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PU.1 inhibits the erythroid program by binding to GATA-1 on DNA and creating a repressive chromatin structure

机译:PU.1通过与DNA上的GATA-1结合并产生抑制性染色质结构来抑制类红细胞程序

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摘要

Transcriptional repression mechanisms are important during differentiation of multipotential hematopoietic progenitors, where they are thought to regulate lineage commitment and to extinguish alternative differentiation programs. PU.1 and GATA-1 are two critical hematopoietic transcription factors that physically interact and mutually antagonize each other's transcriptional activity and ability to promote myeloid and erythroid differentiation, respectively. We find that PU.1 inhibits the erythroid program by binding to GATA-1 on its target genes and organizing a complex of proteins that creates a repressive chromatin structure containing lysine-9 methylated H3 histones and heterochromatin protein 1. Although these features are thought to be stable aspects of repressed chromatin, we find that silencing of PU.1 expression leads to removal of the repression complex, loss of the repressive chromatin marks and reactivation of the erythroid program. This process involves incorporation of the replacement histone variant H3.3 into nucleosomes. Repression of one transcription factor bound to DNA by another transcription factor not on the DNA represents a new mechanism for downregulating an alternative gene expression program during lineage commitment of multipotential hematopoietic progenitors.
机译:转录抑制机制在多能造血祖细胞的分化过程中很重要,据认为它们可调节血统承诺并消除其他分化程序。 PU.1和GATA-1是两个至关重要的造血转录因子,它们在物理上相互作用并相互拮抗彼此的转录活性以及促进髓样和红系分化的能力。我们发现,PU.1通过与目标基因上的GATA-1结合并组织蛋白复合物来抑制红系程序,该蛋白复合物产生了包含赖氨酸9甲基化的H3组蛋白和异染色质蛋白1的阻抑染色质结构。尽管这些特征被认为作为抑制的染色质的稳定方面,我们发现PU.1表达的沉默导致抑制复合物的去除,抑制的染色质标记的丢失和红系程序的重新激活。该过程涉及将替代组蛋白变体H3.3掺入核小体中。用另一种不在DNA上的转录因子抑制与DNA结合的一种转录因子代表了一种新的机制,可在多能造血祖细胞的谱系定型过程中下调另一种基因表达程序。

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