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首页> 外文期刊>Methods: A Companion to Methods in Enzymology >In vivo imaging of DNA double-strand break induced telomere mobility during alternative lengthening of telomeres
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In vivo imaging of DNA double-strand break induced telomere mobility during alternative lengthening of telomeres

机译:在DNA双链中的体内成像中,在端粒的替代延长期间诱导端粒迁移

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Repair of DNA double-strand breaks (DSBs) by homologous recombination (HR) requires mobilization of chromatin for homology searches that allow interaction of the sequence to be repaired and its template DNA. Here we describe a system to rapidly induce DSBs at telomeres and track their movement, as well as a semi-automated workflow for quantitative analysis. We have successfully used this approach to show that DSBs targeted to telomeres in cells utilizing the alternative lengthening of telomeres (ALT) mechanism increase their diffusion and subsequent long-range directional movement to merge with telomeres on other chromosomes. These methods are simple to implement and are compatible with almost any cell line or in vivo microscopy setup. The magnitude of DSB-induced telomere mobility allows the investigator to easily test for factors regulating telomere mobility during ALT. (C) 2016 Elsevier Inc. All rights reserved.
机译:通过同源重组(HR)修复DNA双链断裂(DSB)需要动员染色质的同源搜索,其允许修复序列的相互作用及其模板DNA。 在这里,我们描述了一种快速诱导端粒的DSB的系统并跟踪其运动,以及用于定量分析的半自动工作流程。 我们已成功使用这种方法,以表明利用端粒的替代延长(ALT)机制的替代延长来表明DSB靶向细胞中的端粒(ALT)机制增加了它们的扩散和随后的远程方向运动以与其他染色体上的端粒合并。 这些方法易于实现,并且与几乎任何细胞系或体内显微镜设置兼容。 DSB诱导的端粒移动性的幅度允许调查员在ALT期间容易地测试调节端粒移动性的因素。 (c)2016年Elsevier Inc.保留所有权利。

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