首页> 外文期刊>Mutation Research: International Journal on Mutagenesis, Chromosome Breakage and Related Subjects >G2 phase repair of X-ray-induced chromosomal DNA damage in trichothiodystrophy cells.
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G2 phase repair of X-ray-induced chromosomal DNA damage in trichothiodystrophy cells.

机译:X射线诱导的毛滴虫营养不良细胞中的染色体DNA损伤的G2期修复。

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The repair of X-ray-induced DNA damage during G2 cell-cycle phase has been examined in lines of skin fibroblasts from three patients with trichothiodystrophy (TTD), one with apparently normal and two with defective nucleotide excision repair (NER). These responses are compared with those of five lines from clinically normal controls, lines from xeroderma pigmentosum (XP), Cockayne syndrome (CS), Down syndrome (DS), and ataxia telangiectasia (AT) patients. Chromosomal DNA repair was measured as the chromatid aberration frequency (CAF) or total number of chromatid breaks and long gaps per 100 metaphase cells, determined 0.5-1.5 h after X-irradiation (53 rad). Chromatid breaks and gaps (as defined herein) represent unrepaired DNA strand breaks. Only one of the TTD lines, TTD 1BR, showed an abnormally high CAF. This line was shown subsequently to be of a different complementation group, representing a new nucleotide excision repair gene. An abnormally high CAF was also observed, as reported previously, in XP-C, AT and DS but not in CS skin fibroblasts. In addition, cell lines were examined for DNA incision activity by an indirect method in which chromatid aberrations were enumerated with or without ara-C, an inhibitor of repair synthesis, added after X-irradiation. All TTD lines had abnormally low incision activity.
机译:在来自三名毛发硫代营养不良症(TTD)的一名患者的皮肤成纤维细胞系中,检查了在G2细胞周期阶段X射线诱导的DNA损伤的修复,其中一名患者表面正常,而两名患者核苷酸切除修复不良(NER)。将这些反应与来自临床正常对照的五种细胞系,色素干性皮肤病(XP),Cockayne综合征(CS),唐氏综合症(DS)和共济失调毛细血管扩张(AT)患者的5种细胞的反应进行了比较。染色体DNA修复的测量方法是,在X射线照射后(53 rad)确定0.5-1.5 h的染色质畸变频率(CAF)或染色质断裂总数和每100个中期细胞的长间隙。染色单体断裂和缺口(如本文所定义)代表未修复的DNA链断裂。 TTD行中只有一个TTD 1BR显示异常高的CAF。随后显示该品系属于不同的互补组,代表新的核苷酸切除修复基因。如先前报道,在XP-C,AT和DS中也观察到了异常高的CAF,但在CS皮肤成纤维细胞中却未观察到。此外,通过间接方法检查细胞系的DNA切割活性,其中在X射线照射后添加或不添加ara-C(修复合成抑制剂)的情况下计数染色单体畸变。所有TTD细胞系均具有异常低的切口活性。

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