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An experimental study on astrocytes promoting production of neural stem cells derived from mouse embryonic stem cells

机译:星形胶质细胞促进小鼠胚胎干细胞来源神经干细胞产生的实验研究

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Background The production of neural stem cells ( NSCs) derived from embryonic stem ( ES) cells was usually very low according to previous studies, which was a major obstacle for meeting the needs of clinical application. This study aimed at investigating whether astrocytes could promote production of NSCs derived from ES cells in vitro. Methods Mouse ES cells line-D3 was used to differentiate into NSCs with astrocytes as inducing stromal cells by means of three-stage differentiation procedure. Another group without astrocytes served as control. The totipotency of ES cells was identified by observation of cells' morphology and formation of teratoma in severe combined immunodeficiency disease ( SCID) mice. The quantity and purity of NSCs derived from ES cells were analyzed using clonogenic assay, immunohistochemical staining and flow cytometry assay. The plasticity of NSCs was detected by differentiating test. Octamer-binding transcription factor 4 ( Oct-4) and nestin, the specific marker genes of ES cells and NSCs respectively, were detected continuously using reverse transcription-polymerase chain reaction (RT-PCR) method to monitor the process of cell differentiation. Results The ES cells of D3 line could maintain the ability of differentiating into cellular derivations of all three primary germ layers after continuous passage culture. At the end of two-stage of inducing process, 23.2 ± 3.5 neurospheres per plate formed in astrocyte-induced group and only 0. 8 ± 0.3 per plate in the control group (clonogenic assay, P <0.01) , and the ratio of nestin positive cells was (50.2 ± 2.8)% in astrocyte-induced group and only (1.4±0.5)% in the control group ( flow cytometry, P < 0. 01). With the induction undergoing, the expression of Oct-4 gradually decreased and then disappeared, while the expression of nestin was increased step by step, and the ratio of nestin positive cells was up to 91.4% by the three-stage differentiation. The nestin positive cells could be further induced into neurons, astrocytes, and oligodendrocytes in differentiating medium supplemented with fetal calf serum. The results of differentiating test showed that the ratio of NF-200 and NSE positive cells was (42.7 ± 2.6)% in astrocyte-induced group and only (11.2±1.8)% in the control group (P<0.01). Conclusions Astrocytes can not only increase the production of NSCs derived from ES cells but also promote the differentiation of NSCs toward neuronal lineage.
机译:背景技术根据先前的研究,源自胚胎干(ES)细胞的神经干细胞(NSC)的产量通常非常低,这是满足临床应用需求的主要障碍。这项研究旨在调查星形胶质细胞是否可以在体外促进源自ES细胞的NSC的产生。方法采用小鼠ES细胞系D3通过三阶段分化程序,以星形胶质细胞为基质细胞诱导分化为NSCs。另一组没有星形胶质细胞的作为对照组。通过观察严重的联合免疫缺陷病(SCID)小鼠的细胞形态和畸胎瘤的形成,可以确定ES细胞的全能性。使用克隆形成分析,免疫组织化学染色和流式细胞术分析了来自ES细胞的NSC的数量和纯度。通过分化试验检测NSC的可塑性。用逆转录-聚合酶链反应(RT-PCR)法连续检测ES细胞和NSCs的特异性标记基因Octamer-binding转录因子4(Oct-4)和巢蛋白,以监测细胞分化过程。结果连续传代培养后,D3系的ES细胞可以维持分化为所有三个主要胚层的细胞衍生能力。在诱导过程的两个阶段结束时,星形胶质细胞诱导组每块形成23.2±3.5个神经球,对照组中每块仅形成0. 8±0.3个(克隆性试验,P <0.01),巢蛋白的比例星形胶质细胞诱导组中阳性细胞为(50.2±2.8)%,而对照组中仅为(1.4±0.5)%(流式细胞仪,P <0. 01)。随着诱导的进行,Oct-4的表达逐渐降低然后消失,而巢蛋白的表达则逐步增加,通过三阶段分化,巢蛋白阳性细胞的比例高达91.4%。 Nestin阳性细胞可以在补充胎牛血清的分化培养基中进一步诱导为神经元,星形胶质细胞和少突胶质细胞。分化试验结果显示,星形胶质细胞诱导组中NF-200和NSE阳性细胞的比例为(42.7±2.6)%,而对照组仅为(11.2±1.8)%(P <0.01)。结论星形胶质细胞不仅可以增加ES细胞来源的NSCs的产生,而且可以促进NSCs向神经元谱系的分化。

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