| 人胚不同脑区神经前体细胞的分离培养及分化特性的比较 |
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| 引用本文: | 桂伶俐,刘志恒,张传汉,祝畅,高峰.人胚不同脑区神经前体细胞的分离培养及分化特性的比较[J].中国组织化学与细胞化学杂志,2007,16(2):129-133. |
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| 作者姓名: | 桂伶俐 刘志恒 张传汉 祝畅 高峰 |
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| 作者单位: | 1. 华中科技大学同济医学院附属同济医院麻醉学教研室,武汉,430030
2. 华中科技大学同济医学院附属同济医院麻醉学教研室,武汉,430030;深圳市第二人民医院麻醉科,深圳,518035 |
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| 摘 要: | 目的研究人胚不同脑区神经前体细胞(neural progenitor cells,NPCs)培养及增殖分化特性。方法取14-17周人胚脑区组织,分为新皮质、纹状体、间脑、中脑、后脑和延髓组,悬浮培养。鉴定细胞球巢蛋白抗原的表达,分化及自我更新能力。观察各脑区培养细胞的生长、增殖状况。新皮质、纹状体及间脑来源的神经球分化后,运用免疫荧光细胞化学法比较神经元及星形胶质细胞的比例。结果各脑区培养出的悬浮细胞球巢蛋白抗原阳性,可分化为MAP2或GFAP阳性细胞,且BrdU掺入实验阳性。体外培养第3d,纹状体及间脑组均可见大量神经球,且纹状体组明显多于间脑组;新皮质组传代后可见较多神经球;其它组仅见个别神经球。新皮质、纹状体、间脑来源的NPCs诱导分化后,MAP2或GFAP阳性细胞率各组间比较差异无显著性。结论人胚不同脑区均可培养出NPCs,从易到难依次为纹状体、间脑、新皮质及其它脑区。新皮质、纹状体、间脑来源的NPCs体外分化比例一致。
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| 关 键 词: | 细胞培养 神经前体细胞 细胞分化 空间特异性 |
| 修稿时间: | 2006-08-25 |
COMPARATIVE STUDY IN VITRO ON THE CULTURE, PROLIFERATION AND DIFFERENTIATION CHARACTERISTICS OF HUMAN NEURAL PROGENITOR CELLS DERIVED FROM DIFFERENT EMBRYONIC BRAIN REGIONS |
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| Gui Lingli,Liu Zhiheng,Zhang Chuanhan,Zhu Chang,Gao Feng.COMPARATIVE STUDY IN VITRO ON THE CULTURE, PROLIFERATION AND DIFFERENTIATION CHARACTERISTICS OF HUMAN NEURAL PROGENITOR CELLS DERIVED FROM DIFFERENT EMBRYONIC BRAIN REGIONS[J].Chinese Journal of Histochemistry and Cytochemistry,2007,16(2):129-133. |
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| Authors: | Gui Lingli Liu Zhiheng Zhang Chuanhan Zhu Chang Gao Feng |
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| Abstract: | Objective To investigate the culture,proliferation and differentiation of humanneural progenitor cells derived from different embryonic brain regions.Methods The free-floating cells of neocortex,striatum,diencephalon,mesencephalon,metencephalon and myelencephalon from 14-17-week embryonic brains were cultured.The expressionof nestin,self-renewal and multipotential property of the cell clusters were examinated.The growth and proliferation of the cells isolated from different brain regions were analysed.After the neurospheres from neocortex,striatumand diencephalonwere induced,the percentage of neurons or astrocytes was investigatedby immunocytochemical staining.Results Nestin and Brdu immunochemical staining was positive in the cell aggregations derived from different brain regions,and all of them could differentiate into MAP2 or GFAP positive cells.On day 3 of culture,many neurospheres were formed in diencephalonand striatum groups,but more in striatum.By contrast,much less neurospheres were formed in neocortex,and only few in other groups.After differentiation of neural progenitor cells from neocortex,striatum and diencephalon,the percentage of MAP2 or GFAP positive cells did not show significant difference among the groups.Conclusion In vitro,neural progenitor cells can be isolated from different embryonic brain regions.The rate of neurosphere formation is higher in striatumthan in diencephalon,neocortex and other regions.Under the same culture conditions,the percentage of differentiated cells does not show difference in the neural progenitor cells from striatum,diencephalon and neocortex. |
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| Keywords: | Cells Cultured Neural progenitor cell Cell differentiation Region-specificity |
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