The secondary resistome of multidrug-resistant Klebsiella pneumoniae

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作者
Bimal Jana
Amy K. Cain
William T. Doerrler
Christine J. Boinett
Maria C. Fookes
Julian Parkhill
Luca Guardabassi
机构
[1] Faculty of Health and Medical Sciences,Department of Veterinary Disease Biology
[2] University of Copenhagen,Department of Biomedical Sciences
[3] Ross University School of Veterinary Medicine,Department of Biological Sciences
[4] Basseterre,undefined
[5] St Kitts,undefined
[6] Pathogen Genomics,undefined
[7] Wellcome Trust Sanger Institute,undefined
[8] Louisiana State University,undefined
[9] Present address: Liverpool School of Tropical Medicine,undefined
[10] Malawi-Liverpool-Wellcome Trust Clinical Research Programme,undefined
[11] Blantyre,undefined
[12] Malawi.,undefined
[13] Present address: Hospital for Tropical Diseases,undefined
[14] Wellcome Trust Major Overseas Programme,undefined
[15] Oxford University Clinical Research Unit,undefined
[16] Ho Chi Minh City,undefined
[17] Vietnam.,undefined
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Scientific Reports | / 7卷
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摘要
Klebsiella pneumoniae causes severe lung and bloodstream infections that are difficult to treat due to multidrug resistance. We hypothesized that antimicrobial resistance can be reversed by targeting chromosomal non-essential genes that are not responsible for acquired resistance but essential for resistant bacteria under therapeutic concentrations of antimicrobials. Conditional essentiality of individual genes to antimicrobial resistance was evaluated in an epidemic multidrug-resistant clone of K. pneumoniae (ST258). We constructed a high-density transposon mutant library of >430,000 unique Tn5 insertions and measured mutant depletion upon exposure to three clinically relevant antimicrobials (colistin, imipenem or ciprofloxacin) by Transposon Directed Insertion-site Sequencing (TraDIS). Using this high-throughput approach, we defined three sets of chromosomal non-essential genes essential for growth during exposure to colistin (n = 35), imipenem (n = 1) or ciprofloxacin (n = 1) in addition to known resistance determinants, collectively termed the “secondary resistome”. As proof of principle, we demonstrated that inactivation of a non-essential gene not previously found linked to colistin resistance (dedA) restored colistin susceptibility by reducing the minimum inhibitory concentration from 8 to 0.5 μg/ml, 4-fold below the susceptibility breakpoint (S ≤ 2 μg/ml). This finding suggests that the secondary resistome is a potential target for developing antimicrobial “helper” drugs that restore the efficacy of existing antimicrobials.
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