POST-DOCKING ROLE FOR SYNAPTOBREVIN IN SYNAPTIC VESICLE FUSION

被引:208
|
作者
HUNT, JM
BOMMERT, K
CHARLTON, MP
KISTNER, A
HABERMANN, E
AUGUSTINE, GJ
BETZ, H
机构
[1] MARINE BIOL LAB, WOODS HOLE, MA 02543 USA
[2] MAX PLANCK INST HIRNFORSCH, NEUROCHEM ABT, D-60528 FRANKFURT, GERMANY
[3] UNIV TORONTO, DEPT PHYSIOL, TORONTO M5S 1A8, ON, CANADA
[4] UNIV GIESSEN, RUDOLF BUCHHEIM INST PHARMAKOL, D-35392 GIESSEN, GERMANY
关键词
D O I
10.1016/0896-6273(94)90443-X
中图分类号
Q189 [神经科学];
学科分类号
071006 ;
摘要
We have used the squid giant synapse to determine the role of synaptobrevin, integral membrane proteins of small synaptic vesicles, in neurotransmitter release. The sequence of squid synaptobrevin, deduced by cDNA cloning, is 65%-68% identical to mammalian isoforms and includes the conserved cleavage site for tetanus and botulinum B toxins. Injection of either toxin into squid nerve terminals caused a slow, irreversible inhibition of release without affecting the Ca2+ signal which triggers release. Microinjection of a recombinant protein corresponding to the cytoplasmic domain of synaptobrevin produced a more rapid and reversible inhibition of release, whereas two smaller peptide fragments were without effect. Electron microscopy of tetanus-injected terminals revealed an increased number of both docked and undocked synaptic vesicles. These data indicate that synaptobrevin participates in neurotransmitter release at a step between vesicle docking and fusion.
引用
收藏
页码:1269 / 1279
页数:11
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