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通过破坏钙离子通道/ syntaxin相互作用改变神经递质释放对钙离子的依赖性。

Alteration of Ca2+ dependence of neurotransmitter release by disruption of Ca2+ channel/syntaxin interaction.

作者信息

Rettig J, Heinemann C, Ashery U, Sheng Z H, Yokoyama C T, Catterall W A, Neher E

机构信息

Department of Membrane Biophysics, Max-Planck-Institute for Biophysical Chemistry, 37077 Göttingen, Germany.

出版信息

J Neurosci. 1997 Sep 1;17(17):6647-56. doi: 10.1523/JNEUROSCI.17-17-06647.1997.

Abstract

Presynaptic N-type calcium channels interact with syntaxin and synaptosome-associated protein of 25 kDa (SNAP-25) through a binding site in the intracellular loop connecting domains II and III of the alpha1 subunit. This binding region was loaded into embryonic spinal neurons of Xenopus by early blastomere injection. After culturing, synaptic transmission of peptide-loaded and control cells was compared by measuring postsynaptic responses under different external Ca2+ concentrations. The relative transmitter release of injected neurons was reduced by approximately 25% at physiological Ca2+ concentration, whereas injection of the corresponding region of the L-type Ca2+ channel had virtually no effect. When applied to a theoretical model, these results imply that 70% of the formerly linked vesicles have been uncoupled after action of the peptide. Our data suggest that severing the physical interaction between presynaptic calcium channels and synaptic proteins will not prevent synaptic transmission at this synapse but will make it less efficient by shifting its Ca2+ dependence to higher values.

摘要

突触前N型钙通道通过α1亚基中连接结构域II和III的细胞内环中的一个结合位点,与 syntaxin 和 25 kDa 的突触体相关蛋白(SNAP-25)相互作用。通过早期卵裂球注射,将该结合区域导入非洲爪蟾的胚胎脊髓神经元。培养后,通过测量不同细胞外Ca2+浓度下的突触后反应,比较加载肽的细胞和对照细胞的突触传递。在生理Ca2+浓度下,注射神经元的相对递质释放减少了约25%,而注射L型钙通道的相应区域几乎没有影响。当应用于理论模型时,这些结果表明,在肽作用后,70%以前相连的囊泡已经解偶联。我们的数据表明,切断突触前钙通道和突触蛋白之间的物理相互作用不会阻止该突触的突触传递,但会通过将其Ca2+依赖性转移到更高的值而使其效率降低。

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