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Coordinated generation of multiple ocular-like cell lineages and fabrication of functional corneal epithelial cell sheets from human iPS cells

外胚层 生物 细胞生物学 诱导多能干细胞 干细胞 6号乘客 移植 神经外胚层 人口 祖细胞 胚胎干细胞 解剖 中胚层 胚胎发生 医学 胚胎 遗传学 环境卫生 基因 转录因子 外科
作者
Ryuhei Hayashi,Yuki Ishikawa,Ryousuke Katori,Yuzuru Sasamoto,Yuki Taniwaki,Hiroshi Takayanagi,Motokazu Tsujikawa,Kiyotoshi Sekiguchi,Andrew J. Quantock,Kohji Nishida
出处
期刊:Nature Protocols [Springer Nature]
卷期号:12 (4): 683-696 被引量:109
标识
DOI:10.1038/nprot.2017.007
摘要

This protocol describes how to grow a functional and transplantable corneal epithelium and how to generate ocular-like cell lineages resembling neuroectoderm, neural crest, ocular-surface ectoderm, or surface ectoderm derived from human iPS cells. We describe a protocol for the generation of a functional and transplantable corneal epithelium derived from human induced pluripotent stem (iPS) cells. When this protocol is followed, a proportion of iPS cells spontaneously form circular colonies, each of which is composed of four concentric zones. Cells in these zones have different morphologies and immunostaining characteristics, resembling neuroectoderm, neural crest, ocular-surface ectoderm, or surface ectoderm. We have named this 2D colony a 'SEAM' (self-formed ectodermal autonomous multizone), and previously demonstrated that cells within the SEAM have the potential to give rise to anlages of different ocular lineages, including retinal cells, lens cells, and ocular-surface ectoderm. To investigate the translational potential of the SEAM, cells within it that resemble ocular-surface epithelia can be isolated by pipetting and FACS sorting into a population of corneal epithelial-like progenitor cells. These can be expanded and differentiated to form an epithelial layer expressing K12 and PAX6, and able to recover function in an animal model of corneal epithelial dysfunction after surgical transplantation. The whole protocol, encompassing human iPS cell preparation, autonomous differentiation, purification, and subsequent differentiation, takes between 100 and 120 d, and is of potential use to researchers with an interest in eye development and/or ocular-surface regeneration. Experience with human iPS cell culture and sorting via FACS will be of benefit for researchers performing this protocol.
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