Affiliation:
1. Cell Biology and Metabolism Branch, National Institute of Child Health and Human Development, National Institutes of Health, Bethesda, Maryland 20892,1 and
2. Biochemical Science and Engineering, Central Research and Development, E. I. DuPont de Nemours and Company, Wilmington, Delaware 19880-03282
Abstract
ABSTRACT
The genome-wide transcription profile of
Escherichia coli
cells treated with hydrogen peroxide was examined with a DNA microarray composed of 4,169
E. coli
open reading frames. By measuring gene expression in isogenic wild-type and
oxyR
deletion strains, we confirmed that the peroxide response regulator OxyR activates most of the highly hydrogen peroxide-inducible genes. The DNA microarray measurements allowed the identification of several new OxyR-activated genes, including the
hemH
heme biosynthetic gene; the six-gene
suf
operon, which may participate in Fe-S cluster assembly or repair; and four genes of unknown function. We also identified several genes, including
uxuA,
encoding mannonate hydrolase, whose expression might be repressed by OxyR, since their expression was elevated in the Δ
oxyR
mutant strain. In addition, the induction of some genes was found to be OxyR independent, indicating the existence of other peroxide sensors and regulators in
E. coli
. For example, the
isc
operon, which specifies Fe-S cluster formation and repair activities, was induced by hydrogen peroxide in strains lacking either OxyR or the superoxide response regulators SoxRS. These results expand our understanding of the oxidative stress response and raise interesting questions regarding the nature of other regulators that modulate gene expression in response to hydrogen peroxide.
Publisher
American Society for Microbiology
Subject
Molecular Biology,Microbiology
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