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对发育中的人类红系祖细胞进行转录调控网络分析,揭示了共调控模式和潜在的转录调节因子。

Transcriptional regulatory network analysis of developing human erythroid progenitors reveals patterns of coregulation and potential transcriptional regulators.

作者信息

Keller M A, Addya S, Vadigepalli R, Banini B, Delgrosso K, Huang H, Surrey S

机构信息

Cardeza Foundation of Hematologic Research, Jefferson Medical College, Philadelphia, Pennsylvania 19107, USA.

出版信息

Physiol Genomics. 2006 Dec 13;28(1):114-28. doi: 10.1152/physiolgenomics.00055.2006. Epub 2006 Aug 29.

DOI:10.1152/physiolgenomics.00055.2006
PMID:16940433
Abstract

Deciphering the molecular basis for human erythropoiesis should yield information benefiting studies of the hemoglobinopathies and other erythroid disorders. We used an in vitro erythroid differentiation system to study the developing red blood cell transcriptome derived from adult CD34+ hematopoietic progenitor cells. mRNA expression profiling was used to characterize developing erythroid cells at six time points during differentiation (days 1, 3, 5, 7, 9, and 11). Eleven thousand seven hundred sixty-three genes (20,963 Affymetrix probe sets) were expressed on day 1, and 1,504 genes, represented by 1,953 probe sets, were differentially expressed (DE) with 537 upregulated and 969 downregulated. A subset of the DE genes was validated using real-time RT-PCR. The DE probe sets were subjected to a cluster metric and could be divided into two, three, four, five, or six clusters of genes with different expression patterns in each cluster. Genes in these clusters were examined for shared transcription factor binding sites (TFBS) in their promoters by comparing enrichment of each TFBS relative to a reference set using transcriptional regulatory network analysis. The sets of TFBS enriched in genes up- and downregulated during erythropoiesis were distinct. This analysis identified transcriptional regulators critical to erythroid development, factors recently found to play a role, as well as a new list of potential candidates, including Evi-1, a potential silencer of genes upregulated during erythropoiesis. Thus this transcriptional regulatory network analysis has yielded a focused set of factors and their target genes whose role in differentiation of the hematopoietic stem cell into distinct blood cell lineages can be elucidated.

摘要

破解人类红细胞生成的分子基础应能产生有助于血红蛋白病和其他红系疾病研究的信息。我们使用体外红系分化系统来研究源自成人CD34+造血祖细胞的发育中红细胞转录组。mRNA表达谱用于在分化的六个时间点(第1、3、5、7、9和11天)表征发育中的红系细胞。第1天有11763个基因(20963个Affymetrix探针集)表达,1504个基因(由1953个探针集代表)差异表达(DE),其中537个上调,969个下调。使用实时RT-PCR对一部分DE基因进行了验证。对DE探针集进行聚类度量,可分为两、三、四、五或六个基因簇,每个簇具有不同的表达模式。通过使用转录调控网络分析比较每个转录因子结合位点(TFBS)相对于参考集的富集情况,检查这些簇中的基因在其启动子中的共享TFBS。在红细胞生成过程中上调和下调的基因中富集的TFBS集是不同的。该分析确定了对红系发育至关重要的转录调节因子、最近发现起作用的因子以及一系列新的潜在候选因子,包括Evi-1,它可能是红细胞生成过程中上调基因的沉默子。因此,这种转录调控网络分析产生了一组重点关注的因子及其靶基因,其在造血干细胞分化为不同血细胞谱系中的作用可以得到阐明。

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