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大鼠小脑中GABA(B1)和GABA(B2)受体蛋白的细胞及亚细胞定位

Cellular and sub-cellular localisation of GABA(B1) and GABA(B2) receptor proteins in the rat cerebellum.

作者信息

Ige A O, Bolam J P, Billinton A, White J H, Marshall F H, Emson P C

机构信息

Department of Neurobiology, Babraham Institute, Babraham, CB2 4AT, Cambridge, UK.

出版信息

Brain Res Mol Brain Res. 2000 Nov 10;83(1-2):72-80. doi: 10.1016/s0169-328x(00)00199-6.

Abstract

Following the recent discovery that GABA(B) receptors expressed in cell lines are only functional when both GABA(B1) and GABA(B2) are expressed, the present study reports on the development of polyclonal antisera specific for carboxyl-terminal portions of the two related GABA(B) receptor components respectively. Western blotting indicated the specificity of affinity-purified antibodies for native or recombinant expressed GABA(BR1) and GABA(BR2), with no cross-reactivity, both antisera detecting the heterodimer in rat cerebellar membranes. Immunohistochemistry revealed a distinct distribution of both receptor proteins in rat cerebellum. GABA(B1) immunoreactivity was primarily located in the granule cell layer and Purkinje cells, with discrete immuno-positive cell bodies being present in the molecular layer. GABA(B2) staining revealed intense immunoreactivity in the molecular layer, with weaker staining in the granule cell layer. Purkinje cell bodies were less intensely immuno-positive for GABA(B2). Co-localisation of both receptor proteins was observed using double immunofluorescence techniques, consistent with the notion that both proteins are required for the formation of functional GABA(B) receptors in vivo. Immunofluorescence also indicated that GABA(B) receptors did not co-localise with glial fibrillary acid protein, confirming a neuronal localisation for GABA(B) receptors. Electron microscopic analysis of the molecular layer revealed that the distribution of immunolabelling for both GABA(B1) and GABA(B2) was mainly located on the membrane of Purkinje cell dendrites and spines and in parallel fibre terminals.

摘要

最近发现细胞系中表达的GABA(B)受体只有在同时表达GABA(B1)和GABA(B2)时才具有功能,本研究报告了分别针对两种相关GABA(B)受体成分羧基末端部分的多克隆抗血清的研制情况。蛋白质免疫印迹法表明亲和纯化抗体对天然或重组表达的GABA(BR1)和GABA(BR2)具有特异性,无交叉反应,两种抗血清均能检测大鼠小脑膜中的异二聚体。免疫组织化学揭示了两种受体蛋白在大鼠小脑中的不同分布。GABA(B1)免疫反应主要位于颗粒细胞层和浦肯野细胞,分子层中有离散的免疫阳性细胞体。GABA(B2)染色显示分子层有强烈的免疫反应,颗粒细胞层染色较弱。浦肯野细胞体对GABA(B2)的免疫阳性较弱。使用双重免疫荧光技术观察到两种受体蛋白的共定位,这与两种蛋白在体内形成功能性GABA(B)受体所需的观点一致。免疫荧光还表明GABA(B)受体不与胶质纤维酸性蛋白共定位,证实了GABA(B)受体的神经元定位。对分子层的电子显微镜分析显示,GABA(B1)和GABA(B2)的免疫标记分布主要位于浦肯野细胞树突和棘突的膜上以及平行纤维终末。

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