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一种用于评估人类肿瘤细胞中DNA双链断裂修复保真度的新型快速检测方法的开发。

Development of a novel rapid assay to assess the fidelity of DNA double-strand-break repair in human tumour cells.

作者信息

Collis S J, Sangar V K, Tighe A, Roberts S A, Clarke N W, Hendry J H, Margison G P

机构信息

CRC Experimental Radiation Oncology Group, Paterson Institute for Cancer Research, Christie Hospital NHS Trust, Wilmslow Road, Manchester M20 4BX, UK.

出版信息

Nucleic Acids Res. 2002 Jan 15;30(2):E1. doi: 10.1093/nar/30.2.e1.

Abstract

Cellular survival following ionising radiation-mediated damage is primarily a function of the ability to successfully detect and repair DNA double-strand breaks (DSBs). Previous studies have demonstrated that radiosensitivity, determined as a reduction in colony forming ability in vitro, may be related to the incorrect repair (misrepair) of DSBs. The novel rapid dual fluorescence (RDF) assay is a plasmid-based reporter system that rapidly assesses the correct rejoining of a restriction-enzyme produced DSBs within transfected cells. We have utilised this novel assay to determine the fidelity of DSB repair in the prostate tumour cell line LNCaP, the bladder tumour cell line MGH-U1 and a radiosensitive subclone S40b. The two bladder cell lines have been shown in previous studies to differ in their ability to correctly repair plasmids containing a single DSB. Using the RDF assay we found that a substantial portion of LNCaP cells [80.4 +/- 5.3(standard error)%] failed to reconstitute reporter gene expression; however, there was little difference in this measure of DSB repair fidelity between the two bladder cell lines (48.3 +/- 3.5% for MGH-U1; 39.9 +/- 8.2% for S40b). The RDF assay has potential to be developed to study the relationship between DSB repair fidelity and radiosensitivity as well as the mechanisms associated with this type of repair defect.

摘要

电离辐射介导的损伤后细胞存活主要取决于成功检测和修复DNA双链断裂(DSB)的能力。先前的研究表明,放射敏感性(以体外集落形成能力的降低来确定)可能与DSB的错误修复(错配修复)有关。新型快速双荧光(RDF)检测是一种基于质粒的报告系统,可快速评估转染细胞内限制性内切酶产生的DSB的正确重新连接。我们利用这种新型检测方法来确定前列腺肿瘤细胞系LNCaP、膀胱肿瘤细胞系MGH-U1和放射敏感亚克隆S40b中DSB修复的保真度。先前的研究表明,这两种膀胱细胞系在正确修复含有单个DSB的质粒的能力上存在差异。使用RDF检测,我们发现很大一部分LNCaP细胞[80.4 +/- 5.3(标准误差)%]未能恢复报告基因表达;然而,这两种膀胱细胞系在DSB修复保真度的这一指标上几乎没有差异(MGH-U1为48.3 +/- 3.5%;S40b为39.9 +/- 8.2%)。RDF检测有潜力被开发用于研究DSB修复保真度与放射敏感性之间的关系以及与这种修复缺陷相关的机制。

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