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分离小鼠胰腺胰岛 Procr 祖细胞并在体外长期扩增胰岛类器官。

Isolation of mouse pancreatic islet Procr progenitors and long-term expansion of islet organoids in vitro.

机构信息

State Key Laboratory of Cell Biology, CAS Center for Excellence in Molecular Cell Science, Institute of Biochemistry and Cell Biology, University of Chinese Academy of Sciences, Chinese Academy of Sciences, Shanghai, China.

Hubrecht Institute and Oncode Institute, Royal Netherlands Academy of Arts and Sciences (KNAW) and University Medical Centre Utrecht, Netherlands, Utrecht University and Princess Maxima Center, Utrecht, Netherlands.

出版信息

Nat Protoc. 2022 May;17(5):1359-1384. doi: 10.1038/s41596-022-00683-w. Epub 2022 Apr 8.

Abstract

Insulin production is required for glucose homeostasis. Pancreatic islet β cells are the only cells that produce insulin in humans; however, generation of functional β cells in vitro from embryonic or adult tissues has been challenging. Here, we describe isolation of pancreatic islet progenitors from adult mice, which enables the efficient generation and long-term expansion of functional islet organoids in vitro. This protocol starts with purification of protein C receptor (Procr)-expressing islet progenitors. Coculture with endothelial cells generates islet organoids in vitro that can be expanded by passage. Functional maturation is achieved as a consequence of a prolonged culture period and cyclic glucose stimulation. Primary islet organoids form in 7-10 days. Subsequently, each passage takes 1 week, with the final maturation step requiring 3 weeks of additional culture. The resulting organoids are predominantly composed of β cells but also contain small proportions of α, δ and pancreatic polypeptide cells. The organoids sense glucose and secrete insulin. This approach thus provides a strategy for β cell generation in vitro and an organoid system to study islet regeneration and diseases.

摘要

胰岛素的产生是葡萄糖稳态所必需的。人胰腺胰岛β细胞是唯一产生胰岛素的细胞;然而,从胚胎或成体组织体外生成功能性β细胞一直具有挑战性。在这里,我们描述了从成年小鼠中分离胰岛前体细胞,这使得能够在体外高效地生成和长期扩增功能性胰岛类器官。该方案从纯化表达蛋白 C 受体(Procr)的胰岛前体细胞开始。与内皮细胞共培养可在体外生成胰岛类器官,通过传代进行扩增。经过长时间的培养和周期性的葡萄糖刺激,实现了功能成熟。原代胰岛类器官在 7-10 天内形成。随后,每个传代需要 1 周,最后的成熟步骤需要再培养 3 周。所得的类器官主要由β细胞组成,但也含有少量的α、δ和胰多肽细胞。类器官能够感知葡萄糖并分泌胰岛素。因此,该方法为体外β细胞生成提供了一种策略,并为胰岛再生和疾病的研究提供了一种类器官系统。

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