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Atypical RNA polymerase subunits required for RNA-directed DNA methylation

机译:RNA指导的DNA甲基化所需的非典型RNA聚合酶亚基

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RNA- directed DNA methylation, one of several RNA interference - mediated pathways in the nucleus(1), has been documented in plants(2,3) and in human cells(4,5). Despite progress in identifying the DNA methyltransferases, histone-modifying enzymes and RNA interference proteins needed for RNA- directed DNA methylation(1), the mechanism remains incompletely understood. We screened for mutants defective in RNA- directed DNA methylation and silencing of a transgene promoter in Arabidopsis thaliana and identified three drd complementation groups(6). DRD1 is a SNF2- like protein(6) required for RNA- directed de novo methylation. We report here that DRD2 and DRD3 correspond to the second- largest subunit and largest subunit, respectively, of a fourth class of DNA- dependent RNA polymerase ( polymerase IV) that is unique to plants. DRD3 is a functionally diversified homolog of NRPD1a or SDE4, identified in a separate screen for mutants defective in post- transcriptional gene silencing(7,8). The identical DNA methylation patterns observed in all three drd mutants suggest that DRD proteins cooperate to create a substrate for RNA- directed de novo methylation.
机译:RNA定向的DNA甲基化是细胞核中几种RNA干扰介导的途径之一(1),已在植物(2,3)和人细胞(4,5)中得到记录。尽管在鉴定DNA定向的DNA甲基化所需的DNA甲基转移酶,组蛋白修饰酶和RNA干扰蛋白方面取得了进展(1),但其机理尚不完全清楚。我们筛选了拟南芥中RNA定向DNA甲基化和转基因启动子沉默的缺陷突变体,并确定了三个drd互补组(6)。 DRD1是RNA导向的从头甲基化所需的SNF2样蛋白(6)。我们在这里报告DRD2和DRD3分别对应于植物特有的第四类DNA依赖性RNA聚合酶(聚合酶IV)的第二大亚基和最大亚基。 DRD3是NRPD1a或SDE4的功能多样化同源物,在针对转录后基因沉默缺陷的突变体的单独筛选中鉴定出(7,8)。在所有三个drd突变体中观察到的相同的DNA甲基化模式表明DRD蛋白协同作用为RNA定向的从头甲基化创造了底物。

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