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人胎儿脊髓干细胞系 NSI-566RSC 的鉴定及其向功能性运动神经元的诱导分化。

Characterization of a human fetal spinal cord stem cell line, NSI-566RSC, and its induction to functional motoneurons.

机构信息

NanoScience Technology Center, University of Central Florida, Orlando, FL 32826, USA.

出版信息

J Tissue Eng Regen Med. 2010 Mar;4(3):181-93. doi: 10.1002/term.223.

Abstract

Specific neuronal subtypes, especially motoneurons (MNs), derived from human stem cells provide a significant therapeutic potential for spinal cord diseases, such as amyotrophic lateral sclerosis (ALS) and spinal cord injury. So far, in vitro, MNs have only been successfully induced from embryonic stem cells (hESC) and human fetal cortical progenitors. Although neural progenitors from spinal cord would be a likely source for generating MNs, there has been no study reporting successful in vitro differentiation of MNs from spinal cord progenitors. This study first characterized a polyclonal spinal cord stem cell line isolated from an 8 week-old fetus. Then a paradigm was introduced to successfully induce MNs from this cell line, which was demonstrated by immunostaining using the MN markers HB9, Islet1 and choline acetyl transferase (ChAT). The combination of HB9 and ChAT immunostainings indicated that approximately 20% of the cells were MNs after this induction protocol. The presence of other cell types in the differentiated culture was also analysed. Finally, the electrophysiological properties of these differentiated MNs were characterized to confirm their functional integrity. The majority of these MNs fired repetitive action potentials (APs), which is an indicator of functional maturation. The recordings of spontaneous excitatory postsynaptic currents (EPSCs) confirmed the formation of synapses onto these MNs. This study reports the first successful differentiation of MNs from human spinal cord stem cells in vitro, providing a novel approach for obtaining functional MNs when designing the therapeutic strategy for spinal cord diseases or injuries.

摘要

特定的神经元亚型,尤其是运动神经元(MNs),来源于人类干细胞,为脊髓疾病(如肌萎缩侧索硬化症和脊髓损伤)提供了重要的治疗潜力。到目前为止,体外只能成功地从胚胎干细胞(hESC)和人胎儿皮质祖细胞中诱导 MNs。尽管来自脊髓的神经前体细胞可能是生成 MNs 的一个潜在来源,但目前还没有研究报告从脊髓祖细胞成功体外分化出 MNs。本研究首先对从小鼠胚胎 8 周龄胎儿中分离得到的多能脊髓干细胞系进行了鉴定。然后引入了一种方案,成功地从该细胞系中诱导出 MNs,通过 MN 标志物 HB9、Islet1 和胆碱乙酰转移酶(ChAT)的免疫染色进行了验证。经过诱导后,HB9 和 ChAT 免疫染色的组合表明,约有 20%的细胞是 MNs。分化培养物中其他细胞类型的存在也进行了分析。最后,对这些分化的 MNs 的电生理特性进行了表征,以确认其功能完整性。这些 MNs 中的大多数都能发出重复的动作电位(APs),这是功能成熟的一个指标。自发兴奋性突触后电流(EPSCs)的记录证实了这些 MNs 上形成了突触。本研究首次报道了体外从小鼠脊髓干细胞中成功分化出 MNs,为设计脊髓疾病或损伤的治疗策略时获得功能性 MNs 提供了一种新方法。

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