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The alternative role of DNA methylation in splicing regulation

机译:DNA甲基化在剪接调控中的替代作用

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Although DNA methylation was originally thought to only affect transcription, emerging evidence shows that it also regulates alternative splicing. Exons, and especially splice sites, have higher levels of DNA methylation than flanking introns, and the splicing of about 22% of alternative exons is regulated by DNA methylation. Two different mechanisms convey DNA methylation information into the regulation of alternative splicing. The first involves modulation of the elongation rate of RNA polymerase II (Pol II) by CCCTC-binding factor (CTCF) and methyl-CpG binding protein 2 (MeCP2); the second involves the formation of a protein bridge by heterochromatin protein 1 (HP1) that recruits splicing factors onto transcribed alternative exons. These two mechanisms, however, regulate only a fraction of such events, implying that more underlying mechanisms remain to be found.
机译:尽管最初认为DNA甲基化仅影响转录,但新出现的证据表明,DNA甲基化还调节其他剪接。外显子,尤其是剪接位点,比侧翼内含子具有更高的DNA甲基化水平,约22%的替代性外显子的剪接受DNA甲基化调节。两种不同的机制将DNA甲基化信息传递到替代剪接的调控中。第一个涉及CCCTC结合因子(CTCF)和甲基CpG结合蛋白2(MeCP2)对RNA聚合酶II(Pol II)延伸率的调节;第二个涉及由异染色质蛋白1(HP1)形成的蛋白桥,该蛋白桥将剪接因子募集到转录的替代外显子上。然而,这两种机制仅调节了此类事件的一小部分,这意味着仍有更多潜在的机制被发现。

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