蛋白质微图案分析:蛋白质 - 蛋白质相互作用的定量分析
Protein Micropatterning Assay: Quantitative Analysis of Protein-Protein Interactions.
作者信息
Schütz Gerhard J, Weghuber Julian, Lanzerstorfer Peter, Sevcsik Eva
机构信息
Institute of Applied Physics, TU Wien, Getreidemarkt 9, 1060, Vienna, Austria.
School of Engineering and Environmental Sciences, University of Applied Sciences Upper Austria, Stelzhamerstrasse 23, 4600, Wels, Austria.
出版信息
Methods Mol Biol. 2017;1550:261-270. doi: 10.1007/978-1-4939-6747-6_18.
Abstract
Characterization, especially quantification, of protein interactions in live cells is usually not an easy endeavor. Here, we describe a straightforward method to identify and quantify the interaction of a membrane protein ("bait") and a fluorescently labeled interaction partner ("prey") (membrane-bound or cytosolic) in live cells using Total Internal Reflection Fluorescence microscopy. The bait protein is immobilized within patterns in the plasma membrane (e.g., via an antibody); the bait-prey interaction strength can be quantified by determining the prey bulk fluorescence intensity with respect to the bait patterns. This method is particularly suitable also for the analysis of weak, transient interactions that are not easily accessible with other methods.
摘要
对活细胞中蛋白质相互作用进行表征,尤其是定量分析,通常并非易事。在此,我们描述了一种直接的方法,可利用全内反射荧光显微镜在活细胞中鉴定并定量一种膜蛋白(“诱饵”)与一种荧光标记的相互作用伴侣(“猎物”,膜结合型或胞质型)之间的相互作用。诱饵蛋白通过例如抗体固定在质膜的图案内;诱饵 - 猎物相互作用强度可通过测定相对于诱饵图案的猎物整体荧光强度来定量。该方法特别适用于分析其他方法难以检测到的弱的、瞬时相互作用。
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