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一种环曲病毒主要蛋白酶的特性分析

Characterization of a torovirus main proteinase.

作者信息

Smits Saskia L, Snijder Eric J, de Groot Raoul J

机构信息

Virology Division, Department of Infectious Diseases and Immunology, Faculty of Veterinary Medicine, Utrecht University, 3584 CL Utrecht, The Netherlands.

出版信息

J Virol. 2006 Apr;80(8):4157-67. doi: 10.1128/JVI.80.8.4157-4167.2006.

Abstract

Viruses of the order Nidovirales encode huge replicase polyproteins. These are processed primarily by the chymotrypsin-like main proteinases (M(pro)s). So far, M(pro)s have been studied only for corona-, arteri-, and roniviruses. Here, we report the characterization of the M(pro) of toroviruses, the fourth main Nidovirus branch. Comparative sequence analysis of polyprotein 1a of equine torovirus (EToV) strain Berne, identified a serine proteinase domain, flanked by hydrophobic regions. Heterologous expression of this domain resulted in autoprocessing at flanking cleavage sites. N-terminal sequence analysis of cleavage products tentatively identified FxxQ downward arrow(S, A) as the substrate consensus sequence. EToV M(pro) combines several traits of its closest relatives. It has a predicted three-domain structure, with two catalytic beta-barrel domains and an additional C-terminal domain of unknown function. With respect to substrate specificity, the EToV M(pro) resembles its coronavirus homologue in its preference for P1-Gln, but its substrate-binding subsite, S1, more closely resembles that of arteri- and ronivirus M(pro)s, which prefer P1-Glu. Surprisingly, in contrast to the M(pro)s of corona- and roniviruses, but like that of arterivirus, the torovirus M(pro) uses serine instead of cysteine as its principal nucleophile. Under the premise that the M(pro)s of corona- and toroviruses are more closely related to each other than to those of arteri- and roniviruses, the transition from serine- to cysteine-based proteolytic catalysis (or vice versa) must have happened more than once in the course of nidovirus evolution. In this respect, it is of interest that a mutant EToV M(pro) with a Ser165-->Cys substitution retained partial enzymatic activity.

摘要

尼多病毒目病毒编码巨大的复制酶多聚蛋白。这些多聚蛋白主要由类胰凝乳蛋白酶样的主要蛋白酶(M蛋白酶)进行加工处理。到目前为止,仅针对冠状病毒、动脉炎病毒和轮状病毒的M蛋白酶进行了研究。在此,我们报告了尼多病毒第四个主要分支——环曲病毒M蛋白酶的特性。对马环曲病毒(EToV)伯尔尼毒株多聚蛋白1a进行的比较序列分析,确定了一个丝氨酸蛋白酶结构域,两侧为疏水区域。该结构域的异源表达导致在侧翼切割位点处进行自我加工。切割产物的N端序列分析初步确定FxxQ↓(S,A)为底物共有序列。EToV M蛋白酶兼具其近亲的多种特征。它具有预测的三结构域结构,有两个催化β桶结构域和一个功能未知的额外C端结构域。在底物特异性方面,EToV M蛋白酶在对P1-Gln的偏好上类似于其冠状病毒同源物,但其底物结合亚位点S1更类似于动脉炎病毒和轮状病毒的M蛋白酶,后者偏好P1-Glu。令人惊讶的是,与冠状病毒和轮状病毒的M蛋白酶不同,但与动脉炎病毒的M蛋白酶一样,环曲病毒M蛋白酶使用丝氨酸而非半胱氨酸作为其主要亲核试剂。在冠状病毒和环曲病毒的M蛋白酶彼此之间比与动脉炎病毒和轮状病毒的M蛋白酶更密切相关的前提下,从基于丝氨酸到基于半胱氨酸的蛋白水解催化的转变(或反之亦然)在尼多病毒进化过程中肯定发生了不止一次。在这方面,有趣的是,具有Ser165→Cys取代的突变型EToV M蛋白酶保留了部分酶活性。

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