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在天然条件下测量膜蛋白稳定性。

Measuring membrane protein stability under native conditions.

机构信息

Department of Chemistry and Biochemistry, UCLA-DOE Institute for Genomics and Proteomics, Molecular Biology Institute, University of California, Los Angeles, CA 90095.

出版信息

Proc Natl Acad Sci U S A. 2014 Jan 7;111(1):219-24. doi: 10.1073/pnas.1318576111. Epub 2013 Dec 23.

Abstract

The thermodynamic stability of proteins is typically measured at high denaturant concentrations and then extrapolated back to zero denaturant conditions to obtain unfolding free energies under native conditions. For membrane proteins, the extrapolations are fraught with considerable uncertainty as the denaturants may have complex effects on the membrane or micellar structure. We therefore sought to measure stability under native conditions, using a method that does not perturb the properties of the membrane or membrane mimetics. We use a technique called steric trapping to measure the thermodynamic stability of bacteriorhodopsin in bicelles and micelles. We find that bacteriorhodopsin has a high thermodynamic stability, with an unfolding free energy of ∼11 kcal/mol in dimyristoyl phosphatidylcholine bicelles. Nevertheless, the stability is much lower than predicted by extrapolation of measurements made at high denaturant concentrations. We investigated the discrepancy and found that unfolding free energy is not linear with denaturant concentration. Apparently, long extrapolations of helical membrane protein unfolding free energies must be treated with caution. Steric trapping, however, provides a method for making these measurements.

摘要

蛋白质的热力学稳定性通常在高变性剂浓度下进行测量,然后外推回零变性剂条件下,以获得在天然条件下的解折叠自由能。对于膜蛋白,外推存在相当大的不确定性,因为变性剂可能对膜或胶束结构产生复杂的影响。因此,我们试图使用不会干扰膜或膜类似物性质的方法在天然条件下测量稳定性。我们使用一种称为空间位阻捕获的技术来测量紫膜在双体和胶束中的热力学稳定性。我们发现,紫膜具有很高的热力学稳定性,在二肉豆蔻酰磷脂酰胆碱双体中,解折叠自由能约为 11kcal/mol。然而,其稳定性远低于高变性剂浓度测量的外推预测值。我们研究了这种差异,发现解折叠自由能与变性剂浓度不是线性关系。显然,对螺旋膜蛋白解折叠自由能的长时间外推必须谨慎处理。然而,空间位阻捕获为进行这些测量提供了一种方法。

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