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首页> 外文期刊>Journal of Molecular Biology >Three-dimensional structure of a monomeric form of a retroviral protease
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Three-dimensional structure of a monomeric form of a retroviral protease

机译:逆转录病毒蛋白酶的单体形式的三维结构

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The assembly of Mason-Pfizer monkey virus Gag polyproteins into immature capsids and their cleavage by the encoded protease are temporally and spatially separated processes, making the virus a particularly useful model for investigation of protease activation. Here we present a high resolution NMR structure of a fully folded monomer of a 12 kDa M-PMV protease (wt 12 PR) and of a Cys7Ala/Asp26Asn/Cys106Ala. mutant (12 PRD26N/C7A/C106A). The overall structures of both wt 12 PR and 12 PRD26N/C7A/C106A follow the conservative structural motif of other retroviral proteases. The most prominent difference from the canonical fold of retroviral proteases is the absence of the interfacial beta-sheet, which leads to the loss of the principal force stabilizing the dimer of M-PMV PR. The monomer-dimer equilibrium can be shifted in favor of the dimer by adding a substrate or an inhibitor, partially compensating for the missing role of the beta-sheet. We also show that cysteines C7 and C106 play a crucial role in stabilizing the dimer and consequently increasing the proteolytic activity of M-PMV PR. This is consistent with the role of reversible oxidative modification of the cysteine residues in the regulation of the maturation of assembled M-PMV capsids in the cytoplasm. (C) 2003 Elsevier Ltd. All rights reserved. [References: 46]
机译:Mason-Pfizer猴病毒Gag多蛋白组装成未成熟的衣壳及其被编码的蛋白酶切割是时间和空间分离的过程,这使该病毒成为研究蛋白酶激活的特别有用的模型。在这里,我们介绍12 kDa M-PMV蛋白酶(wt 12 PR)和Cys7Ala / Asp26Asn / Cys106Ala的完全折叠单体的高分辨率NMR结构。突变体(12 PRD26N / C7A / C106A)。 wt 12 PR和12 PRD26N / C7A / C106A的总体结构均遵循其他逆转录病毒蛋白酶的保守结构基序。与逆转录病毒蛋白酶的标准折叠最显着的区别是界面β-sheet的缺失,这导致稳定M-PMV PR二聚体的主力丧失。通过添加底物或抑制剂,部分补偿β-折叠的缺失作用,可以使单体-二聚体平衡朝着二聚体的方向移动。我们还显示,半胱氨酸C7和C106在稳定二聚体并因此增加M-PMV PR的蛋白水解活性中起关键作用。这与半胱氨酸残基的可逆氧化修饰在调节细胞质中组装的M-PMV衣壳的成熟中的作用是一致的。 (C)2003 Elsevier Ltd.保留所有权利。 [参考:46]

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