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通过细胞计数法检测ATM激活和组蛋白H2AX磷酸化,以评估外源性因素诱导的DNA损伤程度。

Cytometry of ATM activation and histone H2AX phosphorylation to estimate extent of DNA damage induced by exogenous agents.

作者信息

Tanaka Toshiki, Huang Xuan, Halicka H Dorota, Zhao Hong, Traganos Frank, Albino Anthony P, Dai Wei, Darzynkiewicz Zbigniew

机构信息

Brander Cancer Research Institute, New York Medical College, Valhalla, New York 10595, USA.

出版信息

Cytometry A. 2007 Sep;71(9):648-61. doi: 10.1002/cyto.a.20426.

Abstract

This review covers the topic of cytometric assessment of activation of Ataxia telangiectasia mutated (ATM) protein kinase and histone H2AX phosphorylation on Ser139 in response to DNA damage, particularly the damage that involves formation of DNA double-strand breaks. Briefly described are molecular mechanisms associated with activation of ATM and the downstream events that lead to recruitment of DNA repair machinery, engagement of cell cycle checkpoints, and activation of apoptotic pathway. Examples of multiparameter analysis of ATM activation and H2AX phosphorylation vis-a-vis cell cycle phase position and induction of apoptosis that employ flow- and laser scanning-cytometry are provided. They include cells treated with a variety of exogenous genotoxic agents, such as ionizing and UV radiation, DNA topoisomerase I (topotecan) and II (mitoxantrone, etoposide) inhibitors, nitric oxide-releasing aspirin, DNA replication inhibitors (aphidicolin, hydroxyurea, thymidine), and complex environmental carcinogens such as present in tobacco smoke. Also presented is an approach to identify DNA replicating (BrdU incorporating) cells based on selective photolysis of DNA that triggers H2AX phosphorylation. Listed are strategies to distinguish ATM activation and H2AX phosphorylation induced by primary DNA damage by genotoxic agents from those effects triggered by DNA fragmentation that takes place during apoptosis. While we review most published data, recent new findings also are included. Examples of multivariate analysis of ATM activation and H2AX phosphorylation presented in this review illustrate the advantages of cytometric flow- and image-analysis of these events in terms of offering a sensitive and valuable tool in studies of factors that induce DNA damage and/or affect DNA repair and allow one to explore the linkage between DNA damage, cell cycle checkpoints and initiation of apoptosis.

摘要

本综述涵盖了细胞计数评估共济失调毛细血管扩张症突变(ATM)蛋白激酶的激活以及组蛋白H2AX在丝氨酸139位点的磷酸化以响应DNA损伤的主题,特别是涉及DNA双链断裂形成的损伤。简要描述了与ATM激活相关的分子机制以及导致DNA修复机制募集、细胞周期检查点参与和凋亡途径激活的下游事件。提供了针对ATM激活和H2AX磷酸化相对于细胞周期阶段位置以及凋亡诱导的多参数分析示例,这些分析采用了流式细胞术和激光扫描细胞术。它们包括用多种外源性基因毒性剂处理的细胞,如电离辐射和紫外线辐射、DNA拓扑异构酶I(拓扑替康)和II(米托蒽醌、依托泊苷)抑制剂、释放一氧化氮的阿司匹林、DNA复制抑制剂(阿非迪霉素、羟基脲、胸腺嘧啶核苷)以及烟草烟雾中存在的复杂环境致癌物。还介绍了一种基于触发H2AX磷酸化的DNA选择性光解来识别DNA复制(掺入BrdU)细胞的方法。列出了区分由基因毒性剂引起的原发性DNA损伤诱导的ATM激活和H2AX磷酸化与凋亡过程中发生的DNA片段化引发的效应的策略。在回顾大多数已发表数据的同时,也纳入了近期的新发现。本综述中呈现的ATM激活和H2AX磷酸化多变量分析示例说明了对这些事件进行细胞计数流式分析和图像分析的优势,即它们在研究诱导DNA损伤和/或影响DNA修复的因素方面提供了一种灵敏且有价值的工具,并使人们能够探索DNA损伤、细胞周期检查点与凋亡起始之间的联系。

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