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通过单细胞和单分子成像研究DNA修复的组织方式。

Studying the organization of DNA repair by single-cell and single-molecule imaging.

作者信息

Uphoff Stephan, Kapanidis Achillefs N

机构信息

Department of Biochemistry, University of Oxford, Oxford OX1 3QU, United Kingdom.

Biological Physics Research Group, Clarendon Laboratory, Department of Physics, University of Oxford, Oxford OX1 3PU, United Kingdom.

出版信息

DNA Repair (Amst). 2014 Aug;20(100):32-40. doi: 10.1016/j.dnarep.2014.02.015. Epub 2014 Mar 12.

Abstract

DNA repair safeguards the genome against a diversity of DNA damaging agents. Although the mechanisms of many repair proteins have been examined separately in vitro, far less is known about the coordinated function of the whole repair machinery in vivo. Furthermore, single-cell studies indicate that DNA damage responses generate substantial variation in repair activities across cells. This review focuses on fluorescence imaging methods that offer a quantitative description of DNA repair in single cells by measuring protein concentrations, diffusion characteristics, localizations, interactions, and enzymatic rates. Emerging single-molecule and super-resolution microscopy methods now permit direct visualization of individual proteins and DNA repair events in vivo. We expect much can be learned about the organization of DNA repair by linking cell heterogeneity to mechanistic observations at the molecular level.

摘要

DNA修复可保护基因组免受多种DNA损伤剂的影响。尽管许多修复蛋白的机制已在体外分别进行了研究,但对于整个修复机制在体内的协同功能了解甚少。此外,单细胞研究表明,DNA损伤反应会导致细胞间修复活性产生显著差异。本综述聚焦于荧光成像方法,这些方法通过测量蛋白质浓度、扩散特性、定位、相互作用和酶促速率,对单细胞中的DNA修复进行定量描述。新兴的单分子和超分辨率显微镜方法现在能够直接在体内可视化单个蛋白质和DNA修复事件。我们期望通过将细胞异质性与分子水平的机制观察联系起来,可以更多地了解DNA修复的组织方式。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/4ca5/4119245/3745fe07010c/gr1.jpg

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