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2
Munc13-2 differentially affects hippocampal synaptic transmission and plasticity.Munc13-2 对海马体突触传递和可塑性有差异影响。
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3
Synapsin-dependent reserve pool of synaptic vesicles supports replenishment of the readily releasable pool under intense synaptic transmission.突触囊泡的突触素依赖储备池支持在强烈的突触传递下易释放池的补充。
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4
Dynamin 1- and 3-Mediated Endocytosis Is Essential for the Development of a Large Central Synapse In Vivo.发动蛋白1和3介导的内吞作用对于体内大型中枢突触的发育至关重要。
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6
Calcium-dependent isoforms of protein kinase C mediate posttetanic potentiation at the calyx of Held.蛋白激酶 C 的钙依赖性同工型介导了 Held 壶腹的强直后增强。
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The cerebellum-specific Munc13 isoform Munc13-3 regulates cerebellar synaptic transmission and motor learning in mice.小脑特异性Munc13亚型Munc13-3调节小鼠的小脑突触传递和运动学习。
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Munc13-1 C1 domain activation lowers the energy barrier for synaptic vesicle fusion.Munc13-1 C1结构域激活降低了突触小泡融合的能量屏障。
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Differential control of vesicle priming and short-term plasticity by Munc13 isoforms.Munc13亚型对囊泡启动和短期可塑性的差异控制。
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10
Nonconserved Ca(2+)/calmodulin binding sites in Munc13s differentially control synaptic short-term plasticity.Munc13s 中的非保守 Ca(2+)/钙调蛋白结合位点差异调控突触的短期可塑性。
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Two successive oligomeric Munc13 assemblies scaffold vesicle docking and SNARE assembly to support neurotransmitter release.两个连续的寡聚Munc13组装体搭建囊泡对接和SNARE组装的支架,以支持神经递质释放。
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A specific negatively charged sequence confers intramolecular regulation on Munc13-1 function in synaptic exocytosis.一个特定的带负电荷序列赋予Munc13-1在突触胞吐作用中的分子内调节功能。
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7
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8
Clarinet/CLA-1 recruits RIMB-1/RIM-binding protein and UNC-13 to orchestrate presynaptic neurotransmitter release.单簧管/CLA-1 招募 RIMB-1/RIM 结合蛋白和 UNC-13 以协调突触前神经递质释放。
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本文引用的文献

1
The presynaptic active zone.突触前活性区。
Neuron. 2012 Jul 12;75(1):11-25. doi: 10.1016/j.neuron.2012.06.012.
2
Munc13-independent vesicle priming at mouse photoreceptor ribbon synapses.Munc13 非依赖性囊泡引发小鼠光感受器突触上的带状突触
J Neurosci. 2012 Jun 6;32(23):8040-52. doi: 10.1523/JNEUROSCI.4240-11.2012.
3
Actin-dependent rapid recruitment of reluctant synaptic vesicles into a fast-releasing vesicle pool.肌动蛋白依赖性的不情愿突触小泡快速募集到快速释放的囊泡库中。
Proc Natl Acad Sci U S A. 2012 Mar 27;109(13):E765-74. doi: 10.1073/pnas.1114072109. Epub 2012 Mar 5.
4
The calyx of Held synapse: from model synapse to auditory relay.Held 突触花萼:从模式突触到听觉中继。
Annu Rev Physiol. 2012;74:199-224. doi: 10.1146/annurev-physiol-020911-153236. Epub 2011 Oct 24.
5
The crystal structure of a Munc13 C-terminal module exhibits a remarkable similarity to vesicle tethering factors.一个 Munc13 C 末端模块的晶体结构与囊泡连接因子表现出显著的相似性。
Structure. 2011 Oct 12;19(10):1443-55. doi: 10.1016/j.str.2011.07.012.
6
pUNISHER: a high-level expression cassette for use with recombinant viral vectors for rapid and long term in vivo neuronal expression in the CNS.pUNISHER:一种用于重组病毒载体的高级表达盒,可用于在中枢神经系统中快速和长期体内神经元表达。
J Neurophysiol. 2011 Dec;106(6):3230-44. doi: 10.1152/jn.00713.2011. Epub 2011 Sep 28.
7
Molecular in situ topology of Aczonin/Piccolo and associated proteins at the mammalian neurotransmitter release site.哺乳动物神经递质释放位点上 Aczonin/Piccolo 及其相关蛋白的分子原位拓扑结构。
Proc Natl Acad Sci U S A. 2011 Aug 2;108(31):E392-401. doi: 10.1073/pnas.1101707108. Epub 2011 Jun 28.
8
On the classification of pathways in the auditory midbrain, thalamus, and cortex.在听觉中脑、丘脑和皮层的通路分类上。
Hear Res. 2011 Jun;276(1-2):79-87. doi: 10.1016/j.heares.2010.12.012. Epub 2010 Dec 22.
9
Post-tetanic increase in the fast-releasing synaptic vesicle pool at the expense of the slowly releasing pool.在快速释放突触囊泡池中出现强直后增强,而慢速释放池则相应减少。
J Gen Physiol. 2010 Sep;136(3):259-72. doi: 10.1085/jgp.201010437.
10
Quantitative proteomics of the Cav2 channel nano-environments in the mammalian brain.哺乳动物脑内 Cav2 通道纳米环境的定量蛋白质组学。
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Munc13 蛋白在中枢突触中差异调节易释放池动力学和钙依赖性恢复。

