Department of Microbiology and Immunology, University of Texas Medical Branch, Galveston, TX, USA.
J Viral Hepat. 2010 Nov;17(11):784-93. doi: 10.1111/j.1365-2893.2009.01238.x.
Hepatitis C virus (HCV) infection results in several changes in mitochondrial function including increased reactive oxygen species (ROS) production and greater sensitivity to oxidant, Ca(2+) and cytokine-induced cell death. Prior studies in protein over-expression systems have shown that this effect can be induced by the core protein, but other viral proteins and replication events may contribute as well. To evaluate the specific role of core protein in the context of viral replication and infection, we compared mitochondrial sensitivity in Huh7-derived HCV replicon bearing cells with or without core protein expression with that of cells infected with the JFH1 virus strain. JFH1 infection increased hydrogen peroxide production and sensitized cells to oxidant-induced loss of mitochondrial membrane potential and cell death. An identical phenomenon occurred in genome-length replicons-bearing cells but not in cells bearing the subgenomic replicons lacking core protein. Both cell death and mitochondrial depolarization were Ca(2+) dependent and could be prevented by Ca(2+) chelation. The difference in the mitochondrial response of the two replicon systems could be demonstrated even in isolated mitochondria derived from the two cell lines with the 'genome-length' mitochondria displaying greater sensitivity to Ca(2+) -induced cytochrome c release. In vitro incubation of 'subgenomic' mitochondria with core protein increased oxidant sensitivity to a level similar to that of mitochondria derived from cells bearing genome-length replicons. These results indicate that increased mitochondrial ROS production and a reduced threshold for Ca(2+) and ROS-induced permeability transition is a characteristic of HCV infection. This phenomenon is a direct consequence of core protein interactions with mitochondria and is present whenever core is expressed, either in infection, full-length replicon-bearing cells, or in over-expression systems.
丙型肝炎病毒(HCV)感染会导致线粒体功能发生多种变化,包括活性氧(ROS)生成增加以及对氧化剂、Ca2+和细胞因子诱导的细胞死亡更加敏感。在蛋白过表达系统中的先前研究表明,这种效应可以被核心蛋白诱导,但其他病毒蛋白和复制事件也可能有贡献。为了评估核心蛋白在病毒复制和感染背景下的特定作用,我们比较了具有或不具有核心蛋白表达的 Huh7 衍生 HCV 复制子承载细胞与感染 JFH1 病毒株的细胞之间的线粒体敏感性。JFH1 感染增加了过氧化氢的产生,并使细胞对氧化剂诱导的线粒体膜电位丧失和细胞死亡更加敏感。在全长基因组复制子承载细胞中发生了相同的现象,但在缺乏核心蛋白的亚基因组复制子承载细胞中没有发生。细胞死亡和线粒体去极化均依赖于 Ca2+,并且可以通过 Ca2+螯合来预防。即使在从两条细胞系分离的线粒体中也可以证明两种复制子系统的线粒体反应之间的差异,具有“全长”线粒体的线粒体对 Ca2+诱导的细胞色素 c 释放更敏感。在体外孵育“亚基因组”线粒体与核心蛋白可使氧化剂敏感性增加到与源自携带全长复制子的细胞的线粒体相似的水平。这些结果表明,增加的线粒体 ROS 生成和 Ca2+和 ROS 诱导的通透性转换的阈值降低是 HCV 感染的特征。这种现象是核心蛋白与线粒体相互作用的直接后果,只要核心蛋白表达,无论是在感染、全长复制子承载细胞还是在过表达系统中,都会出现这种现象。