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Regulated Expression of pdx-1 Promotes In Vitro Differentiation of Insulin-Producing Cells From Embryonic Stem Cells.

机译:pdx-1的调控表达促进胰岛素产生细胞从胚胎干细胞体外分化。

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Embryonic stem (ES) cells can differentiate into many cell types. Recent reports have shown that ES cells can differentiate into insulin-producing cells. However, the differentiation is not efficient enough to produce insulin-secreting cells for future therapeutic use. Pdx-1, a homeodomain-containing transcription factor, is a crucial regulator for pancreatic development. We established an ES cell line in which exogenous pdx-1 expression was precisely regulated by the Tet-off system integrated into the ROSA26 locus. Using this cell line, we examined the effect of pdx-1 expression during in vitro differentiation via embryoid body formation. The results showed that pdx-1 expression clearly enhanced the expression of the insulin 2, somatostatin, Kir6.2, glucokinase, neurogenin3, p48, Pax6, PC2, and HNF6 genes in the resulting differentiated cells. Immunohistochemical examination also revealed that insulin was highly produced in most of the differentiated ES cells. Thus, exogenous expression of pdx-1 should provide a promising approach for efficiently producing insulin-secreting cells from human ES cells for future therapeutic use in diabetic patients.
机译:胚胎干(ES)细胞可以分化为多种细胞类型。最近的报道表明ES细胞可以分化为产生胰岛素的细胞。然而,这种分化不足以产生胰岛素分泌细胞用于将来的治疗用途。 Pdx-1,一个含同源结构域的转录因子,是胰腺发育的关键调节因子。我们建立了一个ES细胞系,其中外源pdx-1的表达受整合到ROSA26基因座中的Tet-off系统的精确调控。使用该细胞系,我们检查了通过类胚体形成的体外分化过程中pdx-1表达的影响。结果表明,pdx-1的表达明显增强了胰岛素2,生长抑素,Kir6.2,葡萄糖激酶,神经生成素3,p48,Pax6,PC2和HNF6基因的表达。免疫组织化学检查还显示,在大多数分化的ES细胞中胰岛素高产。因此,pdx-1的外源表达应提供一种有前途的方法,可有效地从人ES细胞产生胰岛素分泌细胞,以用于糖尿病患者的未来治疗。

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