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中脑I型星形胶质细胞介导培养的黑质多巴胺能神经元的存活。

Mesencephalic type I astrocytes mediate the survival of substantia nigra dopaminergic neurons in culture.

作者信息

O'Malley E K, Sieber B A, Black I B, Dreyfus C F

机构信息

Department of Neuroscience and Cell Biology, UMDNJ/Robert Wood Johnson Medical School, Piscataway 08854-5635.

出版信息

Brain Res. 1992 Jun 5;582(1):65-70. doi: 10.1016/0006-8993(92)90317-3.

DOI:10.1016/0006-8993(92)90317-3
PMID:1379874
Abstract

We previously demonstrated that substantia nigra (SN) support cells selectively increase SN dopamine (DA) neuron survival in dissociated primary culture. Increased survival was elicited specifically by nigral support cells; glia from other brain regions exerted lesser effects. We now report that Type I astrocytes, the principal component of SN support cell monolayers, mediate the enhanced DA cell survival. Initially, the predominant glial subtypes in SN support cell cultures were identified. Postnatal day 1 rat SN was dissociated and cells were grown to confluence (7-9 days in vitro; DIV). Monolayers were immunostained with antibodies against glial fibrillary acidic protein (GFAP; an astrocyte-specific marker), myelin basic protein (MBP; an oligodendrocyte marker), or A2B5 (recognizes 0-2A progenitors and Type II astrocytes). The number of GFAP+ cells far exceeded MBP+ and A2B5+ cells, suggesting that astrocytes constituted the predominant subpopulation. Further, direct comparison of GFAP+ (Type I and Type II astrocytes) and A2B5+ (Type II astrocytes) cells indicated that the vast majority were Type I astrocytes. Greater than 98% of cells reacted with glial antibodies. To definitively characterize the cellular subtype that augments survival of DA neurons, glial subcultures were established. At 2 DIV, enriched populations of Type I or Type II astrocytes, or oligodendrocytes, were tested for the ability to elicit DA neuron survival. Embryonic day 16 rat SN dissociates were added and DA cell number was assessed with antibody against tyrosine hydroxylase (TH), the DA biosynthetic enzyme.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

我们之前证明,在解离的原代培养中,黑质(SN)支持细胞可选择性地提高SN多巴胺(DA)神经元的存活率。存活率的提高是由黑质支持细胞特异性引起的;来自其他脑区的胶质细胞作用较小。我们现在报告,I型星形胶质细胞是SN支持细胞单层的主要成分,介导了DA细胞存活率的提高。首先,确定了SN支持细胞培养物中主要的胶质细胞亚型。出生后第1天的大鼠SN被解离,细胞生长至汇合(体外培养7 - 9天;DIV)。用抗胶质纤维酸性蛋白(GFAP;一种星形胶质细胞特异性标志物)、髓鞘碱性蛋白(MBP;一种少突胶质细胞标志物)或A2B5(识别0 - 2A祖细胞和II型星形胶质细胞)的抗体对单层细胞进行免疫染色。GFAP+细胞的数量远远超过MBP+和A2B5+细胞,这表明星形胶质细胞构成了主要的亚群。此外,对GFAP+(I型和II型星形胶质细胞)和A2B5+(II型星形胶质细胞)细胞的直接比较表明,绝大多数是I型星形胶质细胞。超过98%的细胞与胶质细胞抗体发生反应。为了明确表征增强DA神经元存活率的细胞亚型,建立了胶质细胞亚培养物。在体外培养第2天,检测富集的I型或II型星形胶质细胞或少突胶质细胞群体引发DA神经元存活的能力。添加胚胎第16天的大鼠SN解离物,并用抗酪氨酸羟化酶(TH,DA生物合成酶)的抗体评估DA细胞数量。(摘要截断于250字)

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