Affiliation:
1. Center for Pharmaceutical Biotechnology, University of Illinois, Chicago, Illinois 60607
Abstract
ABSTRACT
Bacterial genes defining intrinsic resistance to antibiotics encode proteins that can be targeted by antibiotic potentiators. To find such genes, a transposon insertion library of
Acinetobacter baylyi
was screened with subinhibitory concentrations of various antibiotics to find supersusceptible mutants. A DNA microarray printer was used to replica plate 10,000 individual library clones to select mutants unable to grow at 1/10 the MICs of 12 different antibiotics. Transposon insertions in 11 genes were found to cause an eightfold or higher hypersusceptibility to at least one antibiotic. Most of the mutants identified exhibited hypersusceptibility to β-lactam antibiotics. These included mutants with disruptions of genes encoding proteins involved in efflux (
acrB
and
oprM
) as well as genes pertaining to peptidoglycan synthesis and modification (
ampD
,
mpl
, and
pbpG
). However, disruptions of genes encoding proteins with seemingly unrelated functions (
gph
,
argH
,
hisF, and ACIAD0795
) can also render cells hypersusceptible to β-lactam antibiotics. A knockout of
gshA
, involved in glutathione biosynthesis, enhanced the susceptibility to metronidazole, while a knockout of
recD
, involved in recombination and repair, made the bacteria hypersusceptible to ciprofloxacin. Disruption of
acrB
in
Escherichia coli
rendered the cells hypersusceptible to several antibiotics. However, knockout mutants of other homologous genes in
E. coli
showed no significant changes in antibiotic MICs, indicating that the intrinsic resistance genes are species specific.
Publisher
American Society for Microbiology
Subject
Infectious Diseases,Pharmacology (medical),Pharmacology
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