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突触结合蛋白II对小鼠运动终板递质释放的调节作用

Regulation of transmitter release by synapsin II in mouse motor terminals.

作者信息

Samigullin Dmitry, Bill Cynthia A, Coleman William L, Bykhovskaia Maria

机构信息

Lehigh University, Department of Biological Sciences, Bethlehem, PA, USA.

出版信息

J Physiol. 2004 Nov 15;561(Pt 1):149-58. doi: 10.1113/jphysiol.2004.073494. Epub 2004 Sep 23.

Abstract

We investigated quantal release and ultrastructure in the neuromuscular junctions of synapsin II knockout (Syn II KO) mice. Synaptic responses were recorded focally from the diaphragm synapses during electrical stimulation of the phrenic nerve. We found that synapsin II affects transmitter release in a Ca(2+)-dependent manner. At reduced extracellular Ca(2+) (0.5 mM), Syn II KO mice demonstrated a significant increase in evoked and spontaneous quantal release, while at the physiological Ca(2+) concentration (2 mM), quantal release in Syn II KO synapses was unaffected. Protein kinase inhibitor H7 (100 microM) suppressed quantal release significantly stronger in Syn II KO synapses than in wild type (WT), indicating that Syn II KO synapses may compensate for the lack of synapsin II via a phosphorylation-dependent pathway. Electron microscopy analysis demonstrated that the lack of synapsin II results in an approximately 40% decrease in the density of synaptic vesicles in the reserve pool, while the number of vesicles docked to the presynaptic membrane remained unchanged. Synaptic depression in Syn II KO synapses was slightly increased, which is consistent with the depleted vesicle store in these synapses. At reduced Ca(2+) frequency facilitation of synchronous release was significantly increased in Syn II KO, while facilitation of asynchronous release was unaffected. Thus, at the reduced Ca(2+) concentration, synapsin II suppressed transmitter release and facilitation. These results demonstrate that synapsin II can regulate vesicle clustering, transmitter release, and facilitation.

摘要

我们研究了突触结合蛋白II基因敲除(Syn II KO)小鼠神经肌肉接头处的量子释放和超微结构。在膈神经电刺激期间,从膈肌突触局部记录突触反应。我们发现突触结合蛋白II以钙依赖的方式影响递质释放。在细胞外钙浓度降低(0.5 mM)时,Syn II KO小鼠的诱发量子释放和自发量子释放显著增加,而在生理钙浓度(2 mM)时,Syn II KO突触中的量子释放未受影响。蛋白激酶抑制剂H7(100 microM)在Syn II KO突触中比在野生型(WT)突触中更显著地抑制量子释放,这表明Syn II KO突触可能通过磷酸化依赖途径来弥补突触结合蛋白II的缺失。电子显微镜分析表明,突触结合蛋白II的缺失导致储备池中突触小泡密度降低约40%,而停靠在突触前膜上的小泡数量保持不变。Syn II KO突触中的突触抑制略有增加,这与这些突触中囊泡储备的耗尽一致。在钙浓度降低时,Syn II KO中同步释放的频率易化显著增加,而异步释放的易化未受影响。因此,在钙浓度降低时,突触结合蛋白II抑制递质释放和易化。这些结果表明,突触结合蛋白II可以调节囊泡聚集、递质释放和易化。

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