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CpG methylation as a mechanism for the regulation of E2F activity

机译:CpG甲基化作为调节E2F活性的机制

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摘要

Regulation of gene expression in mammals through methylation of cytosine residues at CpG dinucleotides is involved in the development and progression of tumors. Because many genes that are involved in the control of cell proliferation are regulated by members of the E2F family of transcription factors and because some E2F DNA-binding sites are methylated in vivo, we have investigated whether CpG methylation can regulate E2F functions. We show here that methylation of E2F elements derived from the dihydrofolate reductase, E2F1, and cdc2 promoters prevents the binding of all E2F family members tested (E2F1 through E2F5). In contrast, methylation of the E2F elements derived from the c-myc and c-myb promoters minimally affects the binding of E2F2, E2F3, E2F4, and E2F5 but significantly inhibits the binding of E2F1. Consistent with these studies, E2F3, but not E2F1, activates transcription through methylated E2F sites derived from the c-myb and c-myc genes whereas both E2F1 and E2F3 fail to transactivate a reporter gene that is under the control of a methylated dihydrofolate reductase E2F site. Together, these data illustrate a means through which E2F activity can be controlled.
机译:通过在CpG二核苷酸处的胞嘧啶残基甲基化来调节哺乳动物中的基因表达与肿瘤的发生和发展有关。由于许多参与细胞增殖控制的基因均受转录因子E2F家族成员的调节,并且由于某些E2F DNA结合位点在体内被甲基化,因此我们研究了CpG甲基化是否可以调节E2F的功能。我们在这里显示了从二氢叶酸还原酶,E2F1和cdc2启动子衍生的E2F元素的甲基化阻止了所有测试的E2F家族成员(E2F1至E2F5)的结合。相反,衍生自c-myc和c-myb启动子的E2F元素的甲基化对E2F2,E2F3,E2F4和E2F5的结合影响最小,但对E2F1的结合有明显抑制作用。与这些研究一致,E2F3而非E2F1激活通过c-myb和c-myc基因衍生的甲基化E2F位点的转录,而E2F1和E2F3均无法激活由甲基化二氢叶酸还原酶E2F控制的报告基因。现场。这些数据一起说明了可以控制E2F活动的方法。

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