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用于以高通量筛选(HTS)形式定量蛋白质-蛋白质相互作用的荧光偏振分析。

Fluorescence polarization assay to quantify protein-protein interactions in an HTS format.

作者信息

Du Yuhong

机构信息

Department of Pharmacology, Emory Chemical Biology Discovery Center, Emory University School of Medicine, 1510 Clifton Road, Atlanta, GA, 30322, USA,

出版信息

Methods Mol Biol. 2015;1278:529-44. doi: 10.1007/978-1-4939-2425-7_35.

Abstract

Fluorescence polarization (FP) technology is based on the measurement of molecule rotation, and has been widely used to study molecular interactions in solution. This method can be used to measure binding and dissociation between two molecules if one of the binding molecules is relatively small and fluorescent. The fluorescently labeled small molecule (such as a small peptide) rotates rapidly in the solution. Upon excitation by polarized light, the emitted light remains depolarized and gives rise to a low FP signal. When the fluorescent small molecules in solution are bound to bigger molecules (such as a protein), the movement of the complex becomes slower. When such a complex is excited with polarized light, much of the emitted light is polarized because of the slow movement of the complex. Thus, the binding of a fluorescently labeled small molecule to a bigger molecule can be monitored by the change in polarization and measured by the generation of an increased FP signal. This chapter aims to provide a step-by-step practical procedure for developing an FP assay in a multi-well plate format to monitor protein-protein interaction (PPI) in a homogenous format.

摘要

荧光偏振(FP)技术基于对分子旋转的测量,已被广泛用于研究溶液中的分子相互作用。如果其中一个结合分子相对较小且具有荧光性,该方法可用于测量两个分子之间的结合和解离。荧光标记的小分子(如小肽)在溶液中快速旋转。在偏振光激发下,发射光保持去偏振状态,并产生低FP信号。当溶液中的荧光小分子与较大分子(如蛋白质)结合时,复合物的运动变得更慢。当用偏振光激发这样的复合物时,由于复合物运动缓慢,大部分发射光会发生偏振。因此,荧光标记的小分子与较大分子的结合可以通过偏振变化来监测,并通过FP信号的增加来测量。本章旨在提供一个逐步的实用程序,用于开发一种以多孔板形式进行的FP分析,以同质形式监测蛋白质-蛋白质相互作用(PPI)。

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