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Pdx1和Foxa2过表达对人胚胎干细胞分化为胰腺细胞的影响。

The effect of overexpression of Pdx1 and Foxa2 on the differentiation of human embryonic stem cells into pancreatic cells.

作者信息

Lavon Neta, Yanuka Ofra, Benvenisty Nissim

机构信息

Department of Genetics, The Hebrew University, Jerusalem 91904, Israel.

出版信息

Stem Cells. 2006 Aug;24(8):1923-30. doi: 10.1634/stemcells.2005-0397. Epub 2006 May 4.

DOI:10.1634/stemcells.2005-0397
PMID:16675598
Abstract

Human embryonic stem cells (HESCs) are pluripotent cells that may serve as a source of cells for transplantation medicine and as a tool to study human embryogenesis. Using genetic manipulation methodologies, we have investigated the potential of HESCs to differentiate into the various pancreatic cell types. We initially created various HESCs carrying the enhanced green fluorescent protein (eGFP) reporter gene under the control of either the insulin promoter or the pancreatic and duodenal homeobox factor-1 (Pdx1) promoter. Our analysis revealed that during the differentiation of HESCs into embryoid bodies (EBs), we could detect green fluorescent cells when eGFP is regulated by Pdx1 promoter but not by insulin promoter. To examine whether we can induce differentiation into pancreatic cells, we have established human embryonic stem cell lines that constitutively express either Pdx1 or the endodermal transcription factor Foxa2. Following differentiation into EBs, the constitutive expression of Pdx1 enhanced the differentiation of HESCs toward pancreatic endocrine and exocrine cell types. Thus, we have demonstrated expression of several transcription factors that are downstream of Pdx1 and various molecular markers for the different pancreatic cell types. However, the expression of the insulin gene could be demonstrated only when the cells differentiated in vivo into teratomas. We conclude that although overexpression of Pdx1 enhanced expression of pancreatic enriched genes, induction of insulin expression may require additional signals that are only present in vivo.

摘要

人类胚胎干细胞(HESCs)是多能干细胞,可作为移植医学的细胞来源以及研究人类胚胎发育的工具。利用基因操作方法,我们研究了HESCs分化为各种胰腺细胞类型的潜力。我们最初创建了各种携带增强型绿色荧光蛋白(eGFP)报告基因的HESCs,该基因受胰岛素启动子或胰腺十二指肠同源盒因子-1(Pdx1)启动子的控制。我们的分析表明,在HESCs分化为胚状体(EBs)的过程中,当eGFP受Pdx1启动子调控时,我们可以检测到绿色荧光细胞,而受胰岛素启动子调控时则检测不到。为了研究我们是否能够诱导其分化为胰腺细胞,我们建立了组成性表达Pdx1或内胚层转录因子Foxa2的人类胚胎干细胞系。在分化为EBs后,Pdx1的组成性表达增强了HESCs向胰腺内分泌和外分泌细胞类型的分化。因此,我们证明了几种Pdx1下游转录因子以及不同胰腺细胞类型的各种分子标志物的表达。然而,只有当细胞在体内分化为畸胎瘤时才能证明胰岛素基因的表达。我们得出结论,虽然Pdx1的过表达增强了胰腺富集基因的表达,但胰岛素表达的诱导可能需要仅在体内存在的其他信号。

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