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首页> 外文期刊>DNA repair >Modification of the alkaline Comet assay to allow simultaneous evaluation of mitomycin C-induced DNA cross-link damage and repair of specific DNA sequences in RT4 cells.
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Modification of the alkaline Comet assay to allow simultaneous evaluation of mitomycin C-induced DNA cross-link damage and repair of specific DNA sequences in RT4 cells.

机译:修改了碱性彗星实验,可以同时评估丝裂霉素C诱导的DNA交联损伤和RT4细胞中特定DNA序列的修复。

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摘要

The alkaline Comet assay is a simple, sensitive method for measuring the extent of DNA strand breaks in individual cells. Several modifications to the original assay have been developed to increase its applications. One such modification allows the measurement of DNA cross-links by assessing the relative reduction in DNA migration induced by a strand-breaking agent. Another modification includes the application of fluorescent in situ hybridisation (FISH) to investigate the localisation of specific gene domains within a cell. Although several studies have used these approaches separately, no report to date has combined these two versions of the Comet assay. The current study describes the modification of the Comet assay, to allow both measurement of mitomycin C (MMC)-induced cross-links and the subsequent application of FISH to study repair in the TP53 gene region. RT4 human bladder cancer cells were treated with 0, 5, 50 and 200 microg/ml MMC to study dose response, whilst for cross-link repair studies, they were treated with 50 microg/ml MMC and allowed to repair for up to 24 h. A clear dose response to MMC was displayed, demonstrable by a marked reduction in DNA migration, whilst repair studies showed that MMC-induced cross-links take at least 24 h to repair fully in RT4 cells. For Comet-FISH experiments, the number and location of TP53 hybridisation spots was also recorded for each cell. In dose response experiments, the number of spots per cell, and per Comet tail, decreased as MMC dose increased. In repair experiments, the number of spots, particularly in the Comet tail, increased as repair time increased. Furthermore, our results suggest that repair of the TP53 gene region is most rapid within the first 4 h following MMC treatment. We conclude that the novel experimental protocol presented here has considerable potential in evaluating DNA damage and sequence-related repair responses to cross-linking agents.
机译:碱性彗星测定法是一种简单,灵敏的方法,用于测量单个细胞中DNA链断裂的程度。已经开发了对原始测定法的几种修改以增加其应用。一种这样的修饰允许通过评估由链断裂剂诱导的DNA迁移的相对减少来测量DNA交联。另一种修饰包括应用荧光原位杂交(FISH)研究细胞内特定基因结构域的定位。尽管有几项研究单独使用了这些方法,但迄今为止,尚无任何报告将这两种版本的Comet分析结合在一起。当前的研究描述了彗星试验的修改,以允许测量丝裂霉素C(MMC)诱导的交联,并随后应用FISH研究TP53基因区域的修复。用0、5、50和200 microg / ml MMC处理RT4人膀胱癌细胞以研究剂量反应,而对于交联修复研究,将其用50 microg / ml MMC处理并修复长达24小时。显示了对MMC的明确剂量反应,这可以通过DNA迁移的明显减少来证明,而修复研究表明MMC诱导的交联至少需要24小时才能在RT4细胞中完全修复。对于Comet-FISH实验,还记录了每个细胞的TP53杂交点的数量和位置。在剂量反应实验中,随着MMC剂量的增加,每个细胞和每个彗星尾巴的斑点数量减少。在修复实验中,斑点的数量(尤其是彗星尾巴)随着修复时间的增加而增加。此外,我们的结果表明,在MMC治疗后的最初4小时内,TP53基因区域的修复最为迅速。我们得出的结论是,本文介绍的新型实验方案在评估DNA损伤和对交联剂的序列相关修复反应方面具有相当大的潜力。

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