首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Polymerase chain reaction-aided genomic sequencing of an X chromosome-linked CpG island: methylation patterns suggest clonal inheritance CpG site autonomy and an explanation of activity state stability.
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Polymerase chain reaction-aided genomic sequencing of an X chromosome-linked CpG island: methylation patterns suggest clonal inheritance CpG site autonomy and an explanation of activity state stability.

机译:X染色体连锁的CpG岛的聚合酶链反应辅助基因组测序:甲基化模式表明克隆遗传CpG位点自主性和活性状态稳定性的解释。

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摘要

The 5' region of the gene encoding human X chromosome-linked phosphoglycerate kinase 1 (PGK1) is a promoter-containing CpG island known to be methylated at 119 of 121 CpG dinucleotides in a 450-base-pair region on the inactive human X chromosome in the hamster-human cell line X8-6T2. Here we report the use of polymerase chain reaction-aided genomic sequencing to determine the complete methylation pattern of this region in clones derived from X8-6T2 cells after treatment with the methylation inhibitor 5-azacytidine. We find (i) a clone showing full expression of human phosphoglycerate kinase is fully unmethylated in this region; (ii) clones not expressing human phosphoglycerate kinase remain methylated at approximately 50% of CpG sites, with a pattern of interspersed methylated (M) and unmethylated (U) sites different for each clone; (iii) singles, defined as M-U-M or U-M-U, are common; and (iv) a few CpG sites are partially methylated. The data are interpreted according to a model of multiple, autonomous CpG sites, and estimates are made for two key parameters, maintenance efficiency (Em approximately 99.9% per site per generation) and de novo methylation efficiency (Ed approximately 5%). These parameter values and the hypothesis that several independent sites must be unmethylated for transcription can explain the stable maintenance of X chromosome inactivation. We also consider how the active region is kept free of methylation and suggest that transcription inhibits methylation by decreasing Em so that methylation cannot be maintained. Thus, multiple CpG sites, independent with respect to a dynamic methylation system, can stabilize two alternative states of methylation and transcription.
机译:编码人X染色体连锁的磷酸甘油酸激酶1(PGK1)的基因的5'区是一个含有启动子的CpG岛,已知该CpG岛在不活动的人X染色体的450个碱基对区域的121个CpG二核苷酸中的119个处被甲基化。在仓鼠-人细胞系X8-6T2中。在这里我们报告了使用甲基化抑制剂5-氮杂胞苷处理后,使用聚合酶链反应辅助的基因组测序来确定该区域在源自X8-6T2细胞的克隆中该区域的完全甲基化模式。我们发现(i)一个显示人磷酸甘油酸激酶完整表达的克隆在该区域完全未甲基化; (ii)不表达人磷酸甘油酸激酶的克隆在大约50%的CpG位点保持甲基化,每个克隆的散布的甲基化(M)和未甲基化(U)位点的模式不同; (iii)定义为M-U-M或U-M-U的单打是常见的; (iv)一些CpG位点被部分甲基化。根据多个自主CpG站点的模型对数据进行解释,并对两个关键参数进行估计,即维护效率(Em约为每个站点每个世代99.9%)和从头甲基化效率(Ed约为5%)。这些参数值和几个独立位点必须未甲基化才能进行转录的假设可以解释X染色体失活的稳定维持。我们还考虑了如何使活性区域保持无甲基化,并建议转录通过降低Em抑制甲基化,从而使甲基化无法维持。因此,相对于动态甲基化系统而言,多个CpG位点可以稳定甲基化和转录的两个替代状态。

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