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纳米盘膜蛋白的超薄层 MALDI 质谱法。

Ultra-thin layer MALDI mass spectrometry of membrane proteins in nanodiscs.

机构信息

Department of Chemistry, University of Illinois Urbana-Champaign, Urbana, IL 61801, USA.

出版信息

Anal Bioanal Chem. 2012 Jan;402(2):721-9. doi: 10.1007/s00216-011-5512-3. Epub 2011 Nov 6.

Abstract

Nanodiscs have become a leading technology to solubilize membrane proteins for biophysical, enzymatic, and structural investigations. Nanodiscs are nanoscale, discoidal lipid bilayers surrounded by an amphipathic membrane scaffold protein (MSP) belt. A variety of analytical tools has been applied to membrane proteins in nanodiscs, including several recent mass spectrometry studies. Mass spectrometry of full-length proteins is an important technique for analyzing protein modifications, for structural studies, and for identification of proteins present in binding assays. However, traditional matrix-assisted laser desorption/ionization-time-of-flight (MALDI-TOF) mass spectrometry methods for analyzing full-length membrane proteins solubilized in nanodiscs are limited by strong signal from the MSP belt and weak signal from the membrane protein inside the nanodisc. Herein, we show that an optimized ultra-thin layer MALDI sample preparation technique dramatically enhances the membrane protein signal and nearly completely eliminates the MSP signal. First-shot MALDI and MALDI imaging are used to characterize the spots formed by the ultra-thin layer method. Furthermore, the membrane protein enhancement and MSP suppression are shown to be independent of the type of membrane protein and are applicable to mixtures of membrane proteins in nanodiscs.

摘要

纳米盘已成为用于生物物理、酶学和结构研究的膜蛋白可溶性的主要技术。纳米盘是由亲脂性膜支架蛋白(MSP)带环绕的纳米级盘状脂质双层。多种分析工具已应用于纳米盘中的膜蛋白,包括最近的一些质谱研究。全长蛋白的质谱分析是分析蛋白修饰、结构研究以及鉴定结合测定中存在的蛋白的重要技术。然而,用于分析溶解在纳米盘中的全长膜蛋白的传统基质辅助激光解吸/电离飞行时间(MALDI-TOF)质谱方法受到 MSP 带的强信号和纳米盘中膜蛋白的弱信号的限制。本文中,我们展示了优化的超薄层 MALDI 样品制备技术可显著增强膜蛋白信号并几乎完全消除 MSP 信号。首次 MALDI 和 MALDI 成像用于表征超薄层方法形成的斑点。此外,证明了膜蛋白增强和 MSP 抑制与膜蛋白的类型无关,并且适用于纳米盘中的膜蛋白混合物。

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