Active zone scaffolds differentially accumulate Unc13 isoforms to tune Ca2+ channel-vesicle coupling

被引:142
作者
Boehme, Mathias A. [1 ,2 ]
Beis, Christina [1 ]
Reddy-Alla, Suneel [1 ]
Reynolds, Eric [1 ]
Mampell, Malou M. [1 ]
Grasskamp, Andreas T. [2 ,3 ]
Luetzkendorf, Janine [1 ]
Bergeron, Dominique Dufour [1 ]
Driller, Jan H. [4 ]
Babikir, Husam [1 ]
Goettfert, Fabian [5 ]
Robinson, Iain M. [6 ]
O'Kane, Cahir J. [7 ]
Hell, Stefan W. [5 ]
Wahl, Markus C. [4 ]
Stelzl, Ulrich [8 ]
Loll, Bernhard [4 ]
Walter, Alexander M. [3 ]
Sigrist, Stephan J. [1 ,2 ]
机构
[1] Free Univ Berlin, Inst Biol Genet, Berlin, Germany
[2] Charite, Cluster Excellence, NeuroCure, Berlin, Germany
[3] Leibniz Inst Mol Pharmacol, Mol & Theoret Neurosci, Berlin, Germany
[4] Free Univ Berlin, Inst Chem & Biochem Struct Biochem, Berlin, Germany
[5] Max Planck Inst Biophys Chem, Dept Nanobiophoton, Gottingen, Germany
[6] Univ Plymouth, Peninsula Sch Med, Plymouth, Devon, England
[7] Univ Cambridge, Dept Genet, Cambridge, England
[8] Graz Univ, Inst Pharmaceut Sci, Pharmaceut Chem, Graz, Austria
关键词
READILY RELEASABLE POOL; SHORT-TERM PLASTICITY; SYNAPTIC VESICLES; NEUROTRANSMITTER RELEASE; NEUROMUSCULAR-JUNCTIONS; GLUTAMATE-RECEPTOR; DROSOPHILA; PROTEIN; DOMAIN; BRUCHPILOT;
D O I
10.1038/nn.4364
中图分类号
Q189 [神经科学];
学科分类号
071006 ;
摘要
Brain function relies on fast and precisely timed synaptic vesicle (SV) release at active zones (AZs). Efficacy of SV release depends on distance from SV to Ca2+ channel, but molecular mechanisms controlling this are unknown. Here we found that distances can be defined by targeting two unc-13 (Unc13) isoforms to presynaptic AZ subdomains. Super-resolution and intravital imaging of developing Drosophila melanogaster glutamatergic synapses revealed that the Unc13B isoform was recruited to nascent AZs by the scaffolding proteins Syd-1 and Liprin-alpha, and Unc13A was positioned by Bruchpilot and Rim-binding protein complexes at maturing AZs. Unc13B localized 120 nm away from Ca2+ channels, whereas Unc13A localized only 70 nm away and was responsible for docking SVs at this distance. Unc13A(null) mutants suffered from inefficient, delayed and EGTA-supersensitive release. Mathematical modeling suggested that synapses normally operate via two independent release pathways differentially positioned by either isoform. We identified isoform-specific Unc13-AZ scaffold interactions regulating SV-Ca2+-channel topology whose developmental tightening optimizes synaptic transmission.
引用
收藏
页码:1311 / +
页数:19
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