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New methods for inducing the differentiation of amniotic-derived mesenchymal stem cells into motor neuron precursor cells

机译:诱导羊膜间充质干细胞向运动神经元前体细胞分化的新方法

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Our study investigates the differentiation of amniotic-derived mesenchymal stem cells (ADMSCs) into motor neuron (MN) precursor cells induced by a combination of extracellular matrix (ECM) and multi-cell factors. Membrane-like ECM was made by an enzymatic and chemical extraction method and exhibited good biological compatibility. Cells in the experimental group (EG) were treated with ECM and multi-cell factors in a multi-step induction process, while the control group (CG) was treated similarly, except without ECM. In the EG, after induction, the cells formed processes that connected with neighboring cells to form a net that had directionality. In these cells, neuron-specific enolase (NSE) and synaptophysin (SYN) expression levels increased and glial fibrillary acidic protein (GFAP) expression decreased. The SYN expression in the EG cells was higher compared with those in the CG. In the CG, NSE expression increased, while the expression of Nestin and SYN did not change. These were several changes in the levels of other genes: ADMSCs at passage 1 expressed Nanog, SOX2, octamer-binding transcription factor 4 (OCT4) and Nestin. In the EG, at the beginning of induction, the expression of Nanog decreased and that of SOX2 and Nestin increased. After 2 days, the cells expressed Nestin, OCT4 and SYNIII, and after 3 days, they expressed Olig2, OCT4, Nestin, SYNII and Islet1 (ISL1). Finally, at day 6, the cells expressed Nestin, SYNI, SYNIII, ISL-1, homeobox 9 (Hb9) and oligodendrocyte lineage transcription factor 2 (Olig2). In the CG, the cells never expressed SYNI, SYNII or Hb9. Our studies therefore demonstrate that the extracted ECM was capable of promoting the maturation of synapses. Human ADMSCs are composed of multiple cell subsets, including neural progenitor cells. The multi-step induction method used in this study causes human ADMSCs to differentiate into MN precursor cells
机译:我们的研究调查了羊水来源的间充质干细胞(ADMSCs)向细胞外基质(ECM)和多细胞因子的组合诱导的运动神经元(MN)前体细胞的分化。膜状ECM采用酶法和化学萃取法制备,具有良好的生物相容性。实验组(EG)中的细胞在多步诱导过程中用ECM和多细胞因子处理,而对照组(CG)的处理类似,除了没有ECM以外。在EG中,诱导后,细胞形成与相邻细胞连接的过程,形成具有方向性的网。在这些细胞中,神经元特异性烯醇化酶(NSE)和突触素(SYN)的表达水平增加,而神经胶质纤维酸性蛋白(GFAP)的表达减少。 EG细胞中的SYN表达高于CG细胞中的SYN表达。在CG中,NSE表达增加,而Nestin和SYN的表达未改变。这些是其他基因水平的一些变化:第1代的ADMSC表达了Nanog,SOX2,八聚体结合转录因子4(OCT4)和Nestin。在EG中,在诱导开始时,Nanog的表达降低,而SOX2和Nestin的表达增加。 2天后,细胞表达Nestin,OCT4和SYNIII,三天后,它们表达Olig2,OCT4,Nestin,SYNII和Islet1(ISL1)。最后,在第6天,细胞表达Nestin,SYNI,SYNIII,ISL-1,同源盒9(Hb9)和少突胶质细胞谱系转录因子2(Olig2)。在CG中,细胞从不表达SYNI,SYNII或Hb9。因此,我们的研究表明,提取的ECM能够促进突触的成熟。人的ADMSC由多个细胞亚群组成,包括神经祖细胞。本研究中使用的多步诱导方法使人ADMSC分化为MN前体细胞

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