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Genome-wide analysis of the H3K4 histone demethylase RBP2 reveals a transcriptional program controlling differentiation.

机译:H3K4组蛋白脱甲基酶RBP2的全基因组分析揭示了控制分化的转录程序。

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摘要

Retinoblastoma protein (pRB) mediates cell-cycle withdrawal and differentiation by interacting with a variety of proteins. RB-Binding Protein 2 (RBP2) has been shown to be a key effector. We sought to determine transcriptional regulation by RBP2 genome-wide by using location analysis and gene expression profiling experiments. We describe that RBP2 shows high correlation with the presence of H3K4me3 and its target genes are separated into two functionally distinct classes: differentiation-independent and differentiation-dependent genes. The former class is enriched by genes that encode mitochondrial proteins, while the latter is represented by cell-cycle genes. We demonstrate the role of RBP2 in mitochondrial biogenesis, which involves regulation of H3K4me3-modified nucleosomes. Analysis of expression changes upon RBP2 depletion depicted genes with a signature of differentiation control, analogous to the changes seen upon reintroduction of pRB. We conclude that, during differentiation, RBP2 exerts inhibitory effects on multiple genes through direct interaction with their promoters.
机译:视网膜母细胞瘤蛋白(pRB)通过与多种蛋白相互作用来介导细胞周期的退出和分化。 RB结合蛋白2(RBP2)已被证明是关键效应子。我们试图通过使用位置分析和基因表达谱实验来确定全基因组RBP2的转录调控。我们描述RBP2显示与H3K4me3的存在高度相关,其目标基因分为两个功能不同的类别:分化独立和分化依赖基因。前一类富含编码线粒体蛋白的基因,而后者则以细胞周期基因为代表。我们证明RBP2在线粒体生物发生,其中涉及H3K4me3修饰的核小体调控的作用。 RBP2耗尽后的表达变化分析显示了具有分化控制特征的基因,类似于重新引入pRB时看到的变化。我们得出的结论是,在分化过程中,RBP2通过与其启动子直接相互作用而对多个基因产生抑制作用。

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