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ChIP-Seq and RNA-Seq Analyses Identify Components of the Wnt and Fgf Signaling Pathways as Prep1 Target Genes in Mouse Embryonic Stem Cells

机译:ChIP-Seq和RNA-Seq分析将Wnt和Fgf信号通路的成分鉴定为小鼠胚胎干细胞中的Prep1目标基因

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摘要

The Prep1 (Pknox1) homeodomain transcription factor is essential at multiple stages of embryo development. In the E11.5 embryo trunk, we previously estimated that Prep1 binds about 3,300 genomic sites at a highly specific decameric consensus sequence, mainly governing basal cellular functions. We now show that in embryonic stem (ES) cells Prep1 binding pattern only partly overlaps that of the embryo trunk, with about 2,000 novel sites. Moreover, in ES cells Prep1 still binds mostly to promoters, as in total embryo trunk but, among the peaks bound exclusively in ES cells, the percentage of enhancers was three-fold higher. RNA-seq identifies about 1800 genes down-regulated in Prep1 -/- ES cells which belong to gene ontology categories not enriched in the E11.5 Prep1i/i differentiated embryo, including in particular essential components of the Wnt and Fgf pathways. These data agree with aberrant Wnt and Fgf expression levels in the Prep1 -/- ES cells with a deficient embryoid bodies (EBs) formation and differentiation. Re-establishment of the Prep1 level rescues the phenotype.
机译:Prep1(Pknox1)同源域转录因子在胚胎发育的多个阶段至关重要。在E11.5胚胎干中,我们先前估计Prep1在高度特异性的十聚共有序列上结合约3,300个基因组位点,主要控制基础细胞功能。现在,我们显示在胚胎干(ES)细胞中,Prep1的结合模式仅与胚胎干的部分重叠,约有2,000个新位点。此外,在ES细胞中,Prep1仍主要与启动子结合,就像在整个胚胎干中一样,但在仅与ES细胞结合的峰中,增强子的百分比高出三倍。 RNA-seq可识别Prep1 -/- ES细胞中约1800个被下调的基因,这些基因属于未在E11.5 Prep1 i / i 分化的胚胎中富集的基因本体论类别。 ,尤其是Wnt和Fgf途径的重要组成部分。这些数据与胚状体(EBs)形成和分化不足的Prep1 -/- ES细胞中异常的Wnt和Fgf表达水平相符。 Prep1水平的重新建立可以挽救表型。

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