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核糖核酸酶关键残基的基因选择

Genetic selection for critical residues in ribonucleases.

作者信息

Smith Bryan D, Raines Ronald T

机构信息

Department of Biochemistry, University of Wisconsin-Madison, Madison, WI 53706, USA.

出版信息

J Mol Biol. 2006 Sep 22;362(3):459-78. doi: 10.1016/j.jmb.2006.07.020. Epub 2006 Jul 15.

DOI:10.1016/j.jmb.2006.07.020
PMID:16920150
Abstract

Homologous mammalian proteins were subjected to an exhaustive search for residues that are critical to their structure/function. Error-prone polymerase chain reactions were used to generate random mutations in the genes of bovine pancreatic ribonuclease (RNase A) and human angiogenin, and a genetic selection based on the intrinsic cytotoxicity of ribonucleolytic activity was used to isolate inactive variants. Twenty-three of the 124 residues in RNase A were found to be intolerant to substitution with at least one particular amino acid. Twenty-nine of the 123 residues in angiogenin were likewise intolerant. In both RNase A and angiogenin, only six residues appeared to be wholly intolerant to substitution: two histidine residues involved in general acid/base catalysis and four cysteine residues that form two disulfide bonds. With few exceptions, the remaining critical residues were buried in the hydrophobic core of the proteins. Most of these residues were found to tolerate only conservative substitutions. The importance of a particular residue as revealed by this genetic selection correlated with its sequence conservation, though several non-conserved residues were found to be critical for protein structure/function. Despite voluminous research on RNase A, the importance of many residues identified herein was unknown, and those can now serve as targets for future work. Moreover, a comparison of the critical residues in RNase A and human angiogenin, which share only 35% amino acid sequence identity, provides a unique perspective on the molecular evolution of the RNase A superfamily, as well as an impetus for applying this methodology to other ribonucleases.

摘要

对同源哺乳动物蛋白质进行了详尽搜索,以寻找对其结构/功能至关重要的残基。利用易错聚合酶链反应在牛胰核糖核酸酶(RNase A)和人血管生成素的基因中产生随机突变,并基于核糖核酸酶活性的内在细胞毒性进行遗传筛选,以分离无活性变体。发现RNase A的124个残基中有23个对至少一种特定氨基酸的取代不耐受。血管生成素的123个残基中有29个同样不耐受。在RNase A和血管生成素中,只有六个残基似乎完全不耐受取代:两个参与一般酸碱催化的组氨酸残基和四个形成两个二硫键的半胱氨酸残基。除少数例外,其余关键残基都埋藏在蛋白质的疏水核心中。发现这些残基中的大多数仅耐受保守取代。通过这种遗传筛选揭示的特定残基的重要性与其序列保守性相关,尽管发现几个非保守残基对蛋白质结构/功能至关重要。尽管对RNase A进行了大量研究,但本文确定的许多残基的重要性尚不清楚,现在这些残基可作为未来研究的目标。此外,对RNase A和人血管生成素中关键残基的比较,它们的氨基酸序列同一性仅为35%,这为RNase A超家族的分子进化提供了独特的视角,也为将该方法应用于其他核糖核酸酶提供了动力。

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