首页> 外文期刊>Stem Cells >NG2 and Olig2 expression provides evidence for phenotypic deregulation of cultured central nervous system and peripheral nervous system neural precursor cells.
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NG2 and Olig2 expression provides evidence for phenotypic deregulation of cultured central nervous system and peripheral nervous system neural precursor cells.

机译:NG2和Olig2的表达为培养的中枢神经系统和周围神经系统神经前体细胞的表型失调提供了证据。

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Neural stem cells cultured with fibroblast growth factor 2 (FGF2)/epidermal growth factor (EGF) generate clonal expansions called neurospheres (NS), which are widely used for therapy in animal models. However, their cellular composition is still poorly defined. Here, we report that NS derived from several embryonic and adult central nervous system (CNS) regions are composed mainly of remarkable cells coexpressing radial glia markers (BLBP, RC2, GLAST), oligodendrogeniceurogenic factors (Mash1, Olig2, Nkx2.2), and markers that in vivo are typical of the oligodendrocyte lineage (NG2, A2B5, PDGFR-alpha). On NS differentiation, the latter remain mostly expressed in neurons, together with Olig2 and Mash1. Using cytometry, we show that in growing NS the small population of multipotential self-renewing NS-forming cells are A2B5(+) and NG2(+). Additionally, we demonstrate that these NS-forming cells in the embryonic spinal cord were initially NG2(-) and rapidly acquired NG2 in vitro. NG2 and Olig2 were foundto be rapidly induced by cell culture conditions in spinal cord neural precursor cells. Olig2 expression was also induced in astrocytes and embryonic peripheral nervous system (PNS) cells in culture after EGF/FGF treatment. These data provide new evidence for profound phenotypic modifications in CNS and PNS neural precursor cells induced by culture conditions.
机译:用成纤维细胞生长因子2(FGF2)/表皮生长因子(EGF)培养的神经干细胞可产生称为神经球(NS)的克隆扩增,已广泛用于动物模型的治疗。但是,它们的细胞组成仍然不清楚。在这里,我们报告说,来自几个胚胎和成年中枢神经系统(CNS)地区的NS主要由共同表达radial神经胶质标志物(BLBP,RC2,GLAST),少突胶质/神经形成因子(Mash1,Olig2,Nkx2.2)的显着细胞组成和在体内是少突胶质细胞谱系的典型标记(NG2,A2B5,PDGFR-alpha)。在NS分化中,后者与Olig2和Mash1一起主要在神经元中表达。使用流式细胞仪,我们显示,在正在生长的NS中,多能自我更新NS形成细胞的小群体是A2B5(+)和NG2(+)。此外,我们证明了胚胎脊髓中这些NS形成细胞最初是NG2(-),并在体外迅速获得了NG2。发现NG2和Olig2在脊髓神经前体细胞中被细胞培养条件快速诱导。 EGF / FGF处理后,在培养的星形胶质细胞和胚胎外周神经系统(PNS)细胞中也诱导了Olig2表达。这些数据为由培养条件诱导的CNS和PNS神经前体细胞的深刻表型修饰提供了新的证据。

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