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Volume 271,
Number 15,
Issue of April 12, 1996 pp. 9120-9128
©1996 by The American Society for Biochemistry and Molecular Biology, Inc.
Cloning and
Characterization of the Yeast HEM14 Gene Coding for
Protoporphyrinogen Oxidase, the Molecular Target of Diphenyl
Ether-type Herbicides
(Received for publication, December 18,
1995)
Jean-Michel
Camadro ,
Pierre
Labbe
Protoporphyrinogen oxidase, which catalyzes the oxygen-dependent
aromatization of protoporphyrinogen IX to protoporphyrin IX, is the
molecular target of diphenyl ether type herbicides. The structural gene
for the yeast protoporphyrinogen oxidase, HEM14, was isolated
by functional complementation of a hem14-1 protoporphyrinogen
oxidase-deficient yeast mutant, using a novel one-step colored
screening procedure to identify heme-synthesizing cells. The hem14-1 mutation was genetically linked to URA3, a
marker on chromosome V, and HEM14 was physically mapped on the
right arm of this chromosome, between PRP22 and FAA2.
Disruption of the HEM14 gene leads to protoporphyrinogen
oxidase deficiency in vivo (heme deficiency and accumulation
of heme precursors), and in vitro (lack of immunodetectable
protein or enzyme activity). The HEM14 gene encodes a
539-amino acid protein (59,665 Da; pI 9.3) containing an
ADP-  -binding fold similar to those of several other
flavoproteins. Yeast protoporphyrinogen oxidase was somewhat similar to
the HemY gene product of Bacillus subtilis and to the
human and mouse protoporphyrinogen oxidases. Studies on
protoporphyrinogen oxidase overexpressed in yeast and purified as
wild-type enzyme showed that (i) the NH -terminal
mitochondrial targeting sequence of protoporphyrinogen oxidase is not
cleaved during importation; (ii) the enzyme, as purified, had a typical
flavin semiquinone absorption spectrum; and (iii) the enzyme was
strongly inhibited by diphenyl ether-type herbicides and readily
photolabeled by a diazoketone derivative of tritiated acifluorfen. The
mutant allele hem14-1 contains two mutations, L422P and K424E,
responsible for the inactive enzyme. Both mutations introduced
independently in the wild-type HEM14 gene completely
inactivated the protein when analyzed in an Escherichia coli expression system.

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Copyright © 1996 by the American Society for Biochemistry and Molecular Biology.
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