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基因本体驱动的CD34 +细胞启动的巨核细胞培养转录分析确定了巨核细胞生成的新转录调节因子。

Gene Ontology-driven transcriptional analysis of CD34+ cell-initiated megakaryocytic cultures identifies new transcriptional regulators of megakaryopoiesis.

作者信息

Fuhrken Peter G, Chen Chi, Apostolidis Pani A, Wang Min, Miller William M, Papoutsakis Eleftherios T

机构信息

Department of Chemical and Biological Engineering, Northwestern University, Evanston, Illinois, USA.

出版信息

Physiol Genomics. 2008 Apr 22;33(2):159-69. doi: 10.1152/physiolgenomics.00127.2007. Epub 2008 Feb 5.

DOI:10.1152/physiolgenomics.00127.2007
PMID:18252802
Abstract

Differentiation of hematopoietic stem and progenitor cells is an intricate process controlled in large part at the level of transcription. While some key megakaryocytic transcription factors have been identified, the complete network of megakaryocytic transcriptional control is poorly understood. Using global gene expression microarray analysis, Gene Ontology-based functional annotations, and a novel interlineage comparison with parallel, isogenic granulocytic cultures as a negative control, we closely examined the mRNA level of transcriptional regulators in megakaryocytes derived from human mobilized peripheral blood CD34(+) hematopoietic cells. This approach identified 199 differentially expressed transcription factors or transcriptional regulators. We identified and detailed the transcriptional kinetics of most known megakaryocytic transcription factors including GATA1, FLI1, and MAFG. Furthermore, many genes with transcription factor activity or transcription factor binding activity were identified in megakaryocytes that had not previously been associated with that lineage, including BTEB1, NR4A2, FOXO1A, MEF2C, HDAC5, VDR, and several genes associated with the tumor suppressor p53 (HIPK2, FHL2, and TADA3L). Protein expression and nuclear localization were confirmed in megakaryocytic cells for four of the novel candidate megakaryocytic transcription factors: FHL2, MXD1, E2F3, and RFX5. In light of the hypothesis that transcription factors expressed in a particular differentiation program are important contributors to such a program, these data substantially expand our understanding of transcriptional regulation in megakaryocytic differentiation of stem and progenitor cells.

摘要

造血干细胞和祖细胞的分化是一个复杂的过程,在很大程度上受转录水平的控制。虽然已经鉴定出一些关键的巨核细胞转录因子,但对巨核细胞转录控制的完整网络仍知之甚少。我们使用全局基因表达微阵列分析、基于基因本体论的功能注释,以及与平行的同基因粒细胞培养物进行新型谱系间比较作为阴性对照,密切研究了源自人动员外周血CD34(+)造血细胞的巨核细胞中转录调节因子的mRNA水平。这种方法鉴定出199种差异表达的转录因子或转录调节因子。我们鉴定并详细研究了大多数已知的巨核细胞转录因子的转录动力学,包括GATA1、FLI1和MAFG。此外,在巨核细胞中鉴定出许多以前未与该谱系相关联的具有转录因子活性或转录因子结合活性的基因,包括BTEB1、NR4A2、FOXO1A、MEF2C、HDAC5、VDR,以及几个与肿瘤抑制因子p53相关的基因(HIPK2、FHL2和TADA3L)。在巨核细胞中证实了四种新型候选巨核细胞转录因子(FHL2、MXD1、E2F3和RFX5)的蛋白表达和核定位。鉴于在特定分化程序中表达的转录因子是该程序的重要贡献者这一假设,这些数据极大地扩展了我们对干细胞和祖细胞巨核细胞分化中转录调控的理解。

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