干扰素调节的抗病毒蛋白PKR和RNase L参与呼肠孤病毒诱导的细胞翻译关闭。
Involvement of the interferon-regulated antiviral proteins PKR and RNase L in reovirus-induced shutoff of cellular translation.
作者信息
Smith Jennifer A, Schmechel Stephen C, Williams Bryan R G, Silverman Robert H, Schiff Leslie A
机构信息
Department of Microbiology, University of Minnesota, 420 Delaware St., Minneapolis, MN 55455, USA.
出版信息
J Virol. 2005 Feb;79(4):2240-50. doi: 10.1128/JVI.79.4.2240-2250.2005.
Cellular translation is inhibited following infection with most strains of reovirus, but the mechanisms responsible for this phenomenon remain to be elucidated. The extent of host shutoff varies in a strain-dependent manner; infection with the majority of strains leads to strong host shutoff, while infection with strain Dearing results in minimal inhibition of cellular translation. A genetic study with reassortant viruses and subsequent biochemical analyses led to the hypothesis that the interferon-induced, double-stranded RNA-activated protein kinase, PKR, is responsible for reovirus-induced host shutoff. To directly determine whether PKR is responsible for reovirus-induced host shutoff, we used a panel of reovirus strains and mouse embryo fibroblasts derived from knockout mice. This approach revealed that PKR contributes to but is not wholly responsible for reovirus-induced host shutoff. Studies with cells lacking RNase L, the endoribonuclease component of the interferon-regulated 2',5'-oligoadenylate synthetase-RNase L system, demonstrated that RNase L also down-regulates cellular protein synthesis in reovirus-infected cells. In many viral systems, PKR and RNase L have well-characterized antiviral functions. An analysis of reovirus replication in cells lacking these molecules indicated that, while they contributed to host shutoff, neither PKR nor RNase L exerted an antiviral effect on reovirus growth. In fact, some strains of reovirus replicated more efficiently in the presence of PKR and RNase L than in their absence. Data presented in this report illustrate that the inhibition of cellular translation following reovirus infection is complex and involves multiple interferon-regulated gene products. In addition, our results suggest that reovirus has evolved effective mechanisms to avoid the actions of the interferon-stimulated antiviral pathways that include PKR and RNase L and may even benefit from their expression.
感染大多数呼肠孤病毒株后,细胞翻译会受到抑制,但导致这种现象的机制仍有待阐明。宿主关闭的程度因毒株而异;大多数毒株感染会导致强烈的宿主关闭,而狄氏毒株感染对细胞翻译的抑制作用最小。一项对重配病毒的遗传学研究及后续生化分析提出了一个假说,即干扰素诱导的双链RNA激活蛋白激酶PKR是呼肠孤病毒诱导宿主关闭的原因。为了直接确定PKR是否是呼肠孤病毒诱导宿主关闭的原因,我们使用了一组呼肠孤病毒株和来自基因敲除小鼠的小鼠胚胎成纤维细胞。这种方法表明,PKR对呼肠孤病毒诱导的宿主关闭有作用,但并非完全负责。对缺乏RNase L(干扰素调节的2',5'-寡腺苷酸合成酶-RNase L系统的核糖核酸内切酶成分)的细胞进行的研究表明,RNase L也会下调呼肠孤病毒感染细胞中的细胞蛋白质合成。在许多病毒系统中,PKR和RNase L具有明确的抗病毒功能。对缺乏这些分子的细胞中呼肠孤病毒复制的分析表明,虽然它们对宿主关闭有作用,但PKR和RNase L对呼肠孤病毒的生长均未发挥抗病毒作用。事实上,一些呼肠孤病毒株在有PKR和RNase L存在时比没有时复制得更有效。本报告中的数据表明,呼肠孤病毒感染后细胞翻译的抑制是复杂的,涉及多种干扰素调节的基因产物。此外,我们的结果表明,呼肠孤病毒已经进化出有效的机制来避免包括PKR和RNase L在内的干扰素刺激的抗病毒途径的作用,甚至可能从它们的表达中受益。
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