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荧光光谱法在pH依赖性膜蛋白插入的热力学和动力学分析中的应用

Fluorescence spectroscopy in thermodynamic and kinetic analysis of pH-dependent membrane protein insertion.

作者信息

Ladokhin Alexey S

机构信息

Department of Biochemistry and Molecular Biology, University of Kansas Medical Center, Kansas City, Kansas, USA.

出版信息

Methods Enzymol. 2009;466:19-42. doi: 10.1016/S0076-6879(09)66002-X. Epub 2009 Nov 13.

Abstract

Experimental determination of the free energy stabilizing the structure of membrane proteins in their native lipid environment is undermined by a lack of appropriate methods and suitable model systems. Here, we demonstrate how fluorescence correlation spectroscopy can be used to characterize thermodynamics of pH-triggered bilayer insertion of nonconstitutive membrane proteins (e.g., bacterial toxins, colicins). The experimental design is guided by the appropriate thermodynamic scheme which considers two independent processes: pH-dependent formation of a membrane-competent form and its insertion into the lipid bilayer. Measurements of a model protein annexin B12 under conditions of lipid saturation demonstrate that protonation leading to the formation of the membrane-competent state occurs near membrane interface. Lipid titration experiments demonstrate that the free energy of transfer to the intermediate interfacial state is especially favorable, while the free energy of final insertion is modulated by interplay of hydrophobic and electrostatic interactions on the bilayer interface. The general principles of kinetic measurements along the insertion pathway containing interfacial intermediate are discussed and practical examples emphasizing appropriate fitting and normalization procedures are presented.

摘要

由于缺乏合适的方法和适用的模型系统,在天然脂质环境中稳定膜蛋白结构的自由能的实验测定受到了阻碍。在此,我们展示了如何利用荧光相关光谱来表征非组成型膜蛋白(如细菌毒素、大肠杆菌素)pH触发的双层插入的热力学。实验设计以适当的热力学方案为指导,该方案考虑了两个独立的过程:pH依赖的膜活性形式的形成及其插入脂质双层。在脂质饱和条件下对模型蛋白膜联蛋白B12的测量表明,导致形成膜活性状态的质子化发生在膜界面附近。脂质滴定实验表明,转移到中间界面状态的自由能特别有利,而最终插入的自由能则由双层界面上疏水和静电相互作用的相互作用调节。讨论了沿着包含界面中间体的插入途径进行动力学测量的一般原则,并给出了强调适当拟合和归一化程序的实际例子。

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