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Extranucleosomal DNA enhances the activity of the LSD1/CoREST histone demethylase complex

机译:核小体外DNA增强LSD1 / CoREST组蛋白脱甲基酶复合物的活性

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The promoter regions of active genes in the eukaryotic genome typically contain nucleosomes post-translationally modified with a trimethyl mark on histone H3 lysine 4 (H3K4), while transcriptional enhancers are marked with monomethylated H3K4. The flavin-dependent monoamine oxidase LSD1 (lysine-specific demethylase 1, also known as KDM1) demethylates mono-and dimethylated H3K4 in peptide substrates, but requires the corepressor protein, CoREST, to demethylate nucleosome substrates. The molecular basis for how the LSD1/CoREST complex interacts with its physiological nucleosome substrate remains largely unknown. We examine here the role of extranucleosomal DNA beyond the nucleosome core particle for LSD1/CoREST function. Our studies of LSD1/CoREST's enzyme activity and nucleosome binding show that extranucleosomal DNA dramatically enhances the activity of LSD1/CoREST, and that LSD1/CoREST binds to the nucleosome as a 1: 1 complex. Our photocrosslinking experiments further indicate both LSD1 and CoREST subunits are in close contact with DNA around the nucleosome dyad as well as extranucleosomal DNA. Our results suggest that the LSD1/CoREST interacts with extranucleosomal DNA when it productively engages its nucleosome substrate.
机译:真核生物基因组中活性基因的启动子区域通常含有核糖体,该核糖体经过翻译后修饰后具有组蛋白H3赖氨酸4(H3K4)上的三甲基标记,而转录增强子则被单甲基化的H3K4标记。黄素依赖性单胺氧化酶LSD1(赖氨酸特异性脱甲基酶1,也称为KDM1)使肽底物中的H3K4和二甲基化的H3K4去甲基化,但需要共核心蛋白CoREST来使核小体底物脱甲基化。 LSD1 / CoREST复合物如何与其生理性核小体底物相互作用的分子基础仍然未知。我们在这里检查LSD1 / CoREST功能的核小体核心颗粒以外的核小体DNA的作用。我们对LSD1 / CoREST的酶活性和核小体结合的研究表明,核小体外DNA显着增强了LSD1 / CoREST的活性,而LSD1 / CoREST以1:1的复合物形式与核小体结合。我们的光交联实验进一步表明,LSD1和CoREST亚基都与核小体周围的DNA以及核小体DNA紧密接触。我们的结果表明,当LSD1 / CoREST有效结合其核小体底物时,它会与核小体外DNA相互作用。

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