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Imaging Mismatch Repair and Cellular Responses to DNA Damage in Bacillus subtilis

机译:成像错配修复和细胞对枯草芽孢杆菌DNA损伤的反应。

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摘要

Both prokaryotes and eukaryotes respond to DNA damage through a complex set of physiological changes. Alterations in gene expression, the redistribution of existing proteins, and the assembly of new protein complexes can be stimulated by a variety of DNA lesions and mismatched DNA base pairs. Fluorescence microscopy has been used as a powerful experimental tool for visualizing and quantifying these and other responses to DNA lesions and to monitor DNA replication status within the complex subcellular architecture of a living cell. Translational fusions between fluorescent reporter proteins and components of the DNA replication and repair machinery have been used to determine the cues that target DNA repair proteins to their cognate lesions in vivo and to understand how these proteins are organized within bacterial cells. In addition, transcriptional and translational fusions linked to DNA damage inducible promoters have revealed which cells within a population have activated genotoxic stress responses. In this review, we provide a detailed protocol for using fluorescence microscopy to image the assembly of DNA repair and DNA replication complexes in single bacterial cells. In particular, this work focuses on imaging mismatch repair proteins, homologous recombination, DNA replication and an SOS-inducible protein in Bacillus subtilis. All of the procedures described here are easily amenable for imaging protein complexes in a variety of bacterial species.
机译:原核生物和真核生物均通过一系列复杂的生理变化来应对DNA损伤。基因表达的改变,现有蛋白质的重新分布以及新蛋白质复合物的组装都可以通过多种DNA损伤和错配的DNA碱基对来刺激。荧光显微镜已被用作功能强大的实验工具,用于可视化和量化对DNA损伤的这些和其他响应,并监视活细胞复杂的亚细胞结构内的DNA复制状态。荧光报道蛋白与DNA复制和修复机制的组成部分之间的翻译融合已用于确定将DNA修复蛋白靶向体内同源损伤的线索,并了解这些蛋白如何在细菌细胞内组织。此外,与DNA损伤诱导型启动子相连的转录和翻译融合揭示了种群中的哪些细胞具有激活的遗传毒性应激反应。在这篇综述中,我们提供了使用荧光显微镜对单个细菌细胞中DNA修复和DNA复制复合物的组装进行成像的详细协议。特别地,这项工作着重于对枯草芽孢杆菌中的错配修复蛋白,同源重组,DNA复制和SOS诱导蛋白进行成像。此处描述的所有步骤均易于使各种细菌物种中的蛋白质复合物成像。

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