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转录偶联修复在仓鼠细胞中是可诱导的。

Transcription-coupled repair is inducible in hamster cells.

作者信息

Germanier M, Defais M, Bohr V A, Larminat F

机构信息

Institut de Pharmacologie et de Biologie Structurale, UMR 5089, CNRS, 205 Route de Narbonne, 31400 Toulouse, France.

出版信息

Nucleic Acids Res. 2000 Dec 1;28(23):4674-8. doi: 10.1093/nar/28.23.4674.

Abstract

In mammalian cells, the rate of nucleotide excision repair of UV dimers is heterogeneous throughout the genome, with repair occurring more rapidly in the transcribed strand of active genes than in the genome overall. This repair pathway is termed transcription-coupled repair (TCR) and is thought to permit the rapid resumption of RNA synthesis following UV irradiation. To evaluate the inducibility of the TCR process, we examined the repair of UV-induced cyclobutane pyrimidine dimers (CPDs) at the level of the gene following exposure of hamster cells to a sub-lethal UV fluence, 3 h prior to a higher dose. Repair was detected by a well-established technique allowing quantification of CPDs at the level of a specific strand by Southern blot hybridization. Here, we show that prior low-dose irradiation clearly enhanced the early rate of CPD removal in the transcribed strand of the active DHFR gene. Furthermore, the RNA synthesis recovery following UV exposure was stimulated by the priming UV dose. Thus, we provide evidence for an inducible TCR response to CPDs in hamster cells. This pathway is independent of the p53 activation, since the hamster cell line that we used expresses high levels of mutant p53 protein.

摘要

在哺乳动物细胞中,紫外线二聚体的核苷酸切除修复速率在整个基因组中是不均匀的,活跃基因转录链上的修复比整个基因组中的修复发生得更快。这种修复途径被称为转录偶联修复(TCR),被认为可以使紫外线照射后RNA合成迅速恢复。为了评估TCR过程的诱导性,我们在仓鼠细胞暴露于亚致死紫外线通量3小时后,在更高剂量照射前,检测了基因水平上紫外线诱导的环丁烷嘧啶二聚体(CPD)的修复情况。通过一种成熟的技术检测修复情况,该技术允许通过Southern印迹杂交在特定链水平上对CPD进行定量。在这里,我们表明先前的低剂量照射明显提高了活跃的二氢叶酸还原酶(DHFR)基因转录链中CPD去除的早期速率。此外,紫外线暴露后的RNA合成恢复受到引发紫外线剂量的刺激。因此,我们提供了仓鼠细胞中对CPD的诱导性TCR反应的证据。该途径独立于p53激活,因为我们使用的仓鼠细胞系表达高水平的突变p53蛋白。

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