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AML1/RUNX1 increases during G1 to S cell cycle progression independent of cytokine-dependent phosphorylation and induces cyclin D3 gene expression.AML1/RUNX1在G1期到S期细胞周期进程中增加,与细胞因子依赖性磷酸化无关,并诱导细胞周期蛋白D3基因表达。
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Runx1在哺乳动物神经系统中特定祖细胞的增殖和神经元分化中的作用。

Role for Runx1 in the proliferation and neuronal differentiation of selected progenitor cells in the mammalian nervous system.

作者信息

Theriault Francesca M, Nuthall Hugh N, Dong Zhifeng, Lo Rita, Barnabe-Heider Fanie, Miller Freda D, Stifani Stefano

机构信息

Center for Neuronal Survival, Montreal Neurological Institute, McGill University, Montreal, Quebec, H3A 2B4 Canada.

出版信息

J Neurosci. 2005 Feb 23;25(8):2050-61. doi: 10.1523/JNEUROSCI.5108-04.2005.

DOI:10.1523/JNEUROSCI.5108-04.2005
PMID:15728845
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6726063/
Abstract

Neurogenesis requires factors that regulate the decision of dividing progenitors to leave the cell cycle and activate the neuronal differentiation program. It is shown here that the murine runt-related gene Runx1 is expressed in proliferating cells on the basal side of the olfactory epithelium. These include both Mash1+ olfactory receptor neuron (ORN) progenitors and NeuroD+ ORN precursors. Disruption of Runx1 function in vivo does not cause a change in Mash1 expression but leads to a decrease in the number of NeuroD+ neuronal precursors and an increase in differentiated ORNs. These effects result in premature and ectopic ORN differentiation. It is shown further that exogenous Runx1 expression in cultured olfactory neural progenitors causes an expansion of the mitotic cell population. In agreement with these findings, exogenous Runx1 expression also promotes cortical neural progenitor cell proliferation without inhibiting neuronal differentiation. These effects are phenocopied by a chimeric protein containing ETO, the eight twenty one transcriptional repressor, fused to the Runx1 DNA-binding domain, which suggests the involvement of transcription repression mechanisms. Consistent with this possibility, Runx1 represses transcription driven by the promoter of the cell cycle inhibitor p21Cip 1 in cortical progenitors. Together, these findings suggest a previously unrecognized role for Runx1 in coordinating the proliferation and neuronal differentiation of selected populations of neural progenitors.

摘要

神经发生需要一些因子来调节分裂中的祖细胞退出细胞周期并启动神经元分化程序的决定。本文表明,小鼠的 runt 相关基因 Runx1 在嗅觉上皮基底侧的增殖细胞中表达。这些细胞包括 Mash1+嗅觉受体神经元(ORN)祖细胞和 NeuroD+ORN 前体细胞。体内 Runx1 功能的破坏不会导致 Mash1 表达的改变,但会导致 NeuroD+神经元前体细胞数量减少以及分化的 ORN 增加。这些效应导致 ORN 过早和异位分化。进一步表明,在培养的嗅觉神经祖细胞中外源表达 Runx1 会导致有丝分裂细胞群体的扩大。与这些发现一致,外源 Runx1 表达也促进皮质神经祖细胞增殖而不抑制神经元分化。含有 ETO(八二一转录抑制因子)并与 Runx1 DNA 结合域融合的嵌合蛋白模拟了这些效应,这表明转录抑制机制的参与。与此可能性一致,Runx1 在皮质祖细胞中抑制由细胞周期抑制剂 p21Cip 1 的启动子驱动的转录。总之,这些发现表明 Runx1 在协调特定神经祖细胞群体的增殖和神经元分化方面具有先前未被认识的作用。