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病毒诱导的核孔蛋白磷酸化与心肌病毒引起的核运输抑制相关。

Leader-induced phosphorylation of nucleoporins correlates with nuclear trafficking inhibition by cardioviruses.

作者信息

Porter Frederick W, Palmenberg Ann C

机构信息

Institute for Molecular Virology and Department of Biochemistry, University of Wisconsin-Madison, 53706, USA.

出版信息

J Virol. 2009 Feb;83(4):1941-51. doi: 10.1128/JVI.01752-08. Epub 2008 Dec 10.

Abstract

Picornaviruses disrupt nucleocytoplasmic trafficking pathways during infection. Poliovirus and rhinovirus inhibit nuclear protein import/export through a series of 2A protease-dependent cleavages within nuclear pore proteins (nucleoporins [Nups]), including Nup62, Nup98, and Nup153. Cardioviruses lack the same protease and instead affect trafficking inhibition through an activity mapped to their leader (L) protein, a 67- to 76-amino acid (aa) polypeptide with no known enzymatic activity. We have shown that L from encephalomyocarditis virus (EMCV) binds and inhibits the activity of Ran-GTPase, a key regulator of nucleocytoplasmic transport. We now report that recombinant EMCV L triggers the unregulated efflux of protein cargo from preloaded HeLa cell nuclei in cell-free reactions dependent upon Xenopus egg cytosol or HeLa cell-derived cytosol. Recombinant L was the only viral protein necessary for this activity or for nuclear protein import inhibition. Mutational disruption of the L protein zinc finger domain (C(19)A) abrogated the inhibitory activity for both import and efflux in cell extracts, but mutations in the C-terminal acidic domain of L (aa 37 to 61) did not. Notably, HeLa cell nuclei treated with L, or those from EMCV-infected cells, showed reproducibly altered patterns of nucleoporin phosphorylation. Nup62, Nup153, and Nup214 each became hyperphosphorylated in an L-dependent manner. Staurosporine, a broad-spectrum kinase inhibitor, blocked this phosphorylation and rescued nuclear import/export activity from L-dependent inhibition. Therefore, cardioviruses target the same group of nucleoporins as enteroviruses, but the effector mechanism triggered by L (or L-Ran complexes) involves a unique cytosol-dependent phosphorylation cascade rather than proteolysis.

摘要

微小核糖核酸病毒在感染过程中会破坏核质运输途径。脊髓灰质炎病毒和鼻病毒通过对核孔蛋白(核孔素 [Nups])(包括 Nup62、Nup98 和 Nup153)进行一系列 2A 蛋白酶依赖性切割来抑制核蛋白的输入/输出。心病毒缺乏相同的蛋白酶,而是通过定位到其前导(L)蛋白的活性来影响运输抑制,L 蛋白是一种 67 至 76 个氨基酸(aa)的多肽,没有已知的酶活性。我们已经表明,脑心肌炎病毒(EMCV)的 L 蛋白结合并抑制 Ran-GTP 酶的活性,Ran-GTP 酶是核质运输的关键调节因子。我们现在报告,重组 EMCV L 在依赖非洲爪蟾卵母细胞胞质溶胶或 HeLa 细胞来源胞质溶胶的无细胞反应中触发预加载的 HeLa 细胞核中蛋白质货物的不受调控的外流。重组 L 是这种活性或核蛋白输入抑制所必需的唯一病毒蛋白。L 蛋白锌指结构域(C(19)A)的突变破坏消除了细胞提取物中输入和外流的抑制活性,但 L 蛋白 C 末端酸性结构域(氨基酸 37 至 61)的突变则没有。值得注意的是,用 L 处理的 HeLa 细胞核或 EMCV 感染细胞的细胞核显示出核孔素磷酸化模式的可重复改变。Nup62、Nup153 和 Nup214 各自以 L 依赖的方式过度磷酸化。广谱激酶抑制剂星形孢菌素阻断了这种磷酸化,并从 L 依赖的抑制中挽救了核输入/输出活性。因此,心病毒与肠道病毒靶向同一组核孔素,但由 L(或 L-Ran 复合物)触发的效应机制涉及独特的胞质溶胶依赖性磷酸化级联反应而非蛋白水解。

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