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一种用于量化二十面体病毒中准等效性的通用方法。

A general method to quantify quasi-equivalence in icosahedral viruses.

作者信息

Damodaran K V, Reddy Vijay S, Johnson John E, Brooks Charles L

机构信息

Department of Molecular Biology, The Scripps Research Institute, 10550 North Torrey Pines Road, La Jolla, CA 92037, USA.

出版信息

J Mol Biol. 2002 Dec 6;324(4):723-37. doi: 10.1016/s0022-2836(02)01138-5.

DOI:10.1016/s0022-2836(02)01138-5
PMID:12460573
Abstract

A quantitative, atom-based, method is described for comparing protein subunit interfaces in icosahedral virus capsids with quasi-equivalent surface lattices. An integrated, normalized value (between 0 and 1) based on equivalent residue contacts (Q-score) is computed for every pair of subunit interactions and scores that are significantly above zero readily identify interfaces that are quasi-equivalent to each other. The method was applied to all quasi-equivalent capsid structures (T=3, 4, 7 and 13) in the Protein Data Bank and the Q-scores were interpreted in terms of their structural underpinnings. The analysis allowed classification of T=3 structures into three groups with architectures that resemble different polyhedra with icosahedral symmetry. The preference of subunits to form dimers in the T=4 human Hepatitis B virus capsid (HBV) was clearly reflected in high Q-scores of quasi-equivalent dimers. Interesting differences between the classical T=7 capsid and polyoma-like capsids were also identified. Application of the method to the outer-shell of the T=13 Blue tongue virus core (BTVC) highlighted the modest distortion between the interfaces of the general trimers and the strict trimers of VP7 subunits. Furthermore, the method identified the quasi 2-fold symmetry in the inner capsids of the BTV and reovirus cores. The results show that the Q-scores of various quasi-symmetries represent a "fingerprint" for a particular virus capsid architecture allowing particle classification into groups based on their underlying structural and geometric features.

摘要

描述了一种基于原子的定量方法,用于比较二十面体病毒衣壳中具有准等效表面晶格的蛋白质亚基界面。针对每对亚基相互作用计算基于等效残基接触的综合归一化值(介于0和1之间,即Q分数),显著高于零的分数能够轻易识别出彼此准等效的界面。该方法应用于蛋白质数据库中所有准等效衣壳结构(T = 3、4、7和13),并根据其结构基础对Q分数进行了解释。分析将T = 3结构分为三组,其结构类似于具有二十面体对称性的不同多面体。在T = 4人乙型肝炎病毒衣壳(HBV)中,亚基形成二聚体的偏好明显反映在准等效二聚体的高Q分数上。还发现了经典T = 7衣壳与多瘤病毒样衣壳之间有趣的差异。将该方法应用于T = 13蓝舌病毒核心(BTVC)的外壳,突出了一般三聚体与VP7亚基严格三聚体界面之间的适度扭曲。此外,该方法还识别出BTV和呼肠孤病毒核心内壳中的准2倍对称性。结果表明,各种准对称性的Q分数代表了特定病毒衣壳结构的“指纹”,允许根据其潜在的结构和几何特征将病毒颗粒分类成组。

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