SM protein Sly1 and a SNARE Habc domain promote membrane fusion through multiple mechanisms

Author:

Duan Mengtong1ORCID,Gao Guanbin2ORCID,Lin Ariel1ORCID,Mackey Emma J.1ORCID,Banfield David K.2ORCID,Merz Alexey J.1ORCID

Affiliation:

1. University of Washington 1 Department of Biochemistry, , Seattle, WA, USA

2. The Hong Kong University of Science and Technology 2 The Division of Life Science, , Kowloon, Hong Kong

Abstract

SM proteins including Sly1 are essential cofactors of SNARE-mediated membrane fusion. Using SNARE and Sly1 mutants and chemically defined in vitro assays, we separate and assess proposed mechanisms through which Sly1 augments fusion: (i) opening the closed conformation of the Qa-SNARE Sed5; (ii) close-range tethering of vesicles to target organelles, mediated by the Sly1-specific regulatory loop; and (iii) nucleation of productive trans-SNARE complexes. We show that all three mechanisms are important and operate in parallel, and that close-range tethering promotes trans-complex assembly when cis-SNARE assembly is a competing process. Further, we demonstrate that the autoinhibitory N-terminal Habc domain of Sed5 has at least two positive activities: it is needed for correct Sed5 localization, and it directly promotes Sly1-dependent fusion. “Split Sed5,” with Habc presented solely as a soluble fragment, can function both in vitro and in vivo. Habc appears to facilitate events leading to lipid mixing rather than promoting opening or stability of the fusion pore.

Funder

National Institutes of Health

National Institute of General Medical Sciences

University of Washington

Hong Kong Research Council

Publisher

Rockefeller University Press

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