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肠道病毒 71 依赖 RNA 的 RNA 聚合酶与其蛋白引物 VPg 复合物的晶体结构:VPg 尿苷酰化的转译机制研究。

Crystal structure of enterovirus 71 RNA-dependent RNA polymerase complexed with its protein primer VPg: implication for a trans mechanism of VPg uridylylation.

机构信息

Structural Biology Laboratory and MOE Laboratory of Protein Science, School of Medicine and Life Science, Tsinghua University, Beijing, China.

出版信息

J Virol. 2013 May;87(10):5755-68. doi: 10.1128/JVI.02733-12. Epub 2013 Mar 13.

DOI:10.1128/JVI.02733-12
PMID:23487447
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3648134/
Abstract

Picornavirus RNA replication is initiated by VPg uridylylation, during which the hydroxyl group of the third tyrosine residue of the virally encoded protein VPg is covalently linked to two UMP molecules by RNA-dependent RNA polymerase (RdRp; also known as 3D(pol)). We previously identified site 311, located at the base of the palm domain of the enterovirus 71 (EV71) RdRp, to be the site for EV71 VPg binding and uridylylation. Here we report the crystal structure of EV71 3D(pol) complexed with VPg. VPg was anchored at the bottom of the palm domain of the 3D(pol) molecule and exhibited an extended V-shape conformation. The corresponding interface on 3D(pol) was mainly formed by residues within site 311 and other residues in the palm and finger domains. Mutations of the amino acids of 3D(pol) involved in the VPg interaction (3DL319A, 3DD320A, and 3DY335A) significantly disrupted VPg binding to 3D(pol), resulting in defective VPg uridylylation. In contrast, these mutations did not affect the RNA elongation activity of 3D(pol). In the context of viral genomic RNA, mutations that abolished VPg uridylylation activity were lethal for EV71 replication. Further in vitro analysis showed that the uridylylation activity was restored by mixing VPg-binding-defective and catalysis-defective mutants, indicating a trans mechanism for EV71 VPg uridylylation. Our results, together with previous results of other studies, demonstrate that different picornaviruses use distinct binding sites for VPg uridylylation.

摘要

小核糖核酸病毒的 RNA 复制是由 VPg 尿苷酰化启动的,在此过程中病毒编码蛋白 VPg 的第三个酪氨酸残基的羟基通过 RNA 依赖性 RNA 聚合酶(RdRp;也称为 3D(pol))与两个 UMP 分子共价连接。我们之前确定位于肠道病毒 71(EV71)RdRp 棕榈域底部的 311 位是 EV71 VPg 结合和尿苷酰化的位点。在这里,我们报告了 EV71 3D(pol)与 VPg 复合物的晶体结构。VPg 锚定在 3D(pol)分子的棕榈域底部,呈现出伸展的 V 形构象。3D(pol)上相应的界面主要由位于 311 位的残基和棕榈域和手指域中的其他残基形成。涉及 VPg 相互作用的 3D(pol)氨基酸突变(3DL319A、3DD320A 和 3DY335A)显著破坏了 VPg 与 3D(pol)的结合,导致 VPg 尿苷酰化缺陷。相比之下,这些突变并不影响 3D(pol)的 RNA 延伸活性。在病毒基因组 RNA 的背景下,消除 VPg 尿苷酰化活性的突变对 EV71 复制是致命的。进一步的体外分析表明,VPg 结合缺陷和催化缺陷突变体的混合可恢复尿苷酰化活性,表明 EV71 VPg 尿苷酰化是一种转位机制。我们的结果与其他研究的先前结果一起表明,不同的小核糖核酸病毒使用不同的 VPg 尿苷酰化结合位点。

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Crystal structure of enterovirus 71 RNA-dependent RNA polymerase complexed with its protein primer VPg: implication for a trans mechanism of VPg uridylylation.肠道病毒 71 依赖 RNA 的 RNA 聚合酶与其蛋白引物 VPg 复合物的晶体结构:VPg 尿苷酰化的转译机制研究。
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