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使用荧光检测尺寸排阻色谱法对膜蛋白进行高通量纳米级表征

High-Throughput Nano-Scale Characterization of Membrane Proteins Using Fluorescence-Detection Size-Exclusion Chromatography.

作者信息

Vecchio Alex J, Stroud Robert M

机构信息

Department of Biochemistry and Biophysics, University of California, San Francisco, San Francisco, CA, USA.

Department of Biochemistry, University of Nebraska-Lincoln, Lincoln, NE, USA.

出版信息

Methods Mol Biol. 2019;2025:361-388. doi: 10.1007/978-1-4939-9624-7_17.

Abstract

Structural biology has revealed predicting heterologous expression levels, homogeneity, and stability of a protein from its primary structure are exceedingly difficult. Membrane proteins, in particular, present numerous challenges that make obtaining milligram quantities of quality samples problematic. For structural and functional investigation of these molecules, however, this is what is required. Fluorescence size-exclusion chromatography (F-SEC), a technique where a protein of biological interest is fused to green fluorescent protein (GFP) and monitored, circumvents many bottlenecks inherent to membrane protein structural biology. In vivo expression yields, as well as in vitro homogeneity and stability, can be rapidly evaluated utilizing nanogram quantities of unpurified protein. In this chapter we describe our most current protocols for expression screening and biochemical characterization of membrane proteins using F-SEC, as it pertains to a high-throughput (HTP) crystallographic pipeline. Therein, the methods and workflow were designed and optimized for structure-function elucidation of eukaryotic integral membrane proteins, but may be applied to prokaryotic or water-soluble proteins with minor modifications, thus making it a useful general approach.

摘要

结构生物学表明,从蛋白质的一级结构预测其异源表达水平、均一性和稳定性极其困难。尤其是膜蛋白,存在诸多挑战,使得获得毫克级质量的样品成为难题。然而,对于这些分子的结构和功能研究而言,这是必需的。荧光尺寸排阻色谱法(F-SEC)是一种将感兴趣的生物蛋白与绿色荧光蛋白(GFP)融合并进行监测的技术,它规避了膜蛋白结构生物学中固有的许多瓶颈。利用纳克级未纯化的蛋白质,可以快速评估体内表达产量以及体外均一性和稳定性。在本章中,我们描述了使用F-SEC进行膜蛋白表达筛选和生化表征的最新方案,这与高通量(HTP)晶体学流程相关。其中,这些方法和工作流程是为阐明真核整合膜蛋白的结构功能而设计和优化的,但经过微小修改后也可应用于原核或水溶性蛋白,因此使其成为一种有用的通用方法。

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