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在定义明确和可扩展的培养条件下从人多能干细胞中生产和冷冻保存确定内胚层。

Production and cryopreservation of definitive endoderm from human pluripotent stem cells under defined and scalable culture conditions.

机构信息

Leibniz Research Laboratories for Biotechnology and Artificial Organs (LEBAO), REBIRTH-Research Center for Translational and Regenerative Medicine, Hannover Medical School, Hannover, Germany.

Biomedical Research in Endstage and Obstructive Lung Disease Hannover (BREATH), German Center for Lung Research (DZL), Hannover Medical School, Hannover, Germany.

出版信息

Nat Protoc. 2021 Mar;16(3):1581-1599. doi: 10.1038/s41596-020-00470-5. Epub 2021 Feb 12.

Abstract

The endodermal germ layer gives rise to respiratory epithelium, hepatocytes, pancreatic cells and intestinal lineages, among other cell types. These lineages can be differentiated from human pluripotent stem cells (hPSCs) via a common definitive endoderm (DE) intermediate that is characterized by the co-expression of the cell surface markers CXCR4, c-KIT and EPCAM and the transcription factors SOX17 and FOXA2. Here we provide a detailed protocol for mass production of DE from hPSCs in scalable and easy-to-handle suspension culture using a rotating Erlenmeyer flask or a sophisticated, fully controllable, 150-ml stirred tank bioreactor. This protocol uses two different media formulations that are chemically defined and xeno free and therefore good manufacturing practice ready. Our protocol allows for efficient hPSC-derived DE specification in multicellular aggregates within 3 days and generates up to 1 × 10 DE cells with >92% purity in one differentiation batch when using the bioreactor. The hPSC-derived DE cells that are generated can be cryopreserved for later downstream differentiation into various endodermal lineages. This protocol should facilitate the flexible production of mature DE derivatives for physiologically relevant disease models, high-throughput drug screening, toxicology testing and cellular therapies.

摘要

内胚层原基产生呼吸上皮细胞、肝细胞、胰腺细胞和肠谱系细胞等多种细胞类型。这些谱系细胞可以通过共同的限定内胚层 (DE) 中间态从人多能干细胞 (hPSC) 中分化而来,其特征是共同表达细胞表面标记物 CXCR4、c-KIT 和 EPCAM 以及转录因子 SOX17 和 FOXA2。在此,我们提供了一种详细的方案,使用旋转摇瓶或复杂的、完全可控的 150 毫升搅拌槽生物反应器,在可扩展且易于处理的悬浮培养中从 hPSC 大规模生产 DE。该方案使用了两种不同的化学定义和无动物源的培养基配方,因此具备良好的生产规范准备。我们的方案允许在 3 天内通过细胞聚集体高效地从 hPSC 中特化出 DE,并且在使用生物反应器时,每批分化可产生多达 1×10^6 的 DE 细胞,纯度超过 92%。生成的 hPSC 衍生的 DE 细胞可以冷冻保存,以备以后分化为各种内胚层谱系。该方案应有助于灵活生产成熟的 DE 衍生物,用于生理相关的疾病模型、高通量药物筛选、毒理学测试和细胞治疗。

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