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首页> 外文期刊>Stem cell reviews and Reports >A Critical Re-Evaluation of CD24-Positivity of Human Embryonic Stem Cells Differentiated into Pancreatic Progenitors
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A Critical Re-Evaluation of CD24-Positivity of Human Embryonic Stem Cells Differentiated into Pancreatic Progenitors

机译:关键的重新评估人类胚胎干细胞分化成胰腺祖细胞的CD24阳性。

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Differentiation of embryonic stem cells (ESCs) into insulin-producing cells for cell replacement therapy of diabetes mellitus comprises the stepwise recapitulation of in vivo developmental stages of pancreatic organogenesis in an in vitro differentiation protocol. The chemical compounds IDE-1 and (-)-indolactam-V can be used to direct mouse and human ESCs through these stages to form definitive endoderm via an intermediate mesendodermal stage and finally into pancreatic endoderm. Cells of the pancreatic endoderm express the PDX1 transcription factor and contribute to all pancreatic cell types upon further in vitro or in vivo differentiation. Even though this differentiation approach is highly effective and reproducible, it generates heterogeneous populations containing PDX1-expressing pancreatic progenitors amongst other cell types. Thus, a technique to separate PDX1-expressing cells from this mixture is very desirable. Recently it has been reported that PDX1-positive pancreatic progenitors, derived from human embryonic stem cells, express the surface marker CD24. Therefore were subjected mouse and human ESCs to a small molecule differentiation approach and the expression of the surface marker CD24 was monitored in undifferentiated cells, cells committed to the definitive endoderm and cells reminiscent of the pancreatic endoderm. We observed that both mouse and human ESCs expressed CD24 in the pluripotent state, during the whole process of endoderm formation and upon further differentiation towards pancreatic endoderm. Thus CD24 is not a suitable cell surface marker for identification of PDX1-positive progenitor cells.
机译:胚胎干细胞(ESC)分化为胰岛素生成细胞以用于糖尿病的细胞替代治疗,包括体外分化方案中胰腺器官发生的体内发育阶段的逐步概括。化合物IDE-1和(-)-吲哚内酰胺-V可用于指导小鼠和人类ESC通过这些阶段,通过中间的中胚层阶段形成定形内胚层,最后进入胰腺内胚层。胰腺内胚层的细胞表达PDX1转录因子,并在进一步体外或体内分化后对所有胰腺细胞类型有所贡献。即使这种分化方法非常有效且可重现,它仍会产生异种群体,其中包括表达PDX1的胰腺祖细胞以及其他细胞类型。因此,非常需要从该混合物中分离表达PDX1的细胞。最近,据报道,源自人类胚胎干细胞的PDX1阳性胰腺祖细胞表达表面标记CD24。因此,对小鼠和人类ESC进行了小分子分化方法,并在未分化细胞,定形内胚层细胞和胰内胚层细胞中监测了表面标记CD24的表达。我们观察到,在内胚层形成的整个过程中以及在进一步分化为胰腺内胚层的过程中,小鼠和人类ESC都以多能状态表达CD24。因此,CD24不是用于鉴定PDX1阳性祖细胞的合适细胞表面标记。

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