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膜联蛋白V在轴突终末的优先定位。

Preferential localization of annexin V to the axon terminal.

作者信息

Gotow T, Sakata M, Funakoshi T, Uchiyama Y

机构信息

Department of Cell Biology and Anatomy I, Osaka University Medical School, Japan.

出版信息

Neuroscience. 1996 Nov;75(2):507-21. doi: 10.1016/0306-4522(96)00295-3.

Abstract

To examine the participation of annexin V, a member of Ca(2+)-dependent phospholipid-binding proteins, in the process of synaptic vesicle exocytosis, rat central nervous tissue was analysed using biochemical and morphological techniques. By both fluorescence and confocal laser scanning microscopy, immunoreactivity for annexin V was predominantly localized around neuronal somata and dendrites, and the reactivity was mostly co-labeled with that for synaptophysin. The annexin V immunoreactivity was also detectable, but less intensely, in neuronal perikarya, glial cells and endothelial cells. Both immunoblot and immunoelectron microscopic analyses with intact tissues, synaptosomes and purified synaptic vesicles showed that annexin V was expressed in neurons, preferentially concentrated in axon terminals and associated with synaptic vesicles. Purified synaptic vesicles were relatively homogeneously distributed in the medium where Ca2+ was removed and thus the amount of annexin V was reduced drastically. The vesicles tended to be clustered in the fraction where endogenous annexin V is maintained, and the clusters were more conspicuous when purified human annexin V was added. Synaptic vesicles forming the clusters were not directly fused with each other but separated by a 10-15 nm gap that corresponded well with the size of single annexin V molecules. In axon terminals, globular structures 12-13 nm in diameter, similar in dimension to annexin V molecules, were distinctly found to be attached to the cytoplasmic surface of both vesicle membranes when the two vesicles were close to each other. These results suggest that annexin V belongs to the group of synaptic vesicle-associated proteins. Although its localization and significance in non-neuronal cells were not analysed here, at least in the axon terminal annexin V may participate in the cluster formation of synaptic vesicles by linking with the cytoplasmic surface of the vesicles in a Ca(2+)-dependent manner.

摘要

为研究依赖钙离子的磷脂结合蛋白成员膜联蛋白V在突触小泡胞吐过程中的参与情况,运用生化和形态学技术对大鼠中枢神经组织进行了分析。通过荧光显微镜和共聚焦激光扫描显微镜观察,膜联蛋白V的免疫反应主要定位于神经元胞体和树突周围,且该反应大多与突触素的反应共同标记。在神经元核周体、胶质细胞和内皮细胞中也可检测到膜联蛋白V的免疫反应,但强度较弱。对完整组织、突触体和纯化的突触小泡进行免疫印迹和免疫电子显微镜分析均显示,膜联蛋白V在神经元中表达,优先集中于轴突终末并与突触小泡相关。纯化的突触小泡在去除钙离子的培养基中相对均匀分布,因此膜联蛋白V的量急剧减少。小泡倾向于聚集在内源性膜联蛋白V得以维持的组分中,当添加纯化的人膜联蛋白V时,聚集更为明显。形成聚集的突触小泡并非直接相互融合,而是被一个10 - 15纳米的间隙隔开,该间隙与单个膜联蛋白V分子的大小相符。在轴突终末,当两个突触小泡彼此靠近时,明显发现直径为12 - 13纳米的球状结构附着于两个小泡膜的胞质表面,其大小与膜联蛋白V分子相似。这些结果表明膜联蛋白V属于突触小泡相关蛋白组。尽管此处未分析其在非神经元细胞中的定位和意义,但至少在轴突终末,膜联蛋白V可能通过以钙离子依赖的方式与突触小泡的胞质表面相连,参与突触小泡的聚集形成。

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