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Ribonucleoprotein-masked nicks at 50-kbp intervals in the eukaryotic genomic DNA

机译:真核基因组DNA中核糖蛋白掩盖的切口,间隔为50 kbp

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摘要

By using a microscopic approach, field inversion single-cell gel electrophoresis, we show that preformed single-strand discontinuities are present in the chromatin of resting and proliferating mammalian and yeast cells. These single-strand breaks are primarily nicks positioned at ≈50-kbp intervals throughout the entire genome that could be efficiently labeled in situ by DNA polymerase I holoenzyme but not by Klenow fragment and terminal trans-ferase unless after ribonucleolytic treatments. The RNA molecules involved appear to comprise R-loops, recognized by the S9.6 RNA/DNA hybrid-specific antibody. By using the breakpoint cluster region of the Mixed Lineage Leukemia (MLL) gene as a model, we have found that the number of manifest nicks detected by FISH performed after field inversion single-cell gel electrophoresis depends on epigenetic context, but the difference between germ-line and translocated MLL alleles is abolished by protease treatment. Our data imply that the double-stranded genomic DNA is composed of contiguous rather than continuous single strands and reveal an aspect of higher-order chromatin organization with ribonucleoprotein-associated persistent nicks defining ≈50-kbp domains.
机译:通过使用显微镜的方法,现场倒置单细胞凝胶电泳,我们表明在静止和增殖的哺乳动物和酵母细胞的染色质中存在预先形成的单链不连续性。这些单链断裂主要是在整个基因组中以大约50-kbp的间隔定位的缺口,除非经过核糖核酸水解处理,否则可以通过DNA聚合酶I全酶有效地原位标记,而不能通过Klenow片段和末端反式转移酶有效地原位标记。所涉及的RNA分子似乎包含被S9.6 RNA / DNA杂交特异性抗体识别的R环。通过使用混合谱系白血病(MLL)基因的断点簇区域作为模型,我们发现场反转单细胞凝胶电泳后FISH检测到的明显切口数量取决于表观遗传背景,但细菌之间的差异蛋白酶处理消除了线型和易位的MLL等位基因。我们的数据表明,双链基因组DNA由连续的而不是连续的单链组成,揭示了具有与核糖蛋白相关的持久缺口的高级染色质组织的一个方面,这些缺口定义了≈50-kbp结构域。

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