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Probing the chromosome 9p21 region susceptible to DNA double-strand breaks in human cells in vivo by restriction enzyme transfer

机译:通过限制酶转移探测易于DNA双链的染色体9p21区域易受DNA双链中的分裂

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A restriction enzyme, MspI, was introduced into cultured human cells as a probe to detect genomic regions susceptible to DNA double-strand breaks (DSBs). A 2h exposure to MspI at a concentration of 8U/l produced DSBs at MspI sites in more than 80% of HeLa cells. The sensitivity to digestion was examined on chromosomal DNAs for the region containing the p16 tumor suppressor gene and two other related genes, p14ARF and p15, by Southern blot hybridization analysis and linker-mediated capture of DNA fragments digested in vivo. DNAs for the promoter regions of the three genes, respectively, were sensitive to MspI digestion in HeLa cells, while DNA for the p16 promoter region was less sensitive in lung cancer cells with hypermethylation of the region. Breakpoints for interstitial 9p21 deletions removing the p16/p14ARF/p15 locus in a variety of human cancers were significantly over-represented in the three sensitive regions. The results suggest that the MspI sensitivity in vivo of each genomic region reflects its susceptibility to DSBs that trigger chromosome aberrations in human cells. This method could help us understand the pathogenic significance of differential susceptibility to DSBs among genomic regions in human carcinogenesis.
机译:将限制酶MSPI引入培养的人体细胞中作为探针,以检测易于DNA双链断裂(DSB)的基因组区域。在MSPI位点的浓度下,在MSPI位点的浓度下暴露于MSPI,超过80%以上的HeLa细胞。在含有P16肿瘤抑制基因和另外两个相关基因,P14ARF和P15的区域的区域的染色体DNA上检查对消化的敏感性通过Southern印迹杂交分析和在体内消化的DNA片段的接头介导的捕获。对于三种基因的启动子区域的DNA分别对HeLa细胞中的MSPI消化敏感,而P16启动子区的DNA在肺癌细胞中对该区域的高甲基化敏感。在三种敏感区域中,在各种人类癌症中除去P16 / P14ARF / P15基因座的间质9p21缺失的断点是显着的过度代表。结果表明,每个基因组区域的体内MSPI敏感性反映了其对DSB的易感性,其触发人细胞中的染色体畸变。该方法可以帮助我们了解人类致癌基因组区域中对DSB对DSB对DSB的致病意义。

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