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培养的海马细胞上的GABAA受体簇仅部分与功能性突触相关。

Clusters of GABAA receptors on cultured hippocampal cells correlate only partially with functional synapses.

作者信息

Kannenberg K, Sieghart W, Reuter H

机构信息

Department of Pharmacology, University of Bern, Switzerland.

出版信息

Eur J Neurosci. 1999 Apr;11(4):1256-64. doi: 10.1046/j.1460-9568.1999.00533.x.

Abstract

We describe a method to label gamma-aminobutyric acid (GABA)A receptors on the surface of living hippocampal neurons in primary culture, and we compare the distribution of receptors with that of active synapses. To visualize GABAA receptors, the affinity-purified antibody beta3(1-13), recognizing the extracellular N-termini of the GABAA receptor beta2- and beta3-subunits, was used in combination with fluorescent secondary antibodies. The beta2- and beta3-subunits belong to the predominant GABAA receptor subunits in the hippocampus. As expected for aggregates of GABAA receptors in the somato-dendritic plasma membrane, a patchy staining pattern similar to that seen by labelling neurons after fixation was obtained. An antiserum recognizing an intracellular epitope of GABAA receptor beta3-subunits did not label the receptors in living neurons. Whole-cell recordings of GABA-evoked Cl - currents were not affected after decorating GABAA receptors with antibody beta3(1-13). Combining the staining of GABAA receptors with the labelling of active presynaptic terminals with the fluorescent dyes FM1-43 or FM4-64, consistently resulted in the detection of GABAA receptor clusters that were not located at active synapses. These amounted to approximately 50% of all labelled GABAA receptor clusters. GABAA receptor clusters that were not associated with active presynaptic terminals partially colocalized with the synaptic vesicle marker protein sv2, while another fraction had no presynaptic counterpart at all. These findings suggest the presence of presynaptically silent GABAergic synapses in cultured hippocampal neurons. They also indicate that for the maintenance of GABAA receptor aggregates, the release of GABA from an opposing active terminal is not essential.

摘要

我们描述了一种标记原代培养的活海马神经元表面γ-氨基丁酸(GABA)A受体的方法,并将受体的分布与活跃突触的分布进行比较。为了可视化GABAA受体,使用了亲和纯化的抗体β3(1-13),它识别GABAA受体β2和β3亚基的细胞外N端,并与荧光二抗结合使用。β2和β3亚基属于海马中主要的GABAA受体亚基。正如预期的那样,在体细胞-树突质膜中GABAA受体聚集,获得了与固定后标记神经元所见相似的斑点状染色模式。识别GABAA受体β3亚基细胞内表位的抗血清未标记活神经元中的受体。用抗体β3(1-13)修饰GABAA受体后,GABA诱发的Cl-电流的全细胞记录不受影响。将GABAA受体的染色与用荧光染料FM1-43或FM4-64标记活跃的突触前终末相结合,始终能检测到不在活跃突触处的GABAA受体簇。这些约占所有标记的GABAA受体簇的50%。与活跃突触前终末不相关的GABAA受体簇部分与突触囊泡标记蛋白sv2共定位,而另一部分则完全没有突触前对应物。这些发现表明培养的海马神经元中存在突触前沉默的GABA能突触。它们还表明,对于GABAA受体聚集体的维持,来自相对活跃终末的GABA释放并非必不可少。

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