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乳头瘤病毒组装与拆卸过程中的衣壳间二硫键

Intercapsomeric disulfide bonds in papillomavirus assembly and disassembly.

作者信息

Li M, Beard P, Estes P A, Lyon M K, Garcea R L

机构信息

Department of Pediatrics, University of Colorado School of Medicine, Denver 80262, USA.

出版信息

J Virol. 1998 Mar;72(3):2160-7. doi: 10.1128/JVI.72.3.2160-2167.1998.

Abstract

In order to analyze bonding contacts that stabilize the virion or promote capsid assembly, bovine papillomavirus (BPV) virions were subjected to buffer conditions known to disrupt polyomavirus virions. At physiologic ionic strength, incubation with dithiothreitol (DTT), EGTA, or DTT plus EGTA did not disrupt BPV virions as determined by electron microscopy. However, incubation of virions with DTT rendered the BPV L1 protein susceptible to trypsin cleavage at its carboxy terminus and rendered the genome susceptible to digestion with DNase I. When DTT-treated BPV virions were analyzed by analytical ultracentrifugation, they sedimented at 230S compared with 273S for untreated virions, suggesting a capsid shell expansion. Incubation with EGTA had no effect on trypsin or DNase I sensitivity and only a small effect upon the virion S value. A single cysteine residue conserved among BPV and human papillomavirus (HPV) L1 proteins resides within the trypsin-sensitive carboxy terminus of L1, which is required for capsid assembly. A recombinant HPV type 11 L1 protein, which was purified after expression in Escherichia coli and which has a Cys-to-Gly change at this position (Cys424), formed pentamers; however, unlike the wild-type protein, these mutant pentamers could no longer assemble in vitro into capsid-like structures. These results indicate an important role for interpentamer disulfide bonds in papillomavirus capsid assembly and disassembly and suggest a mechanism of virus uncoating in the reducing environment of the cytoplasm.

摘要

为了分析稳定病毒体或促进衣壳组装的结合接触,牛乳头瘤病毒(BPV)病毒体被置于已知会破坏多瘤病毒病毒体的缓冲条件下。在生理离子强度下,通过电子显微镜观察发现,用二硫苏糖醇(DTT)、乙二醇双四乙酸(EGTA)或DTT加EGTA孵育并不会破坏BPV病毒体。然而,用DTT孵育病毒体后,BPV L1蛋白在其羧基末端变得易被胰蛋白酶切割,并且基因组也易被脱氧核糖核酸酶I消化。当通过分析超速离心法分析经DTT处理的BPV病毒体时,它们的沉降系数为230S,而未处理的病毒体为273S,这表明衣壳壳发生了扩张。用EGTA孵育对胰蛋白酶或脱氧核糖核酸酶I的敏感性没有影响,对病毒体的沉降系数只有很小的影响。在BPV和人乳头瘤病毒(HPV)的L1蛋白中保守的一个半胱氨酸残基位于L1的胰蛋白酶敏感羧基末端内,这是衣壳组装所必需的。一种重组的11型HPV L1蛋白,在大肠杆菌中表达后纯化,在这个位置(Cys424)有一个从半胱氨酸到甘氨酸的变化,它形成了五聚体;然而,与野生型蛋白不同的是,这些突变五聚体在体外不再能组装成衣壳样结构。这些结果表明五聚体间二硫键在乳头瘤病毒衣壳组装和解组装中起重要作用,并提示了在细胞质还原环境中病毒脱壳的机制。

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