Antibiotic susceptibilities of Legionella pneumophila strain Paris in THP-1 cells as determined by real-time PCR assay

doi:10.1093/jac/dki141

JAC Advance Access originally published online on May 9, 2005
Journal of Antimicrobial Chemotherapy 2005 55(6):866-871; doi:10.1093/jac/dki141

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© The Author 2005. Published by Oxford University Press on behalf of the British Society for Antimicrobial Chemotherapy. All rights reserved. For Permissions, please e-mail: journals.permissions{at}oupjournals.org

Antibiotic susceptibilities of Legionella pneumophila strain Paris in THP-1 cells as determined by real-time PCR assay

N. Roch and M. Maurin^*

CNRS UMR 5163, Université Joseph Fourier, Faculté de Médecine, Bâtiment Jean Roget, 38700 La Tronche, France

*Corresponding author. Tel: +33-4-76-76-54-79; Fax: +33-4-76-76-59-12; Email: mmaurin{at}chu-grenoble.fr

Objectives: Legionella species are facultative intracellularbacteria. Evaluation of the activity of antibiotics againstintracellular L. pneumophila is more predictive of their invivo efficacy than MICs as determined in axenic medium. However,current methodologies are based on cfu count determination,and are tedious because of the slow growth of Legionella spp.We investigated antibiotic susceptibilities of L. pneumophilastrain Paris in THP-1-derived macrophages, using a real-timePCR assay for evaluation of bacterial growth.

Methods: Intracellular activities of seven antibiotic compoundsagainst two human isolates of L. pneumophila strain Paris weredetermined in THP-1-derived macrophages in vitro. Bacterialgrowth was evaluated using either cfu methodology or a real-timePCR protocol targeting the mip gene.

Results: Bacterial titres as determined using real-time PCRwere well correlated with cfu counts. Antibiotic susceptibilitiesfor the two L. pneumophila isolates tested were comparable whenusing either of the two techniques. MICs were also similar tothose previously reported for other L. pneumophila serogroup1 strains. In particular, rifampicin and the fluoroquinoloneswere the most active compounds, both in extracellular mediumand in THP-1 cells. Real-time PCR, however, was much less laboriousthan the traditional cfu method.

Conclusions: Real-time PCR is better adapted than cfu-basedmethods to evaluating the antibiotic susceptibilities of largeseries of Legionella strains to newer antibiotic compounds.

Keywords: antibacterials , intracellular , macrophages , quantitative PCR

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