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用于单分子荧光共振能量转移的蛋白质标记

Labeling proteins for single-molecule FRET.

作者信息

Joo Chirlmin, Ha Taekjip

出版信息

Cold Spring Harb Protoc. 2012 Sep 1;2012(9):1009-12. doi: 10.1101/pdb.prot071035.

Abstract

Single-molecule (sm) fluorescence detection is a powerful method for studying biological events without time and population averaging. Förster (fluorescence) resonance energy transfer (FRET) is a spectroscopic technique for measuring distances in the 30-80 Å range in which excitation energy of a donor molecule is transferred to an acceptor via interaction between two induced dipoles. A variant of smFRET is based on total internal reflection (TIR) microscopy. This protocol describes the labeling of protein for smFRET with TIR microscopy. It is based on a labeling procedure for E. coli Rep helicase. A different assay (e.g., different chemical conditions) may be required for other proteins.

摘要

单分子(sm)荧光检测是一种强大的方法,可用于研究生物事件,无需进行时间和群体平均。福斯特(荧光)共振能量转移(FRET)是一种光谱技术,用于测量30-80 Å范围内的距离,其中供体分子的激发能量通过两个感应偶极子之间的相互作用转移到受体。smFRET的一种变体基于全内反射(TIR)显微镜。本方案描述了使用TIR显微镜对蛋白质进行smFRET标记的方法。它基于大肠杆菌Rep解旋酶的标记程序。其他蛋白质可能需要不同的检测方法(例如,不同的化学条件)。

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