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在 3%氧气条件下,从 hESCs 高效诱导 NPCs、脊髓运动神经元和中脑多巴胺能神经元。

Efficient derivation of NPCs, spinal motor neurons and midbrain dopaminergic neurons from hESCs at 3% oxygen.

机构信息

Department of Clinical Neurosciences, University of Cambridge, Cambridge, UK.

出版信息

Nat Protoc. 2011 Jul 28;6(8):1229-40. doi: 10.1038/nprot.2011.380.

Abstract

This protocol has been designed to generate neural precursor cells (NPCs) from human embryonic stem cells (hESCs) using a physiological oxygen (O(2)) level of 3% (previously termed hypoxia) and chemically defined conditions. The first stage involves suspension culture of hESC colonies at 3% O(2), where they acquire a neuroepithelial identity over a period of 2 weeks. This timescale is comparable to that observed at 20% O(2), but survival is enhanced. Sequential application of retinoic acid and purmorphamine (PM), from day 14 to day 28, directs differentiation toward spinal motor neurons. Alternatively, addition of fibroblast growth factor-8 and PM generates midbrain dopaminergic neurons. OLIG2 (encoding oligodendrocyte lineage transcription factor 2) induction in motor neuron precursors is twofold greater than that at 20% O(2), whereas EN1 (encoding engrailed homeobox 1) expression is enhanced fivefold. NPCs (at 3% O(2)) can be differentiated into all three neural lineages, and such cultures can be maintained long term in the absence of neurotrophins. The ability to generate defined cell types at 3% O(2) should represent a significant advancement for in vitro disease modeling and potentially for cell-based therapies.

摘要

本方案旨在使用 3%(先前称为低氧)的生理氧(O(2))水平和化学定义的条件,从人胚胎干细胞(hESC)中生成神经前体细胞(NPC)。第一阶段涉及将 hESC 集落在 3%O(2)下进行悬浮培养,在此期间,它们在两周的时间内获得神经上皮特性。这个时间尺度与在 20%O(2)下观察到的时间尺度相当,但存活率得到提高。从第 14 天到第 28 天,连续应用视黄酸和 purmorphamine(PM)将分化方向引导为脊髓运动神经元。或者,添加成纤维细胞生长因子-8 和 PM 可生成中脑细胞多巴胺能神经元。在运动神经元前体中 OLIG2(编码少突胶质细胞谱系转录因子 2)的诱导是在 20%O(2)下的两倍,而 EN1(编码 engrailed homeobox 1)的表达增强了五倍。NPC(在 3%O(2)下)可以分化为所有三种神经谱系,并且在没有神经营养因子的情况下可以长期维持这种培养物。在 3%O(2)下生成定义明确的细胞类型的能力应该代表体外疾病建模的重大进展,并且可能代表细胞为基础的治疗的重大进展。

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