The Munc13 proteins differentially regulate readily releasable pool dynamics and calcium-dependent recovery at a central synapse.

机构信息

School of Life Science and Technology, Huazhong University of Science and Technology, Wuhan, Hubei 430074, China.

出版信息

J Neurosci. 2013 May 8;33(19):8336-51. doi: 10.1523/JNEUROSCI.5128-12.2013.

DOI:10.1523/JNEUROSCI.5128-12.2013
PMID:23658173
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6619620/
Abstract

The Munc13 gene family encodes molecules located at the synaptic active zone that regulate the reliability of synapses to encode information over a wide range of frequencies in response to action potentials. In the CNS, proteins of the Munc13 family are critical in regulating neurotransmitter release and synaptic plasticity. Although Munc13-1 is essential for synaptic transmission, it is paradoxical that Munc13-2 and Munc13-3 are functionally dispensable at some synapses, although their loss in other synapses leads to increases in frequency-dependent facilitation. We addressed this issue at the calyx of Held synapse, a giant glutamatergic synapse that we found to express all these Munc13 isoforms. We studied their roles in the regulation of synaptic transmission and their impact on the reliability of information transfer. Through detailed electrophysiological analyses of Munc13-2, Munc13-3, and Munc13-2-3 knock-out and wild-type mice, we report that the combined loss of Munc13-2 and Munc13-3 led to an increase in the rate of calcium-dependent recovery and a change in kinetics of release of the readily releasable pool. Furthermore, viral-mediated overexpression of a dominant-negative form of Munc13-1 at the calyx demonstrated that these effects are Munc13-1 dependent. Quantitative immunohistochemistry using Munc13-fluorescent protein knock-in mice revealed that Munc13-1 is the most highly expressed Munc13 isoform at the calyx and the only one highly colocalized with Bassoon at the active zone. Based on these data, we conclude that Munc13-2 and Munc13-3 isoforms limit the ability of Munc13-1 to regulate calcium-dependent replenishment of readily releasable pool and slow pool to fast pool conversion in central synapses.

摘要

Munc13 基因家族编码位于突触活性区的分子,调节突触在动作电位响应范围内的广泛频率下编码信息的可靠性。在中枢神经系统中,Munc13 家族的蛋白质在调节神经递质释放和突触可塑性方面至关重要。虽然 Munc13-1 对突触传递是必不可少的,但令人费解的是,Munc13-2 和 Munc13-3 在某些突触中功能上是可有可无的,尽管它们在其他突触中的缺失会导致频率依赖性易化增加。我们在巨大谷氨酸能突触的 Held 突触中解决了这个问题,发现所有这些 Munc13 同工型都在该突触中表达。我们研究了它们在调节突触传递中的作用及其对信息传递可靠性的影响。通过对 Munc13-2、Munc13-3 和 Munc13-2-3 敲除和野生型小鼠的详细电生理分析,我们报告说,Munc13-2 和 Munc13-3 的联合缺失导致钙依赖性恢复速率增加和易释放池释放动力学发生变化。此外,在 Held 突触中,通过病毒介导过表达一种 Munc13-1 的显性负形式的实验表明,这些效应依赖于 Munc13-1。使用 Munc13-荧光蛋白敲入小鼠的定量免疫组织化学显示,Munc13-1 是 Held 突触中表达水平最高的 Munc13 同工型,也是唯一与活性区中的 Bassoon 高度共定位的同工型。基于这些数据,我们得出结论,Munc13-2 和 Munc13-3 同工型限制了 Munc13-1 调节中央突触中钙依赖性易释放池再填充和慢池向快池转化的能力。