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尿素诱导蛋白质变性的相干微观图像。

Coherent microscopic picture for urea-induced denaturation of proteins.

机构信息

Department of Engineering Mechanics, and Soft Matter Research Center, Zhejiang University, Hangzhou 310027, China.

出版信息

J Phys Chem B. 2012 Aug 2;116(30):8856-62. doi: 10.1021/jp304114h. Epub 2012 Jul 24.

DOI:10.1021/jp304114h
PMID:22780326
Abstract

In a previous study, we explored the mechanism of urea-induced denaturation of proteins by performing molecular dynamics (MD) simulations of hen lysozyme in 8 M urea and supported the "direct interaction mechanism" whereby urea denatures protein via dispersion interaction (Hua, L.; Zhou, R. H.; Thirumalai, D.; Berne, B. J. Proc. Natl. Acad. Sci. U.S.A. 2008, 105, 16928). Here we perform large scale MD simulations of five representative protein/peptide systems in aqueous urea to investigate if the above mechanism is common to other proteins. In all cases, accumulations of urea around proteins/peptide are observed, suggesting that urea denatures proteins by directly attacking protein backbones and side chains rather than indirectly disrupting water structure as a "water breaker". Consistent with our previous case study of lysozyme, the current energetic analyses with five protein/peptide systems reveal that urea's preferential binding to proteins mainly comes from urea's stronger dispersion interactions with proteins than with bulk solution, whereas the electrostatic (hydrogen-bonded) interactions only play a relatively minor (even negative) role during this denaturation process. Furthermore, the simulations of the peptide system at different urea concentrations (8 and 4.5 M), and with different force fields (CHARMM and OPLSAA) suggest that the above mechanism is robust, independent of the urea concentration and force field used. Last, we emphasize the importance of periodic boundary conditions in pairwise energetic analyses. This article provides a comprehensive study on the physical mechanism of urea-induced protein denaturation and suggests that the "dispersion-interaction-driven" mechanism should be general.

摘要

在之前的研究中,我们通过对 8 M 尿素中的鸡溶菌酶进行分子动力学(MD)模拟,探索了尿素诱导蛋白质变性的机制,并支持了“直接相互作用机制”,即尿素通过分散相互作用(Hua,L.;Zhou,R. H.;Thirumalai,D.;Berne,B. J.Proc. Natl. Acad. Sci. U.S.A. 2008, 105, 16928)使蛋白质变性。在这里,我们对五个具有代表性的蛋白质/肽体系在水合尿素中的大规模 MD 模拟,以研究上述机制是否适用于其他蛋白质。在所有情况下,都观察到尿素在蛋白质/肽周围的积累,这表明尿素通过直接攻击蛋白质骨架和侧链而不是间接破坏水结构作为“水破坏者”使蛋白质变性。与我们之前对溶菌酶的案例研究一致,目前对五个蛋白质/肽体系的能量分析表明,尿素优先与蛋白质结合主要来自于尿素与蛋白质之间更强的分散相互作用,而静电(氢键)相互作用在变性过程中仅起相对较小(甚至负)的作用。此外,在不同尿素浓度(8 和 4.5 M)和不同力场(CHARMM 和 OPLSAA)下对肽体系的模拟表明,上述机制是稳健的,与使用的尿素浓度和力场无关。最后,我们强调在成对能量分析中周期性边界条件的重要性。本文对尿素诱导蛋白质变性的物理机制进行了全面研究,并表明“分散相互作用驱动”机制应该是普遍的。

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Coherent microscopic picture for urea-induced denaturation of proteins.尿素诱导蛋白质变性的相干微观图像。
J Phys Chem B. 2012 Aug 2;116(30):8856-62. doi: 10.1021/jp304114h. Epub 2012 Jul 24.
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