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Tbx1 调节小鼠诱导多能干细胞的内胚层和中胚层分化。

Tbx1 modulates endodermal and mesodermal differentiation from mouse induced pluripotent stem cells.

机构信息

1 Department of Allied Health Sciences, University of Connecticut , Storrs, Connecticut.

出版信息

Stem Cells Dev. 2014 Jul 1;23(13):1491-500. doi: 10.1089/scd.2013.0488. Epub 2014 Apr 2.

Abstract

The T-box transcriptional factor (Tbx) family of transcriptional factors has distinct roles in a wide range of embryonic differentiation or response pathways. Tbx1, a T-box transcription factor, is an important gene for the human congenital disorder 22q11.2 deletion syndrome. Induced pluripotent stem cell (iPSC) technology offers new opportunities for both elucidation of the pathogenesis of diseases and the development of stem-cell-based therapies. In this study, we generated iPSCs from Tbx1(-/-) and Tbx1(+/+) fibroblasts and investigated the spontaneous differentiation potential of iPSCs by detailed lineage analysis of the iPSC-derived embryoid bodies. Undifferentiated Tbx1(-/-) and Tbx1(+/+) iPSCs showed similar expression levels of pluripotent markers. The ability of the Tbx1(-/-) iPSCs to generate endodermal and mesodermal lineages was compromised upon spontaneous differentiation into embryonic bodies. Restoration of Tbx1 expression in the Tbx1(-/-) iPSCs to normal levels using an inducible lentiviral system rescued these cells from the potential of defective differentiation. Interestingly, overexpression of Tbx1 in the Tbx1(-/-) iPSCs to higher levels than in the Tbx1(+/+) iPSCs again led to a defective differentiation potential. Additionally, we observed that expression of fibroblast growth factor (FGF) 10 and FGF8 was downregulated in the Tbx1(-/-) iPSC-derived cells, which suggests that Tbx1 regulates the expression of FGFs. Taken together, our results implicated the Tbx1 level as an important determinant of endodermal and mesodermal lineage differentiation during embryonic development.

摘要

T 盒转录因子(Tbx)家族转录因子在广泛的胚胎分化或反应途径中具有独特的作用。Tbx1 是 T 盒转录因子,是人类先天性 22q11.2 缺失综合征的重要基因。诱导多能干细胞(iPSC)技术为阐明疾病的发病机制和开发基于干细胞的治疗方法提供了新的机会。在这项研究中,我们从 Tbx1(-/-)和 Tbx1(+/+)成纤维细胞中生成 iPSC,并通过详细的 iPSC 衍生胚状体谱系分析研究 iPSC 的自发分化潜能。未分化的 Tbx1(-/-)和 Tbx1(+/+)iPSC 表现出相似的多能标记物表达水平。在自发分化为胚状体时,Tbx1(-/-)iPSC 生成内胚层和中胚层谱系的能力受损。使用诱导性慢病毒系统将 Tbx1 表达恢复到正常水平,挽救了 Tbx1(-/-)iPSC 从潜在的分化缺陷中恢复过来。有趣的是,在 Tbx1(-/-)iPSC 中过度表达 Tbx1 使其表达水平高于 Tbx1(+/+)iPSC,再次导致分化潜能缺陷。此外,我们观察到 Tbx1(-/-)iPSC 衍生细胞中成纤维细胞生长因子(FGF)10 和 FGF8 的表达下调,这表明 Tbx1 调节 FGFs 的表达。总之,我们的结果表明 Tbx1 水平是胚胎发育过程中内胚层和中胚层谱系分化的重要决定因素。

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