Cryo–electron tomography reveals a critical role of RIM1α in synaptic vesicle tethering

Author:

Fernández-Busnadiego Rubén1,Asano Shoh1,Oprisoreanu Ana-Maria22,Sakata Eri1,Doengi Michael2,Kochovski Zdravko1,Zürner Magdalena22,Stein Valentin2,Schoch Susanne22,Baumeister Wolfgang1,Lučić Vladan1

Affiliation:

1. Department of Molecular Structural Biology, Max Planck Institute of Biochemistry, 82152 Martinsried, Germany

2. Department of Neuropathology, Department of Epileptology, and Institute of Physiology II, University of Bonn, 53105 Bonn, Germany

Abstract

Synaptic vesicles are embedded in a complex filamentous network at the presynaptic terminal. Before fusion, vesicles are linked to the active zone (AZ) by short filaments (tethers). The identity of the molecules that form and regulate tethers remains unknown, but Rab3-interacting molecule (RIM) is a prominent candidate, given its central role in AZ organization. In this paper, we analyzed presynaptic architecture of RIM1α knockout (KO) mice by cryo–electron tomography. In stark contrast to previous work on dehydrated, chemically fixed samples, our data show significant alterations in vesicle distribution and AZ tethering that could provide a structural basis for the functional deficits of RIM1α KO synapses. Proteasome inhibition reversed these structural defects, suggesting a functional recovery confirmed by electrophysiological recordings. Altogether, our results not only point to the ubiquitin–proteasome system as an important regulator of presynaptic architecture and function but also show that the tethering machinery plays a critical role in exocytosis, converging into a structural model of synaptic vesicle priming by RIM1α.

Publisher

Rockefeller University Press

Subject

Cell Biology

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