A single vesicle-vesicle fusion assay for in vitro studies of SNAREs and accessory proteins

Authors
Diao, JiajieIshitsuka, YujiLee, HankiJoo, ChirlminSu, ZengliuSyed, SalmanShin, Yeon-KyunYoon, Tae-YoungHa, Taekjip
Issue Date
2012-04
Publisher
NATURE PUBLISHING GROUP
Citation
NATURE PROTOCOLS, v.7, no.5, pp.921 - 934
Abstract
SNARE (soluble N-ethylmaleimide-sensitive factor attachment protein receptor) proteins are a highly regulated class of membrane proteins that drive the efficient merger of two distinct lipid bilayers into one interconnected structure. This protocol describes our fluorescence resonance energy transfer (FRET)-based single vesicle-vesicle fusion assays for SNAREs and accessory proteins. Both lipid-mixing (with FRET pairs acting as lipophilic dyes in the membranes) and content-mixing assays (with FRET pairs present on a DNA hairpin that becomes linear via hybridization to a complementary DNA) are described. These assays can be used to detect substages such as docking, hemifusion, and pore expansion and full fusion. The details of flow cell preparation, protein-reconstituted vesicle preparation, data acquisition and analysis are described. These assays can be used to study the roles of various SNARE proteins, accessory proteins and effects of different lipid compositions on specific fusion steps. The total time required to finish one round of this protocol is 3-6 d.
Keywords
MEMBRANE-FUSION; LIPID VESICLES; MOLECULE; DRIVEN; MACHINERY; DOCKING; COMPLEX; SURFACE; MEMBRANE-FUSION; LIPID VESICLES; MOLECULE; DRIVEN; MACHINERY; DOCKING; COMPLEX; SURFACE; SNARE; vesicle fusion assay; single vesicle FRET; Content-mixing assay; lipid-mixing assay
ISSN
1754-2189
URI
https://pubs.kist.re.kr/handle/201004/129381
DOI
10.1038/nprot.2012.020
Appears in Collections:
KIST Article > 2012
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