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体外培养和扩增人角膜缘上皮细胞。

In vitro culture and expansion of human limbal epithelial cells.

机构信息

Sudhakar and Sreekanth Ravi Stem Cell Biology Laboratory, L.V. Prasad Eye Institute, Hyderabad, India.

出版信息

Nat Protoc. 2010 Aug;5(8):1470-9. doi: 10.1038/nprot.2010.115. Epub 2010 Jul 29.

Abstract

Limbal stem cells (LSCs) have an important role in the maintenance of the corneal surface epithelium, and autologous cultured limbal epithelial cell transplantations have contributed substantially to the treatment of the visually disabling condition known as LSC deficiency. In this protocol, we describe a method of establishing human limbal epithelial cell cultures by a feeder-free explant culture technique using a small limbal biopsy specimen and human amniotic membrane (hAM) as the culture substrate. This protocol is free of animal-derived products and involves the use of human recombinant growth factors. In addition, the recombinant cell dissociation enzyme TrypLE is used to replace trypsin and autologous serum replaces FBS. It takes approximately 2 weeks to establish a confluent monolayer from which approximately 3 x 10(6) cells can be harvested. This procedure can be adopted for both basic research purposes and clinical applications.

摘要

角膜缘干细胞(LSCs)在维持角膜表面上皮中起着重要作用,自体培养的角膜缘上皮细胞移植为治疗称为 LSC 缺陷的致盲疾病做出了巨大贡献。在本方案中,我们描述了一种使用小的角膜缘活检标本和人羊膜(hAM)作为培养底物的无饲养细胞外植体培养技术来建立人角膜缘上皮细胞培养物的方法。该方案不含动物源性产品,并使用人重组生长因子。此外,重组细胞解离酶 TrypLE 用于替代胰蛋白酶,自体血清替代 FBS。从大约 3 x 10(6)个细胞中可以收获建立一个融合的单层大约需要 2 周的时间。该程序可用于基础研究和临床应用。

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