Generation of insulin-producing pancreatic β cells from multiple human stem cell lines

PDX1型 干细胞 细胞生物学 维甲酸 细胞分化 细胞培养 祖细胞 胰岛素 小岛 生物 定向微分 诱导多能干细胞 化学 胚胎干细胞 内分泌学 生物化学 遗传学 基因
作者
Nathaniel J. Hogrebe,Kristina G. Maxwell,Punn Augsornworawat,Jeffrey R. Millman
出处
期刊:Nature Protocols [Nature Portfolio]
卷期号:16 (9): 4109-4143 被引量:192
标识
DOI:10.1038/s41596-021-00560-y
摘要

We detail a six-stage planar differentiation methodology for generating human pluripotent stem cell–derived pancreatic β cells (SC-β cells) that secrete high amounts of insulin in response to glucose stimulation. This protocol first induces definitive endoderm by treatment with Activin A and CHIR99021, then generates PDX1+/NKX6-1+ pancreatic progenitors through the timed application of keratinocyte growth factor, SANT1, TPPB, LDN193189 and retinoic acid. Endocrine induction and subsequent SC-β-cell specification is achieved with a cocktail consisting of the cytoskeletal depolymerizing compound latrunculin A combined with XXI, T3, ALK5 inhibitor II, SANT1 and retinoic acid. The resulting SC-β cells and other endocrine cell types can then be aggregated into islet-like clusters for analysis and transplantation. This differentiation methodology takes ~34 d to generate functional SC-β cells, plus an additional 1–2 weeks for initial stem cell expansion and final cell assessment. This protocol builds upon a large body of previous work for generating β-like cells. In this iteration, we have eliminated the need for 3D culture during endocrine induction, allowing for the generation of highly functional SC-β cells to be done entirely on tissue culture polystyrene. This change simplifies the differentiation methodology, requiring only basic stem cell culture experience as well as familiarity with assessment techniques common in biology laboratories. In addition to expanding protocol accessibility and simplifying SC-β-cell generation, we demonstrate that this planar methodology is amenable for differentiating SC-β cells from a wide variety of cell lines from various sources, broadening its applicability. Millman and colleagues describe a six-stage monolayer culture differentiation protocol for generating insulin-secreting pancreatic β cells from a variety of human pluripotent stem cell lines and outline steps for in vitro functional assessment.
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