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α/β桶状蛋白中的簇集:对蛋白质结构、功能和折叠的影响:一种图论方法

Clusters in alpha/beta barrel proteins: implications for protein structure, function, and folding: a graph theoretical approach.

作者信息

Kannan N, Selvaraj S, Gromiha M M, Vishveshwara S

机构信息

Molecular Biophysics Unit, Indian Institute of Science, Bangalore 560 012, India.

出版信息

Proteins. 2001 May 1;43(2):103-12. doi: 10.1002/1097-0134(20010501)43:2<103::aid-prot1022>3.0.co;2-x.

DOI:10.1002/1097-0134(20010501)43:2<103::aid-prot1022>3.0.co;2-x
PMID:11276080
Abstract

The alpha/beta barrel fold is adopted by most enzymes performing a variety of catalytic reactions, but with very low sequence similarity. In order to understand the stabilizing interactions important in maintaining the alpha/beta barrel fold, we have identified residue clusters in a dataset of 36 alpha/beta barrel proteins that have less than 10% sequence identity within themselves. A graph theoretical algorithm is used to identify backbone clusters. This approach uses the global information of the nonbonded interaction in the alpha/beta barrel fold for the clustering procedure. The nonbonded interactions are represented mathematically in the form of an adjacency matrix. On diagonalizing the adjacency matrix, clusters and cluster centers are obtained from the highest eigenvalue and its corresponding vector components. Residue clusters are identified in the strand regions forming the beta barrel and are topologically conserved in all 36 proteins studied. The residues forming the cluster in each of the alpha/beta protein are also conserved among the sequences belonging to the same family. The cluster centers are found to occur in the middle of the strands or in the C-terminal of the strands. In most cases, the residues forming the clusters are part of the active site or are located close to the active site. The folding nucleus of the alpha/beta fold is predicted based on hydrophobicity index evaluation of residues and identification of cluster centers. The predicted nucleation sites are found to occur mostly in the middle of the strands. Proteins 2001;43:103-112.

摘要

大多数执行各种催化反应的酶都采用α/β桶状折叠结构,但它们的序列相似性非常低。为了了解在维持α/β桶状折叠结构中起重要作用的稳定相互作用,我们在一个由36种α/β桶状蛋白质组成的数据集中识别出了残基簇,这些蛋白质自身的序列同一性小于10%。使用一种图论算法来识别主链簇。这种方法在聚类过程中利用了α/β桶状折叠结构中非键相互作用的全局信息。非键相互作用以邻接矩阵的形式进行数学表示。对邻接矩阵进行对角化后,从最高特征值及其相应的向量分量中获得簇和簇中心。在形成β桶的链区域中识别出残基簇,并且在所研究的所有36种蛋白质中这些簇在拓扑结构上是保守的。在每个α/β蛋白质中形成簇的残基在属于同一家族的序列中也是保守的。发现簇中心出现在链的中间或链的C末端。在大多数情况下,形成簇的残基是活性位点的一部分或位于活性位点附近。基于残基的疏水性指数评估和簇中心的识别,预测了α/β折叠的折叠核心。发现预测的成核位点大多出现在链的中间。《蛋白质》2001年;43卷:103 - 112页。

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