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利用双突变循环评估工程化表面静电相互作用对蛋白质稳定性的贡献。

Estimating the contribution of engineered surface electrostatic interactions to protein stability by using double-mutant cycles.

作者信息

Serrano L, Horovitz A, Avron B, Bycroft M, Fersht A R

机构信息

MRC Unit for Protein Function and Design, University Chemical Laboratory, Cambridge, U.K.

出版信息

Biochemistry. 1990 Oct 9;29(40):9343-52. doi: 10.1021/bi00492a006.

DOI:10.1021/bi00492a006
PMID:2248951
Abstract

Coulombic interactions between charges on the surface of proteins contribute to stability. It is difficult, however, to estimate their importance by protein engineering methods because mutation of one residue in an ion pair alters the energetics of many interactions in addition to the coulombic energy between the two components. We have estimated the interaction energy between two charged residues, Asp-12 and Arg-16, in an alpha-helix on the surface of a barnase mutant by invoking a double-mutant cycle involving wild-type enzyme (Asp-12, Thr-16), the single mutants Thr----Arg-16 and Asp----Ala-12, and the double mutant Asp----Ala-12, Thr----Arg-16. The changes in free energy of unfolding of the single mutants are not additive because of the coulombic interaction energy. Additivity is restored at high concentrations of salt that shield electrostatic interactions. The geometry of the ion pair in the mutant was assumed to be the same as that in the highly homologous ribonuclease from Bacillus intermedius, binase, which has Asp-12 and Arg-16 in the native enzyme. The ion pair does not form a hydrogen-bonded salt bridge, but the charges are separated by 5-6 A. The mutant barnase containing the ion pair Asp-12/Arg-16 is more stable than wild type by 0.5 kcal/mol, but only a part of the increased stability is attributable to the electrostatic interaction. We present a formal analysis of how double-mutant cycles can be used to measure the energetics of pairwise interactions.

摘要

蛋白质表面电荷之间的库仑相互作用有助于蛋白质的稳定性。然而,通过蛋白质工程方法很难评估它们的重要性,因为离子对中一个残基的突变除了改变两个组分之间的库仑能外,还会改变许多相互作用的能量。我们通过构建一个涉及野生型酶(Asp-12,Thr-16)、单突变体Thr→Arg-16和Asp→Ala-12以及双突变体Asp→Ala-12,Thr→Arg-16的双突变循环,估算了巴那斯酶突变体表面α螺旋中两个带电残基Asp-12和Arg-16之间的相互作用能。由于库仑相互作用能,单突变体去折叠自由能的变化不是可加的。在屏蔽静电相互作用的高盐浓度下,可加性得以恢复。假设突变体中离子对的几何结构与来自中间芽孢杆菌的高度同源核糖核酸酶binase中的相同,binase在天然酶中具有Asp-12和Arg-16。该离子对不形成氢键盐桥,但电荷之间相距5-6埃。含有离子对Asp-12/Arg-16的突变型巴那斯酶比野生型稳定0.5千卡/摩尔,但增加的稳定性只有一部分可归因于静电相互作用。我们对如何利用双突变循环来测量成对相互作用的能量进行了形式化分析。

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