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Genomewide demarcation of RNA polymerase II transcription units revealed by physical fractionation of chromatin

机译:染色质的物理分级显示RNA聚合酶II转录单位的全基因组分界

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摘要

Epigenetic modifications of chromatin serve an important role in regulating the expression and accessibility of genomic DNA. We report here a genomewide approach for fractionating yeast chromatin into two functionally distinct parts, one containing RNA polymerase II transcribed sequences, and the other comprising noncoding sequences and genes transcribed by RNA polymerases I and III. Noncoding regions could be further fractionated into promoters and segments lacking promoters. The observed separations were apparently based on differential crosslinking efficiency of chromatin in different genomic regions. The results reveal a genomewide molecular mechanism for marking promoters and genomic regions that have a license to be transcribed by RNA polymerase II, a previously unrecognized level of genomic complexity that may exist in all eukaryotes. Our approach has broad potential use as a tool for genome annotation and for the characterization of global changes in chromatin structure that accompany different genetic, environmental, and disease states.
机译:染色质的表观遗传修饰在调节基因组DNA的表达和可及性中起重要作用。我们在这里报告了一种全基因组的方法,用于将酵母染色质分为两个功能不同的部分,一个包含RNA聚合酶II转录的序列,另一个包含非编码序列和RNA聚合酶I和III转录的基因。非编码区可以进一步分为启动子和缺乏启动子的片段。观察到的分离显然基于不同基因组区域中染色质的不同交联效率。结果揭示了标记启动子和基因组区域的全基因组分子机制,该启动子和基因组区域具有被RNA聚合酶II转录的许可,RNA聚合酶II是以前在所有真核生物中都无法识别的基因组复杂性水平。我们的方法作为基因组注释工具和表征伴随不同遗传,环境和疾病状态的染色质结构整体变化的特征,具有广泛的潜在用途。

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