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基于全内反射荧光显微镜的RecA突触前细丝动力学单分子检测

TIRF-Based Single-Molecule Detection of the RecA Presynaptic Filament Dynamics.

作者信息

Kim Sung H

机构信息

School of Biological Science, Institute of Molecular Biology and Genetics, Seoul National University, Seoul, Republic of Korea.

出版信息

Methods Enzymol. 2018;600:233-253. doi: 10.1016/bs.mie.2017.11.012. Epub 2018 Feb 1.

Abstract

RecA is a key protein in homologous DNA repair process. On a single-stranded (ss) DNA, which appears as an intermediate structure at a double-strand break site, RecA forms a kilobase-long presynaptic filament that mediates homology search and strand exchange reaction. RecA requires adenosine triphosphate as a cofactor that confers dynamic features to the filament such as nucleation, end-dependent growth and disassembly, scaffold shift along the ssDNA, and conformational change. Due to the complexity of the dynamics, detailed molecular mechanisms of functioning presynaptic filament have been characterized only recently after the advent of single-molecule techniques that allowed real-time observation of each kinetic process. In this chapter, single-molecule fluorescence resonance energy transfer assays, which revealed detailed molecular pictures of the presynaptic filament dynamics, will be discussed.

摘要

RecA是同源DNA修复过程中的关键蛋白。在双链断裂位点处作为中间结构出现的单链(ss)DNA上,RecA形成一个长达千碱基的突触前细丝,介导同源性搜索和链交换反应。RecA需要三磷酸腺苷作为辅助因子,赋予细丝动态特性,如成核、末端依赖性生长和拆卸、沿ssDNA的支架移位以及构象变化。由于动力学的复杂性,直到单分子技术出现后才得以实时观察每个动力学过程,突触前细丝功能的详细分子机制才在最近得到表征。在本章中,将讨论揭示突触前细丝动力学详细分子图景的单分子荧光共振能量转移测定法。

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