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Volume 270,
Number 8,
Issue of February 24, 1995 pp. 4076-4087
©1995 by The American Society for Biochemistry and Molecular Biology, Inc.
Purification and Characterization
of an Isoaspartyl Dipeptidase from Escherichia coli
(Received for publication, June 27, 1994; and in revised form, November 28, 1994)
Jonathan D.
Gary ,
Steven
Clarke
We have identified a gene (iadA) in Escherichia
coli encoding a 41-kDa polypeptide that catalyzes the hydrolytic
cleavage of L-isoaspartyl, or L- -aspartyl,
dipeptides. We demonstrate at least a 3000-fold purification of the
enzyme to homogeneity from crude cytosol. From the amino-terminal amino
acid sequence obtained from this preparation, we designed an
oligonucleotide that allowed us to map the gene to the 98-min region of
the chromosome and to clone and obtain the DNA sequence of the gene.
Examination of the deduced amino acid sequence revealed no similarities
to other peptidases or proteases, while a marked similarity was found
with several dihydroorotases and imidases, reflecting the similarity in
the structures of the substrates for these enzymes. Using an E.
coli strain containing a plasmid overexpressing this gene, we were
able to purify sufficient amounts of the dipeptidase to characterize
its substrate specificity. We also examined the phenotype of two E.
coli strains where this isoaspartyl dipeptidase gene was deleted.
We inserted a chloramphenicol cassette into the disrupted coding region
of iadA in both a parent strain (MC1000) and a derivative
strain (CL1010) lacking pcm, the gene encoding the L-isoaspartyl methyltransferase involved in the repair of
isomerized proteins. We found that the iadA deletion does not
result in reduced stationary phase or heat shock survival. Analysis of
isoaspartyl dipeptidase activity in the deletion strain revealed a
second activity of lower native molecular weight that accounts for
approximately 31% of the total activity in the parent strain MC1000.
The presence of this second activity may account for the absence of an
observable phenotype in the iadA mutant cells.

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Copyright © 1995 by the American Society for Biochemistry and Molecular Biology.
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