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研究盐对核糖核酸酶 t1 模型系统稳定性的影响。

Studying salt effects on protein stability using ribonuclease t1 as a model system.

机构信息

Department of Chemistry, University of Manitoba, Winnipeg, Manitoba, Canada.

出版信息

Biophys Chem. 2012 Feb;161:29-38. doi: 10.1016/j.bpc.2011.11.004. Epub 2011 Dec 2.

DOI:10.1016/j.bpc.2011.11.004
PMID:22197350
Abstract

Salt ions affect protein stability in a variety of ways. In general, these effects have either been interpreted from a charge solvation/charge screening standpoint or they have been considered to be the result of ion-specific interactions with a particular protein. Recent theoretical work suggests that a major contribution to salt effects on proteins is through the interaction of salt ions that are located near the protein surface and their induced point image charges that are located in the low-dielectric protein cavity. These interactions form the basis of "salting-out" interactions. Salt ions induce an image charge of the same sign in the low dielectric protein medium. The interaction between the induced charge and its mirror charge is repulsive and consequently thermodynamically destabilizing. However, a folded protein that has a much smaller surface area will be less destabilized than the unfolded state. Consequently, the folded state will be stabilized relative to the unfolded state. This work analyzes salt effects in the model enzyme ribonuclease t1, and demonstrates that interactions between salt ions and their induced point charges provide a major contribution to the observed salt-induced increase in protein stability. This work also demonstrates that in the case of weakly-binding ions (ions with binding constants that are in the order of 50 M(-1) and less), salting-out effects should still be considered in order to provide a more realistic interpretation of ion binding. These results should therefore be considered when salt effects are used to analyze electrostatic contributions to protein structure or are used to study the thermodynamics of proteins associated with halophillic organisms.

摘要

盐离子以多种方式影响蛋白质的稳定性。一般来说,这些影响要么从电荷溶剂化/电荷屏蔽的角度来解释,要么被认为是与特定蛋白质的离子特异性相互作用的结果。最近的理论工作表明,盐对蛋白质的主要影响之一是通过位于蛋白质表面附近的盐离子与其在低介电常数蛋白质腔中的诱导点电荷之间的相互作用。这些相互作用构成了“盐析”相互作用的基础。盐离子在低介电常数蛋白质介质中诱导相同符号的诱导电荷。诱导电荷与其镜像电荷之间的相互作用是排斥的,因此在热力学上是不稳定的。然而,一个折叠的蛋白质具有较小的表面积,它将比未折叠的状态更稳定。因此,折叠状态相对于未折叠状态将更加稳定。这项工作分析了模型酶核糖核酸酶 t1 中的盐效应,并证明盐离子与其诱导点电荷之间的相互作用对观察到的盐诱导蛋白质稳定性增加有很大贡献。这项工作还表明,对于弱结合离子(结合常数在 50 M(-1)及以下的离子),仍应考虑盐析效应,以便更真实地解释离子结合。因此,在使用盐效应分析蛋白质结构的静电贡献或研究与嗜盐生物相关的蛋白质热力学时,应该考虑这些结果。

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