Generation of human midbrain organoids from induced pluripotent stem cells

Nguyen-Vi Mohamed, M. Mathur, Ronan V. da Silva, Rhalena A. Thomas, Paula Lépine, L. Beitel, E. Fon, T. Durcan
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引用次数: 11

Abstract

The development of brain organoids represents a major technological advance in the stem cell field, a novel bridge between traditional 2D cultures and in vivo animal models. In particular, the development of midbrain organoids containing functional dopaminergic neurons producing neuromelanin granules, a by-product of dopamine synthesis, represents a potential new model for Parkinson’s disease. To generate human midbrain organoids, we introduce specific inductive cues, at defined timepoints, during the 3D culture process to drive the stem cells towards a midbrain fate. In this method paper, we describe a standardized protocol to generate human midbrain organoids (hMOs) from induced pluripotent stem cells (iPSCs). This protocol was developed to demonstrate how human iPSCs can be successfully differentiated into numerous, high quality midbrain organoids in one batch. We also describe adaptations for cryosectioning of fixed organoids for subsequent histological analysis.
诱导多能干细胞产生人中脑类器官
大脑类器官的开发代表了干细胞领域的一项重大技术进步,这是传统2D培养物和体内动物模型之间的一座新桥梁。特别是,含有功能性多巴胺能神经元的中脑类器官的开发,产生多巴胺合成的副产品神经松弛素颗粒,代表了帕金森病的一个潜在的新模型。为了产生人类中脑类器官,我们在3D培养过程中,在特定的时间点引入特定的诱导线索,以驱动干细胞走向中脑命运。在这篇方法论文中,我们描述了一种从诱导多能干细胞(iPSC)产生人类中脑类器官(hMO)的标准化方案。该方案旨在证明人类iPSC如何在一批中成功分化为大量高质量的中脑类器官。我们还描述了冷冻切片固定类器官用于后续组织学分析的适应性。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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