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突触结合蛋白 IV 的缺失导致培养的海马神经元中的突触小泡减少和高尔基体结构变形。

Loss of synaptotagmin IV results in a reduction in synaptic vesicles and a distortion of the Golgi structure in cultured hippocampal neurons.

机构信息

MCD Biology, University of Colorado, Boulder, CO 80309, USA.

出版信息

Neuroscience. 2010 Apr 28;167(1):135-42. doi: 10.1016/j.neuroscience.2010.01.056. Epub 2010 Feb 4.

Abstract

Fusion of synaptic vesicles with the plasma membrane is mediated by the SNARE (soluble NSF attachment receptor) proteins and is regulated by synaptotagmin (syt). There are at least 17 syt isoforms that have the potential to act as modulators of membrane fusion events. Synaptotagmin IV (syt IV) is particularly interesting; it is an immediate early gene that is regulated by seizures and certain classes of drugs, and, in humans, syt IV maps to a region of chromosome 18 associated with schizophrenia and bipolar disease. Syt IV has recently been found to localize to dense core vesicles in hippocampal neurons, where it regulates neurotrophin release. Here we have examined the ultrastructure of cultured hippocampal neurons from wild-type and syt IV -/- mice using electron tomography. Perhaps surprisingly, we observed a potential synaptic vesicle transport defect in syt IV -/- neurons, with the accumulation of large numbers of small clear vesicles (putative axonal transport vesicles) near the trans-Golgi network. We also found an interaction between syt IV and KIF1A, a kinesin known to be involved in vesicle trafficking to the synapse. Finally, we found that syt IV -/- synapses exhibited reduced numbers of synaptic vesicles and a twofold reduction in the proportion of docked vesicles compared to wild-type. The proportion of docked vesicles in syt IV -/- boutons was further reduced, 5-fold, following depolarization.

摘要

突触小泡与质膜的融合是由 SNARE(可溶性 NSF 附着受体)蛋白介导的,受突触融合蛋白(syt)调节。至少有 17 种 syt 异构体有可能作为膜融合事件的调节剂。突触融合蛋白 IV(syt IV)特别有趣;它是一种即时早期基因,受癫痫和某些类药物的调节,在人类中,syt IV 位于与精神分裂症和双相情感障碍相关的染色体 18 区域。最近发现 syt IV 定位于海马神经元的致密核心囊泡,在那里它调节神经营养因子的释放。在这里,我们使用电子断层扫描技术检查了来自野生型和 syt IV -/- 小鼠的培养海马神经元的超微结构。也许令人惊讶的是,我们观察到 syt IV -/- 神经元中存在潜在的突触小泡运输缺陷,大量小而透明的囊泡(假定的轴突运输囊泡)在高尔基体内网络附近积聚。我们还发现 syt IV 与 KIF1A 之间存在相互作用,KIF1A 是一种已知参与囊泡向突触运输的驱动蛋白。最后,我们发现与野生型相比,syt IV -/- 突触的突触小泡数量减少,停靠囊泡的比例减少了两倍。syt IV -/- 末梢中的停靠囊泡比例进一步减少,为 5 倍,随后去极化。

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