Genotypic versus phenotypic characterization, with respect to susceptibility and identification, of 17 clinical isolates of Staphylococcus lugdunensis

doi:10.1093/jac/dki227

JAC Advance Access published online on July 1, 2005
Journal of Antimicrobial Chemotherapy, doi:10.1093/jac/dki227

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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@oupjournals.org
Received February 4, 2005
Revised May 30, 2005
Accepted June 2, 2005

Original article

Genotypic versus phenotypic characterization, with respect to susceptibility and identification, of 17 clinical isolates of Staphylococcus lugdunensis

María Mateo ¹, Juan-Ramón Maestre ¹, Lorenzo Aguilar ², Fabio Cafini ², Pilar Puente ¹, Paloma Sánchez ¹, Luis Alou ², María-José Giménez ², and José Prieto ²^*

¹ Microbiology Department, Hospital Gómez-Ulla, Gta. del Ejército s/n, 28007 Madrid, Spain
² Microbiology Department, School of Medicine, Universidad Complutense, Avda. Complutense s/n, 28040 Madrid, Spain

^* To whom correspondence should be addressed.
José Prieto, E-mail: jprieto{at}med.ucm.es

Abstract

Objectives: To compare different methods for the identificationand determination of susceptibility to penicillin and methicillinof Staphylococcus lugdunensis.

Methods: Seventeen clinical isolatesof S. lugdunensis (identified by PCR amplification and sequencingof the rpoB gene) were studied using the ATB32-Staph, Crystal,Vitek 2 and Wider commercial systems. The clumping factor testand the tube coagulase test were also performed. ${beta}$ -Lactamaseproduction was studied by chromogenic methods. Methicillin resistancewas phenotypically studied by the MRSA slide latex agglutinationtest, growth in MRSA agar, and the Vitek 2 and Wider systems(based on oxacillin MIC), and genotypically studied by detectionof the mecA gene by PCR.

Results: The clumping factor test wasnegative in 35.3% of strains. All isolates were correctly identifiedto species level by the ATB32-Staph system. Species misidentificationrates were 5.9%, 23.5% and 29.4% with the Crystal, the Vitek2 and the Wider systems, respectively, mostly as Staphylococcushaemolyticus. ${beta}$ -Lactamase was present in 11.8% of strains. Whereas76.5% and 47.1% of strains exhibited oxacillin resistance (MICrange 0.5-2 mg/L) by the Vitek 2 system and the Wider system,respectively, none of the strains was positive in the MRSA slidelatex agglutination test or grew in MRSA agar. All strains lackedthe mecA gene.

Conclusions: The clumping factor test and somecommercial systems may misidentify S. lugdunensis. Oxacillinresistance detected by commercial systems is not indicativeof the presence of the mecA gene. These facts, together with ${beta}$ -lactamase production, may preclude adequate treatment of infectionsby this virulent coagulase-negative Staphylococcus.

Keywords: S. lugdunensis; methicillin resistance; ${beta}$ -lactamases; mecA gene; clumping factor.

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