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Screening of a Leptospira biflexa mutant library to identify genes involved in ethidium bromide tolerance
H. Pětrošová, M. Picardeau,
Language English Country United States
Document type Journal Article, Research Support, Non-U.S. Gov't
NLK
Free Medical Journals
from 1976 to 6 months ago
PubMed Central
from 1976 to 6 months ago
Europe PubMed Central
from 1976 to 6 months ago
Open Access Digital Library
from 1953-01-01
PubMed
25063661
DOI
10.1128/aem.01619-14
Knihovny.cz E-resources
- MeSH
- Anti-Infective Agents pharmacology MeSH
- Drug Resistance, Bacterial genetics MeSH
- Bacterial Proteins genetics MeSH
- Biological Transport MeSH
- Ethidium pharmacology MeSH
- Phenotype MeSH
- Gene Library MeSH
- Mutagenesis, Insertional MeSH
- Leptospira genetics physiology MeSH
- Membrane Transport Proteins genetics MeSH
- Microbial Sensitivity Tests MeSH
- Operon genetics MeSH
- Drug Tolerance genetics MeSH
- DNA Transposable Elements genetics MeSH
- Publication type
- Journal Article MeSH
- Research Support, Non-U.S. Gov't MeSH
Leptospira spp. are spirochete bacteria comprising both pathogenic and free-living species. The saprophyte L. biflexa is a model bacterium for studying leptospiral biology due to relative ease of culturing and genetic manipulation. In this study, we constructed a library of 4,996 random transposon mutants in L. biflexa. We screened the library for increased susceptibility to the DNA intercalating agent, ethidium bromide (EtBr), in order to identify genetic determinants that reduce L. biflexa susceptibility to antimicrobial agents. By phenotypic screening, using subinhibitory EtBr concentrations, we identified 29 genes that, when disrupted via transposon insertion, led to increased sensitivity of the bacteria to EtBr. At the functional level, these genes could be categorized by function as follows: regulation and signaling (n=11), transport (n=6), membrane structure (n=5), stress response (n=2), DNA damage repair (n=1), and other processes (n=3), while 1 gene had no predicted function. Genes involved in transport (including efflux pumps) and regulation (two-component systems, anti-sigma factor antagonists, etc.) were overrepresented, demonstrating that these genes are major contributors to EtBr tolerance. This finding suggests that transport genes which would prevent EtBr to enter the cell cytoplasm are critical for EtBr resistance. We identified genes required for the growth of L. biflexa in the presence of sublethal EtBr concentration and characterized their potential as antibiotic resistance determinants. This study will help to delineate mechanisms of adaptation to toxic compounds, as well as potential mechanisms of antibiotic resistance development in pathogenic L. interrogans.
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