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LCP-Tm:一种用于测量和了解膜环境中膜蛋白稳定性的分析方法。

LCP-Tm: an assay to measure and understand stability of membrane proteins in a membrane environment.

机构信息

Department of Molecular Biology, The Scripps Research Institute, La Jolla, California, USA.

出版信息

Biophys J. 2010 Apr 21;98(8):1539-48. doi: 10.1016/j.bpj.2009.12.4296.

Abstract

Structural and functional studies of membrane proteins are limited by their poor stability outside the native membrane environment. The development of novel methods to efficiently stabilize membrane proteins immediately after purification is important for biophysical studies, and is likely to be critical for studying the more challenging human targets. Lipidic cubic phase (LCP) provides a suitable stabilizing matrix for studying membrane proteins by spectroscopic and other biophysical techniques, including obtaining highly ordered membrane protein crystals for structural studies. We have developed a robust and accurate assay, LCP-Tm, for measuring the thermal stability of membrane proteins embedded in an LCP matrix. In its two implementations, protein denaturation is followed either by a change in the intrinsic protein fluorescence on ligand release, or by an increase in the fluorescence of a thiol-binding reporter dye that measures exposure of cysteines buried in the native structure. Application of the LCP-Tm assay to an engineered human beta2-adrenergic receptor and bacteriorhodopsin revealed a number of factors that increased protein stability in LCP. This assay has the potential to guide protein engineering efforts and identify stabilizing conditions that may improve the chances of obtaining high-resolution structures of intrinsically unstable membrane proteins.

摘要

膜蛋白的结构和功能研究受到其在天然膜环境之外的稳定性差的限制。开发在纯化后立即有效稳定膜蛋白的新方法对于生物物理研究很重要,对于研究更具挑战性的人类靶标可能至关重要。脂质立方相 (LCP) 为通过光谱和其他生物物理技术研究膜蛋白提供了合适的稳定基质,包括获得用于结构研究的高度有序的膜蛋白晶体。我们已经开发了一种稳健且准确的测定法,即 LCP-Tm,用于测量嵌入 LCP 基质中的膜蛋白的热稳定性。在其两种实施方式中,要么通过配体释放时内在蛋白荧光的变化,要么通过测量埋藏在天然结构中的半胱氨酸暴露的硫醇结合报告染料的荧光增加来跟踪蛋白质变性。将 LCP-Tm 测定法应用于工程化的人β2-肾上腺素能受体和菌紫质揭示了许多可提高 LCP 中蛋白质稳定性的因素。该测定法有可能指导蛋白质工程努力并确定稳定条件,这可能会增加获得内在不稳定膜蛋白高分辨率结构的机会。

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