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单个神经元释放位点的形态学和分子异质性。

Morphological and molecular heterogeneity in release sites of single neurons.

作者信息

Morgenthaler Florence D, Knott Graham W, Floyd Sarria J-C, Wang Xin, Staple Julie K, Catsicas Stefan, Hirling Harald

机构信息

Institut de Biologie Cellulaire et de Morphologie (IBCM), Rue du Bugnon 9, 1005 Lausanne, Switzerland.

出版信息

Eur J Neurosci. 2003 Apr;17(7):1365-74. doi: 10.1046/j.1460-9568.2003.02572.x.

DOI:10.1046/j.1460-9568.2003.02572.x
PMID:12713639
Abstract

We have previously shown that labelling intensities for synaptic proteins vary strongly among synaptic boutons. Here we addressed the questions as to whether there are heterogeneous levels of integral membrane synaptic vesicle proteins at distinct active release sites of single neurons and if these sites possess the ultrastructural features of synapses. By double-immunostaining with specific antibodies against synaptophysin, synaptotagmin I, VAMP1 and VAMP2, we identified different relative levels of these integral membrane proteins of synaptic vesicles in comparison to boutons of the same rat cortical neuron. This heterogeneity could also be observed between the two isoforms VAMP1 and VAMP2. By studying pairs of these proteins implicated in neurotransmitter release, including both VAMP isoforms, we also show that the sites that contained predominantly one protein were nevertheless functional, as they internalized and released FM1-43 upon potassium stimulation. Using electron microscopy, we show that these active sites could have either synaptic specializations, or the features of vesicle-containing varicosities without a postsynaptic target. Different varicosities of the same neuron showed different intensities for synaptic vesicle proteins; some varicosities were capable of internalizing and releasing FM1-43, while others were silent. These results show that integral membrane synaptic vesicle proteins are differentially distributed among functional release sites of the same neuron.

摘要

我们之前已经表明,突触蛋白的标记强度在突触小体之间差异很大。在这里,我们探讨了以下问题:在单个神经元的不同活性释放位点,整合膜突触小泡蛋白的水平是否存在异质性,以及这些位点是否具有突触的超微结构特征。通过用抗突触素、突触结合蛋白I、VAMP1和VAMP2的特异性抗体进行双重免疫染色,我们确定了与同一大鼠皮质神经元的突触小体相比,这些突触小泡整合膜蛋白的不同相对水平。这种异质性在VAMP1和VAMP2这两种异构体之间也可以观察到。通过研究这些与神经递质释放有关的蛋白质对,包括两种VAMP异构体,我们还表明,主要含有一种蛋白质的位点仍然是有功能的,因为它们在钾离子刺激下内化并释放FM1-43。使用电子显微镜,我们表明这些活性位点可能具有突触特化结构,或者具有不含突触后靶点的含小泡膨体的特征。同一神经元的不同膨体对突触小泡蛋白显示出不同的强度;一些膨体能够内化并释放FM1-43,而另一些则没有活性。这些结果表明,整合膜突触小泡蛋白在同一神经元的功能释放位点之间存在差异分布。

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