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体积排阻和软相互作用对拥挤环境下蛋白质稳定性的影响。

Volume exclusion and soft interaction effects on protein stability under crowded conditions.

机构信息

Department of Chemistry, University of North Carolina, Chapel Hill, North Carolina 27599, USA.

出版信息

Biochemistry. 2010 Aug 24;49(33):6984-91. doi: 10.1021/bi100727y.

Abstract

Most proteins function in nature under crowded conditions, and crowding can change protein properties. Quantification of crowding effects, however, is difficult because solutions containing hundreds of grams of macromolecules per liter often interfere with the observation of the protein being studied. Models for macromolecular crowding tend to focus on the steric effects of crowders, neglecting potential chemical interactions between the crowder and the test protein. Here, we report the first systematic, quantitative, residue-level study of crowding effects on the equilibrium stability of a globular protein. We used a system comprising poly(vinylpyrrolidone)s (PVPs) of varying molecular weights as crowding agents and chymotrypsin inhibitor 2 (CI2) as a small globular test protein. Stability was quantified with NMR-detected amide (1)H exchange. We analyzed the data in terms of hard particle exclusion, confinement, and soft interactions. For all crowded conditions, nearly every observed residue experiences a stabilizing effect. The exceptions are residues for which stabilities are unchanged. At a PVP concentration of 100 g/L, the data are consistent with theories of hard particle exclusion. At higher concentrations, the data are more consistent with confinement. The data show that the crowder also stabilizes the test protein by weakly binding its native state. We conclude that the role of native-state binding and other soft interactions needs to be seriously considered when applying both theory and experiment to studies of macromolecular crowding.

摘要

大多数蛋白质在自然环境下都是在拥挤的条件下发挥功能的,而拥挤会改变蛋白质的性质。然而,拥挤效应的量化是困难的,因为每升含有数百克大分子的溶液通常会干扰正在研究的蛋白质的观察。大分子拥挤的模型往往侧重于拥挤剂的空间位阻效应,而忽略了拥挤剂与测试蛋白之间可能存在的化学相互作用。在这里,我们报告了第一个关于拥挤效应对球形蛋白质平衡稳定性的系统、定量、残基水平研究。我们使用了由不同分子量的聚乙烯吡咯烷酮(PVP)组成的系统作为拥挤剂,胰凝乳蛋白酶抑制剂 2(CI2)作为一个小的球形测试蛋白。稳定性通过 NMR 检测酰胺(1)H 交换来定量。我们根据硬粒子排斥、限制和软相互作用来分析数据。对于所有拥挤的条件,几乎每个观察到的残基都经历了稳定作用。例外是那些稳定性不变的残基。在 100 g/L 的 PVP 浓度下,数据与硬粒子排斥理论一致。在更高的浓度下,数据更符合限制理论。数据表明,拥挤剂还通过弱结合其天然状态来稳定测试蛋白。我们得出结论,在将理论和实验应用于大分子拥挤研究时,需要认真考虑天然状态结合和其他软相互作用的作用。

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