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Vol. 11, Issue 4, 1345-1356, April 2000
§ and
*The Physiological Laboratory, University of Liverpool, Liverpool
L69 3BX, United Kingdom; and An evolutionarily ancient mechanism is used for intracellular
membrane fusion events ranging from endoplasmic reticulum-Golgi traffic in yeast to synaptic vesicle exocytosis in the human brain. At
the heart of this mechanism is the core complex of
N-ethylmaleimide-sensitive fusion protein (NSF), soluble
NSF attachment proteins (SNAPs), and SNAP receptors (SNAREs). Although
these proteins are accepted as key players in vesicular traffic, their
molecular mechanisms of action remain unclear. To illuminate important
structure-function relationships in NSF, a screen for dominant
negative mutants of yeast NSF (Sec18p) was undertaken. This involved
random mutagenesis of a GAL1-regulated
SEC18 yeast expression plasmid. Several dominant negative alleles were identified on the basis of galactose-inducible growth arrest, of which one, sec18-109,
was characterized in detail. The
sec18-109 phenotype (abnormal membrane trafficking
through the biosynthetic pathway, accumulation of a membranous tubular network, growth suppression, increased cell density) is due to a single
A-G substitution in SEC18 resulting in a missense
mutation in Sec18p (Thr394Department of Biomedical
Sciences, University of Edinburgh Medical School, Edinburgh, EH8 9XD,
United Kingdom
Pro). Thr394 is
conserved in most AAA proteins and indeed forms part of the minimal AAA
consensus sequence that serves as a signature of this large protein
family. Analysis of recombinant Sec18-109p indicates that the mutation
does not prevent hexamerization or interaction with yeast 
-SNAP
(Sec17p), but instead results in undetectable ATPase activity that
cannot be stimulated by Sec17p. This suggests a role for the AAA
protein consensus sequence in regulating ATP hydrolysis. Furthermore, this approach of screening for dominant negative mutants in yeast can
be applied to other conserved proteins so as to highlight important
functional domains in their mammalian counterparts.
These authors contributed equally to this work.
§
Present address: Albert Einstein College of
Medicine, Department of Developmental and Molecular Biology, Bronx, NY 10461.
Corresponding author. E-mail address:
amorgan{at}liverpool.ac.uk.
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  L. E. P. Dietrich, T. J. LaGrassa, J. Rohde, M. Cristodero, C. T. A. Meiringer, and C. Ungermann ATP-independent Control of Vac8 Palmitoylation by a SNARE Subcomplex on Yeast Vacuoles J. Biol. Chem., April 15, 2005; 280(15): 15348 - 15355. [Abstract] [Full Text] [PDF]
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A. P. May, S. W. Whiteheart, and W. I. Weis Unraveling the Mechanism of the Vesicle Transport ATPase NSF, the N-Ethylmaleimide-sensitive Factor J. Biol. Chem., June 15, 2001; 276(25): 21991 - 21994. [Full Text] [PDF]
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