Endophilin-A coordinates priming and fusion of neurosecretory vesicles via intersectin

Author:

Gowrisankaran Sindhuja,Houy SébastienORCID,del Castillo Johanna G. Peña,Steubler Vicky,Gelker MonikaORCID,Kroll JanaORCID,Pinheiro Paulo S.,Schwitters Dirk,Halbsgut Nils,Pechstein Arndt,van Weering Jan R. T.,Maritzen TanjaORCID,Haucke VolkerORCID,Raimundo NunoORCID,Sørensen Jakob B.ORCID,Milosevic IraORCID

Abstract

AbstractEndophilins-A are conserved endocytic adaptors with membrane curvature-sensing and -inducing properties. We show here that, independently of their role in endocytosis, endophilin-A1 and endophilin-A2 regulate exocytosis of neurosecretory vesicles. The number and distribution of neurosecretory vesicles were not changed in chromaffin cells lacking endophilin-A, yet fast capacitance and amperometry measurements revealed reduced exocytosis, smaller vesicle pools and altered fusion kinetics. The levels and distributions of the main exocytic and endocytic factors were unchanged, and slow compensatory endocytosis was not robustly affected. Endophilin-A’s role in exocytosis is mediated through its SH3-domain, specifically via a direct interaction with intersectin-1, a coordinator of exocytic and endocytic traffic. Endophilin-A not able to bind intersectin-1, and intersectin-1 not able to bind endophilin-A, resulted in similar exocytic defects in chromaffin cells. Altogether, we report that two endocytic proteins, endophilin-A and intersectin-1, are enriched on neurosecretory vesicles and regulate exocytosis by coordinating neurosecretory vesicle priming and fusion.

Funder

Deutsche Forschungsgemeinschaft

Publisher

Springer Science and Business Media LLC

Subject

General Physics and Astronomy,General Biochemistry, Genetics and Molecular Biology,General Chemistry

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