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通过定点诱变将一种无活性的原核超氧化物歧化酶同源物转化为活性蛋白。

From an inactive prokaryotic SOD homologue to an active protein through site-directed mutagenesis.

作者信息

Banci Lucia, Benvenuti Manuela, Bertini Ivano, Cabelli Diane E, Calderone Vito, Fantoni Adele, Mangani Stefano, Migliardi Manuele, Viezzoli Maria Silvia

机构信息

Department of Chemistry and Centro Risonanze Magnetiche, University of Florence, 50019 Sesto Fiorentino, Italy.

出版信息

J Am Chem Soc. 2005 Sep 28;127(38):13287-92. doi: 10.1021/ja052790o.

Abstract

It is known that several prokaryotic protein sequences, characterized by high homology with the eukaryotic Cu,ZnSODs, lack some of the metal ligands. In the present work, we have stepwise reintroduced the two missing copper ligands in the SOD-like protein of Bacillus subtilis, through site-directed mutagenesis. The mutant with three out of the four His that bind copper is not active, whereas the fully reconstituted mutant displays an activity of about 10% that of human Cu,ZnSOD. The mutated proteins have been characterized in solution and in the solid state. In solution, the proteins experience conformational disorder, which is believed to be partly responsible for the decreased enzymatic activity and sheds light on the tendency of several human SOD mutants to introduce mobility in the protein frame. In the crystal, on the contrary, the protein has a well-defined conformation, giving rise to dimers through the coordination of an exogenous zinc ion. The catalytic properties of the double mutant, which might be regarded as a step in an artificial evolution from a nonactive SOD to a fully functioning enzyme, are discussed on the basis of the structural and dynamical properties.

摘要

已知几种原核生物蛋白质序列与真核生物铜锌超氧化物歧化酶(Cu,ZnSODs)具有高度同源性,但缺少一些金属配体。在本研究中,我们通过定点诱变逐步在枯草芽孢杆菌的类SOD蛋白中重新引入两个缺失的铜配体。结合铜的四个组氨酸中有三个的突变体没有活性,而完全重构的突变体显示出约为人类Cu,ZnSOD活性10%的活性。已对突变蛋白在溶液和固态下进行了表征。在溶液中,蛋白质经历构象紊乱,这被认为是酶活性降低的部分原因,并揭示了几种人类SOD突变体在蛋白质框架中引入流动性的倾向。相反,在晶体中,蛋白质具有明确的构象,通过外源锌离子的配位形成二聚体。基于结构和动力学性质,讨论了双突变体的催化特性,该双突变体可被视为从无活性SOD到功能完全的酶的人工进化过程中的一步。

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