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评估人胚胎干细胞生成多巴胺能神经元过程中基质衍生诱导活性。

Assessment of stromal-derived inducing activity in the generation of dopaminergic neurons from human embryonic stem cells.

作者信息

Vazin Tandis, Chen Jia, Lee Chun-Ting, Amable Rose, Freed William J

机构信息

Department of Health and Human Services, Cellular Neurobiology Research Branch, Intramural Research Program, National Institute on Drug Abuse, National Institutes of Health, Baltimore, Maryland 21224, USA.

出版信息

Stem Cells. 2008 Jun;26(6):1517-25. doi: 10.1634/stemcells.2008-0039. Epub 2008 Apr 3.

Abstract

Producing dopaminergic (DA) neurons is a major goal of human embryonic stem cell (hESC) research. DA neurons can be differentiated from hESC by coculture with the mouse PA6 stromal cell line; this differentiation-inducing effect is termed stromal-derived inducing activity (SDIA). The molecular and biochemical nature of SDIA is, however, unknown. Various studies have suggested that SDIA involves either a fixation-resistant component located on the PA6 cell surface or factors secreted into the medium by PA6 cells. To address this question, hESC were cocultured with PA6 cells for 12 days and then further differentiated with sonic hedgehog homolog, fibroblast growth factor-8, and glial cell line-derived neurotrophic factor. After 18 days, 34% of cells were tyrosine hydroxylase (TH)+. When PA6 cells were fixed or irradiated, the number of TH+ cells was decreased by threefold, whereas mitomycin-c treatment of feeder cells decreased the number of TH+ cells by 32%. The neural-inducing effect of PA6 cells, as monitored by beta-III-tubulin expression, was minimally affected by mitomycin-c treatment or fixation but was decreased 50% by irradiation. Medium conditioned by PA6 cells was ineffective in differentiating TH+ cells when used alone. Conditioned medium combined with heparin and/or fixed PA6 cells produced TH+ cell differentiation, although less effectively than PA6 cell coculture. Thus, PA6 cell surface activity is required for neural differentiation of hESC, but secreted factors are required for the specific DA neuron-inducing effect. Disclosure of potential conflicts of interest is found at the end of this article.

摘要

生成多巴胺能(DA)神经元是人类胚胎干细胞(hESC)研究的主要目标。通过与小鼠PA6基质细胞系共培养,可使hESC分化为DA神经元;这种分化诱导效应被称为基质衍生诱导活性(SDIA)。然而,SDIA的分子和生化本质尚不清楚。各种研究表明,SDIA涉及位于PA6细胞表面的一种抗固定成分或PA6细胞分泌到培养基中的因子。为了解决这个问题,将hESC与PA6细胞共培养12天,然后用音猬因子同源物、成纤维细胞生长因子8和胶质细胞系衍生的神经营养因子进一步分化。18天后,34%的细胞为酪氨酸羟化酶(TH)阳性。当PA6细胞被固定或照射时,TH阳性细胞数量减少了三倍,而用丝裂霉素C处理饲养细胞使TH阳性细胞数量减少了32%。通过β-III-微管蛋白表达监测,PA6细胞的神经诱导作用受丝裂霉素C处理或固定的影响最小,但照射使其降低了50%。单独使用PA6细胞条件培养基在分化TH阳性细胞方面无效。条件培养基与肝素和/或固定的PA6细胞联合使用可诱导TH阳性细胞分化,尽管其效果不如PA6细胞共培养。因此,PA6细胞表面活性是hESC神经分化所必需的,但分泌因子是特定DA神经元诱导效应所必需的。潜在利益冲突的披露见本文末尾。

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