Preparation and characterization of SNARE-containing nanodiscs and direct study of cargo release through fusion pores

被引:25
|
作者
Shi, Lei [1 ]
Howan, Kevin [2 ,3 ]
Shen, Qing-Tao [4 ]
Wang, Yong Jian [2 ,3 ]
Rothman, James E. [1 ]
Pincet, Frederic [1 ,2 ,3 ]
机构
[1] Yale Univ, Sch Med, Dept Cell Biol, New Haven, CT 06510 USA
[2] Univ Paris 06, CNRS, Lab Phys Stat, UMR 8550,ENS, Paris, France
[3] Univ Paris Diderot, Dept Phys, Paris, France
[4] Yale Univ, Dept Mol Biophys & Biochem, New Haven, CT USA
基金
美国国家卫生研究院;
关键词
MEMBRANE-FUSION; T-SNARE; COMPLEX; RECONSTITUTION; PROTEINS;
D O I
10.1038/nprot.2013.048
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
This protocol describes an assay that uses suspended nanomembranes called nanodiscs to analyze fusion events. A nanodisc is a lipid bilayer wrapped by membrane scaffold proteins. Fluorescent lipids and a protein that is part of a fusion machinery, VAMP2 in the example detailed herein, are included in the nanodiscs. Upon fusion of a nanodisc with a nonfluorescent liposome containing cognate proteins (for instance, the VAMP2 cognate syntaxin1/SNAP-25 complex), the fluorescent lipids are dispersed in the liposome and the increase in fluorescence, initially quenched in the nanodisc, is monitored on a plate reader. Because the scaffold proteins restrain pore expansion, the fusion pore eventually reseals. A reducing agent, such as dithionite, which can quench the fluorescence of accessible lipids, can then be used to determine the number of fusion events. A fluorescence-based approach can also be used to monitor the release of encapsulated cargo. From data on the total cargo release and the number of the much faster lipid- mixing events, the researcher may determine the amount of cargo released per fusion event. This assay requires 3 d for preparation and 4 h for data acquisition and analysis.
引用
收藏
页码:935 / 948
页数:14
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