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The highly conserved motif of Saccharomyces cerevisiae H
Volume 270,
Number 15,
Issue of April 14, pp. 8655-8659, 1995
©1995 by The American Society for Biochemistry and Molecular Biology, Inc.
-ATPase
-ATPase
KGAP has been proposed to
participate in the formation of the phosphorylated intermediate during
the catalytic cycle (Portillo, F., and Serrano, R. (1988) EMBO J. 7, 1793-1798). In addition, Lys-474 is the FITC binding site
of the yeast enzyme (Portillo, F. and Serrano, R. (1989) Eur. J.
Biochem. 186, 501-507). We have performed an intragenic
suppressor analysis of the K474R mutation to identify the interacting
regions involved in these functions. Random in vitro mutagenesis of the K474R allele resulted in seven suppressor
(second-site) mutations. One mutation (V396I), located 18 residues away
from the Asp-378 residue, which is phosphorylated during catalysis, is
allele-specific. This provides genetic evidence of a direct interaction
between the KGAP motif and the phosphorylation domain during the
catalytic cycle. Three mutations (V484I, V484I/E485K, and E485K/E486K)
are located near Lys-474 and may compense the structural alteration
introduced by the K474R mutation. Two substitutions at the end of the
predicted transmembrane stretch 2 (A165V and V169I/D170N) and another
in the predicted ATP binding domain (P536L) may act as
allele-nonspecific suppressors, as they are also able to suppress a
mutation at the enzyme's carboxyl terminus.
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