结构蛋白亚细胞定位的共聚焦免疫荧光分析表明,在受感染的细胞中,糖蛋白异二聚体保留在内质网中。然而,与其他研究不同的是,糖蛋白异二聚体没有在其他细胞内区室或质膜上积累。如先前报道的那样,衣壳蛋白与脂滴之间的关联也被观察到。此外,一部分标记与衣壳蛋白定位于与脂滴相关的膜性区室一致。然而,与之前的报道不同的是,衣壳蛋白未在细胞核中发现,也未与线粒体或其他明确的细胞内区室相关联。令人惊讶的是,在受感染的细胞中未观察到糖蛋白异二聚体与衣壳蛋白之间的共定位。电子显微镜分析使我们能够识别出一种类似于先前报道的“膜性网络”的膜改变。然而,在这种结构中未发现病毒样颗粒。此外,在受感染的细胞中很少观察到与病毒颗粒大小和形状相符的致密元件。总之,HCV细胞培养系统首次使我们能够在感染周期的背景下表征HCV结构蛋白的亚细胞定位。

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