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由 G-四链体配体诱导的局部表观遗传重编程。

Local epigenetic reprogramming induced by G-quadruplex ligands.

机构信息

MRC Laboratory of Molecular Biology, Francis Crick Avenue, Cambridge CB2 0QH, UK.

Department of Chemistry, University of Cambridge, Lensfield Road, Cambridge CB2 1EW, UK.

出版信息

Nat Chem. 2017 Nov;9(11):1110-1117. doi: 10.1038/nchem.2828. Epub 2017 Jul 31.

Abstract

DNA and histone modifications regulate transcriptional activity and thus represent valuable targets to reprogram the activity of genes. Current epigenetic therapies target the machinery that regulates these modifications, leading to global transcriptional reprogramming with the potential for extensive undesired effects. Epigenetic information can also be modified as a consequence of disrupting processive DNA replication. Here, we demonstrate that impeding replication by small-molecule-mediated stabilization of G-quadruplex nucleic acid secondary structures triggers local epigenetic plasticity. We report the use of the BU-1 locus of chicken DT40 cells to screen for small molecules able to induce G-quadruplex-dependent transcriptional reprogramming. Further characterization of the top hit compound revealed its ability to induce a dose-dependent inactivation of BU-1 expression in two steps: the loss of H3K4me3 and then subsequent DNA cytosine methylation, changes that were heritable across cell divisions even after the compound was removed. Targeting DNA secondary structures thus represents a potentially new approach for locus-specific epigenetic reprogramming.

摘要

DNA 和组蛋白修饰调节转录活性,因此是重新编程基因活性的有价值的靶点。目前的表观遗传疗法针对的是调节这些修饰的机制,导致广泛的潜在不良影响的全局转录重编程。表观遗传信息也可以作为破坏连续 DNA 复制的结果而被修饰。在这里,我们证明了通过小分子介导的 G-四链体核酸二级结构的稳定来阻碍复制会引发局部表观遗传可塑性。我们报告了使用鸡 DT40 细胞的 BU-1 基因座来筛选能够诱导 G-四链体依赖性转录重编程的小分子。对顶级命中化合物的进一步表征揭示了其能够在两步中诱导 BU-1 表达的剂量依赖性失活:H3K4me3 的丢失,然后是随后的 DNA 胞嘧啶甲基化,即使在化合物被去除后,这些变化在细胞分裂中仍然是可遗传的。因此,靶向 DNA 二级结构代表了一种用于特定基因座的表观遗传重编程的潜在新方法。

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