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Determination of the Culture Time Point to Induce Corneal Epithelial Differentiation in Induced Pluripotent Stem Cells

机译:培养时间点诱导诱导多能干细胞中角膜上皮分化的培养时间点

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Abstract Background Limbal stem cells (LSC) are progenitor cells in the ocular surface that renew the corneal epithelium. Limbal stem cell deficiency usually induces blindness through the loss of corneal transparency, and bilateral cases do not an accurate treatment because of the lack of an autologous source of stem cells. Methods Induced pluripotent stem cells (iPSC) are promising for use in cell therapy because of their autologous origin and the capability to differentiate into corneal epithelial cells. However, there are not standardized protocols to achieve a complete corneal epithelial differentiation. We examined the expression of several markers in a human episomal iPSC line after an induction period from embryoid bodies. Results Progenitor LSC and corneal epithelial differentiation markers, some extracellular matrix protein adhesion molecules, and wingless signaling pathway were studied. Overall, LSC progenitor and corneal epithelium differentiation markers increased after maintaining cell culture in specific conditions for 14 days, whereas pluripotency markers decreased. Conclusions Our approach indicated that the optimal time point to initiate iPSC differentiation into LSC and corneal phenotypes, with the use of specific medium, is from 14 days after initial embryoid bodies treatment induction.
机译:抽象背景角膜缘干细胞(LSC)的祖细胞在眼表面更新角膜上皮。角膜缘干细胞缺乏症通常是通过角膜透明度的丧失导致失明,和双边的情况下做的,因为缺乏干细胞的自体来源的不准确的治疗。方法诱导多能干细胞(iPSC)是有希望的,因为它们自身的起源和能力分化为角膜上皮细胞用于细胞治疗。不过,也有不规范的协议,以实现完整的角膜上皮细胞分化。我们研究的几个标志物的表达在人游离iPSC系从胚状体诱导期之后。结果祖LSC和角膜上皮分化标志物,一些细胞外基质蛋白粘附分子,和无翅信号通路进行了研究。总体而言,LSC祖细胞和角膜上皮分化标记物保持在特定条件下的细胞培养14天后增加,而多能性标记降低。结论:我们的做法表明,最佳时间点启动iPSC细胞分化为LSC和角膜表型,使用特定的介质,是从最初的胚状体诱导治疗后14天。

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