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A cell-free system for Ca2+-regulated exocytosis

被引:9
作者
Edwardson, JM [1 ]
机构
[1] Univ Cambridge, Dept Pharmacol, Cambridge CB2 1QJ, England
来源
METHODS-A COMPANION TO METHODS IN ENZYMOLOGY | 1998年 / 16卷 / 02期
基金
英国惠康基金;
关键词
D O I
10.1006/meth.1998.0669
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
The reconstitution of a membrane fusion event in a cell-free system makes possible a biochemical investigation of the molecular mechanisms underlying it. We have developed an in vitro assay for the fusion of pancreatic zymogen granules with the plasma membrane. The lipid-soluble fluorescent probe octadecyl-rhodamine is loaded into the granule membrane, and the granules are then incubated with unlabeled plasma membranes. Membrane fusion results in a dilution of the probe, which is detected through the dequenching of its fluorescence. The properties of the in vitro fusion event are impressively similar to those of exocytosis from permeabilized pancreatic acini, indicating that dequenching is detecting a physiologically relevant process. In particular, exocytotic membrane fusion both in vitro and in permeabilized acini is stimulated by Ca2+ with an EC50 of 1 mu M, and enhanced by guanosine 5'-0-(3-thiotriphosphate) (GTP gamma S) with an EC50 of 10-20 mu M. Another parallel between the two systems is the incomplete inhibition of fusion/exocytosis by tetanus toxin, despite complete cleavage of synaptobrevin 2 on the zymogen granule membrane. Recently, the in vitro assay for membrane fusion has been used to indicate a role in the control of exocytosis for syncollin, a granule membrane protein that binds to syntaxin in a Ca2+-sensitive manner. The assay should continue to provide information about this exocytotic membrane fusion event in the future. (C) 1998 Academic Press.
引用
收藏
页码:209 / 214
页数:6
相关论文
共 34 条
[1]   RECONSTITUTION OF THE TRANSPORT OF PROTEIN BETWEEN SUCCESSIVE COMPARTMENTS OF THE GOLGI MEASURED BY THE COUPLED INCORPORATION OF N-ACETYLGLUCOSAMINE [J].
BALCH, WE ;
DUNPHY, WG ;
BRAELL, WA ;
ROTHMAN, JE .
CELL, 1984, 39 (02) :405-416
[2]   VESICULAR TRANSPORT BETWEEN THE ENDOPLASMIC-RETICULUM AND THE GOLGI STACK REQUIRES THE NEM-SENSITIVE FUSION PROTEIN [J].
BECKERS, CJM ;
BLOCK, MR ;
GLICK, BS ;
ROTHMAN, JE ;
BALCH, WE .
NATURE, 1989, 339 (6223) :397-398
[3]   SEMI-INTACT CELLS PERMEABLE TO MACROMOLECULES - USE IN RECONSTITUTION OF PROTEIN-TRANSPORT FROM THE ENDOPLASMIC-RETICULUM TO THE GOLGI-COMPLEX [J].
BECKERS, CJM ;
KELLER, DS ;
BALCH, WE .
CELL, 1987, 50 (04) :523-534
[4]   PURIFICATION OF AN N-ETHYLMALEIMIDE-SENSITIVE PROTEIN CATALYZING VESICULAR TRANSPORT [J].
BLOCK, MR ;
GLICK, BS ;
WILCOX, CA ;
WIELAND, FT ;
ROTHMAN, JE .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1988, 85 (21) :7852-7856
[5]   FUSION BETWEEN ENDOCYTIC VESICLES IN A CELL-FREE SYSTEM [J].
BRAELL, WA .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1987, 84 (05) :1137-1141
[6]   INVITRO RECONSTITUTION OF EXOCYTOSIS FROM PLASMA-MEMBRANE AND ISOLATED SECRETORY VESICLES [J].
CRABB, JH ;
JACKSON, RC .
JOURNAL OF CELL BIOLOGY, 1985, 101 (06) :2263-2273
[7]   VESICLE FUSION FOLLOWING RECEPTOR-MEDIATED ENDOCYTOSIS REQUIRES A PROTEIN ACTIVE IN GOLGI TRANSPORT [J].
DIAZ, R ;
MAYORGA, LS ;
WEIDMAN, PJ ;
ROTHMAN, JE ;
STAHL, PD .
NATURE, 1989, 339 (6223) :398-400
[8]   SYNAPTOBREVIN BINDING TO SYNAPTOPHYSIN - A POTENTIAL MECHANISM FOR CONTROLLING THE EXOCYTOTIC FUSION MACHINE [J].
EDELMANN, L ;
HANSON, PI ;
CHAPMAN, ER ;
JAHN, R .
EMBO JOURNAL, 1995, 14 (02) :224-231
[9]   SYNTHETIC PEPTIDES OF THE RAB3-EFFECTOR DOMAIN STIMULATE A MEMBRANE-FUSION EVENT INVOLVED IN REGULATED EXOCYTOSIS [J].
EDWARDSON, JM ;
MACLEAN, CM ;
LAW, GJ .
FEBS LETTERS, 1993, 320 (01) :52-56
[10]   RAT PANCREATIC ACINI PERMEABILIZED WITH STREPTOLYSIN-O SECRETE AMYLASE AT CA-2+ CONCENTRATIONS IN THE MICROMOLAR RANGE, WHEN PROVIDED WITH ATP AND GTP-GAMMA-S [J].
EDWARDSON, JM ;
VICKERY, C ;
CHRISTY, LJ .
BIOCHIMICA ET BIOPHYSICA ACTA, 1990, 1053 (01) :32-36
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