Chen C M, You L R, Hwang L H, Lee Y H
Institute of Biochemistry, National Yang-Ming University, Taipei, Taiwan, Republic of China.
J Virol. 1997 Dec;71(12):9417-26. doi: 10.1128/JVI.71.12.9417-9426.1997.
Previous studies suggest that the core protein of hepatitis C virus (HCV) has a pleiotropic function in the replication cycle of the virus. To understand the role of this protein in HCV pathogenesis, we used a yeast two-hybrid protein interaction cloning system to search for cellular proteins physically interacting with the HCV core protein. One such cellular gene was isolated and characterized as the gene encoding the lymphotoxin-beta receptor (LT-betaR). In vitro binding analysis demonstrated that the HCV core protein binds to the C-terminal 98 amino acids within the intracellular domain of the LT-betaR that is involved in signal transduction, although the binding affinity of the full-length HCV core protein was weaker than that of its C-terminally truncated form. Our results also indicated that the N-terminal 40-amino-acid segment of the HCV core protein was sufficient for interaction with LT-betaR and that the core protein could form complexes with the oligomeric form of the intracellular domain of LT-betaR, which is a prerequisite for downstream signaling of this receptor. Similar to other members of the tumor necrosis factor (TNF) receptor superfamily, LT-betaR is involved in the cytotoxic effect of the signaling pathway, and thus we have elucidated the biological consequence of interaction between the HCV core protein and LT-betaR. Our results indicated that in the presence of the synergizing agent gamma interferon, the HCV core protein enhances the cytotoxic effects of recombinant forms of LT-betaR ligand in HeLa cells but not in hepatoma cells. Furthermore, this enhancement of the cytolytic activity was cytokine specific, since in the presence of cycloheximide, the expression of the HCV core protein did not elicit an increase in the cytolytic activity of TNF in both HeLa and hepatoma cells. In summary, the HCV core protein can associate with LT-betaR, and this protein-protein interaction has a modulatory effect on the signaling pathway of LT-betaR in certain cell types. Given the known roles of LT-betaR/LT-alpha1,beta2 receptor-ligand interactions in the normal development of peripheral lymphoid organs and in triggering cytolytic activity and NF-kappaB activation in certain cell types, our finding implies that the HCV core protein may aggravate these biological functions of LT-betaR, resulting in pathogenesis in HCV-infected cells.
先前的研究表明,丙型肝炎病毒(HCV)的核心蛋白在病毒复制周期中具有多效性功能。为了解该蛋白在HCV发病机制中的作用,我们使用酵母双杂交蛋白相互作用克隆系统来寻找与HCV核心蛋白发生物理相互作用的细胞蛋白。分离出了一个这样的细胞基因,并将其鉴定为编码淋巴毒素β受体(LT-βR)的基因。体外结合分析表明,HCV核心蛋白与LT-βR细胞内结构域中参与信号转导的C末端98个氨基酸结合,尽管全长HCV核心蛋白的结合亲和力弱于其C末端截短形式。我们的结果还表明,HCV核心蛋白的N末端40个氨基酸片段足以与LT-βR相互作用,并且核心蛋白可以与LT-βR细胞内结构域的寡聚形式形成复合物,这是该受体下游信号传导的先决条件。与肿瘤坏死因子(TNF)受体超家族的其他成员类似,LT-βR参与信号通路的细胞毒性作用,因此我们阐明了HCV核心蛋白与LT-βR之间相互作用的生物学后果。我们的结果表明,在协同剂γ干扰素存在的情况下,HCV核心蛋白增强了重组形式的LT-βR配体在HeLa细胞中的细胞毒性作用,但在肝癌细胞中未增强。此外,这种溶细胞活性的增强具有细胞因子特异性,因为在放线菌酮存在的情况下,HCV核心蛋白的表达并未引起HeLa细胞和肝癌细胞中TNF溶细胞活性的增加。总之,HCV核心蛋白可以与LT-βR结合,并且这种蛋白质-蛋白质相互作用在某些细胞类型中对LT-βR的信号通路具有调节作用。鉴于LT-βR/LT-α1,β2受体-配体相互作用在周围淋巴器官的正常发育以及在某些细胞类型中触发溶细胞活性和NF-κB激活方面的已知作用,我们的发现意味着HCV核心蛋白可能会加重LT-βR的这些生物学功能,从而导致HCV感染细胞中的发病机制。
