Prevalence of qnr genes among extended-spectrum β-lactamase-producing enterobacterial isolates in Barcelona, Spain

Objectives To evaluate the presence of qnr genes among enterobacterial isolates carrying extended-spectrum β-lactamases (ESBLs) in Barcelona, Spain. Methods Screening for the qnrA, qnrB and qnrS genes was carried out by PCR amplification with specific primers in 305 non-duplicate, clinically relevan...

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Published in:Journal of antimicrobial chemotherapy 2008-02, Vol.61 (2), p.291-295
Main Authors: Lavilla, S., González-López, J. J., Sabaté, M., García-Fernández, A., Larrosa, M. N., Bartolomé, R. M., Carattoli, A., Prats, G.
Format: Article
Language:English
Subjects:
Antibiotics. Antiinfectious agents. Antiparasitic agents
Bacterial Proteins - genetics
Bacterial Proteins - isolation & purification
beta-Lactamases - genetics
beta-Lactamases - isolation & purification
Biological and medical sciences
Enterobacter cloacae
enterobacteria
Enterobacteriaceae - genetics
Enterobacteriaceae - isolation & purification
ESBLs
Escherichia coli
Escherichia coli Proteins - genetics
Escherichia coli Proteins - isolation & purification
Humans
Klebsiella pneumoniae
Medical sciences
Pharmacology. Drug treatments
Prevalence
quinolones
Spain - epidemiology
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Summary:Objectives To evaluate the presence of qnr genes among enterobacterial isolates carrying extended-spectrum β-lactamases (ESBLs) in Barcelona, Spain. Methods Screening for the qnrA, qnrB and qnrS genes was carried out by PCR amplification with specific primers in 305 non-duplicate, clinically relevant ESBL-producing enterobacterial isolates obtained from February 2003 to August 2004. ESBLs from all qnr-positive isolates were characterized by isoelectric focusing, PCR amplification and DNA sequencing. Plasmid analysis was performed by S1 digestion and hybridization with specific probes for the qnr and bla genes. Plasmids containing qnr genes were transferred by conjugation or transformation. The genetic environment of qnrA1 in selected isolates was characterized by cloning experiments. Results Fifteen isolates, each from a different individual, carried qnr. Among them, 14 had qnrA1 (6 Klebsiella pneumoniae, 6 Enterobacter cloacae and 2 Escherichia coli isolates) and 1 had qnrS1 (K. pneumoniae). None of the isolates carried qnrB. Among the qnrA1-carrying isolates, 10 possessed both blaCTX-M-9 and blaSHV-12, 2 had both blaCTX-M-9 and blaSHV-92 and 2 had blaCTX-M-9 alone. The isolate with qnrS1 possessed blaSHV-12. The qnrA1 and ESBL genes were located together on plasmids ranging in size from 40 to 320 kb. qnrS1 and blaSHV-12 were not located on the same plasmid. Transfer of quinolone resistance was successfully achieved from all but three isolates. The cloned region surrounding qnrA in two K. pneumoniae isolates revealed a novel genetic organization. Conclusions The prevalence of qnr among enterobacterial clinical isolates carrying ESBLs between 2003 and 2004 in Barcelona was 4.9%. qnrA1 was the most prevalent, whereas only one qnrS and no qnrB were detected.
ISSN:0305-7453
1460-2091
DOI:10.1093/jac/dkm448