Mechanisms of Azole Resistance in a Clinical Isolate of Candida tropicalis

doi:10.1128/AAC.49.11.4608-4615.2005

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Antimicrobial Agents and Chemotherapy, November 2005, p. 4608-4615, Vol. 49, No. 11
0066-4804/05/$08.00+0 doi:10.1128/AAC.49.11.4608-4615.2005
Copyright © 2005, American Society for Microbiology. All Rights Reserved.

Mechanisms of Azole Resistance in a Clinical Isolate of Candida tropicalis

Patrick Vandeputte,¹^* Gérald Larcher,¹ Thierry Bergès,² Gilles Renier,³ Dominique Chabasse,¹ and Jean-Philippe Bouchara¹

Groupe d'Etude des Interactions Hôte-Parasite, UPRES-EA 3142, Laboratoire de Parasitologie-Mycologie,¹ Laboratoire d'Immunologie, Centre Hospitalier Universitaire, 49933 Angers Cedex 9,³ Laboratoire de Génétique de la Levure, CNRS UMR 6161, Faculté des Sciences, 86022 Poitiers Cedex, France²

Received 6 January 2005/ Returned for modification 1 July 2005/ Accepted 24 August 2005

Azole resistance has been insufficiently investigated in theyeast Candida tropicalis. Here we determined the molecular mechanismsresponsible for azole resistance in a clinical isolate of thispathogenic yeast. Antifungal susceptibility testing performedby a disk diffusion method showed resistance or markedly decreasedsusceptibility to azoles, which was confirmed by determinationof MICs. Considering the relationship between azole susceptibilityand the respiration reported for other yeast species, the respiratoryactivity of this isolate was investigated. Flow cytometry usingrhodamine 123 and oxygraphy demonstrated an increased respiratoryactivity, which was not linked to an overexpression or increasednumber of copies of the mitochondrial genome. Among previouslydescribed resistance mechanisms, an increased activity of effluxpumps was investigated by flow cytometry using rhodamine 6G.However, the efflux of rhodamine 6G was lower in the resistantisolate than in susceptible ones. Likewise, real-time reversetranscription-PCR quantification of the expression of C. tropicalisMDR1 (CtMDR1), which encodes an efflux protein belonging tothe major facilitator superfamily, did not show overexpressionof this gene. In contrast, the resistant isolate overexpressedthe CtERG11 gene coding for lanosterol 14 ${alpha}$ -demethylase. Thiswas in agreement with the larger amount of ergosterol foundin this isolate. Moreover, sequencing of CtERG11 showed a pointmutation leading to a tyrosine substitution in the protein sequence,which might lead to decreased binding affinity for azoles. Inconclusion, overexpression of CtERG11 associated with a missensemutation in this gene seemed to be responsible for the acquiredazole resistance of this clinical isolate.

* Corresponding author. Mailing address: Groupe d'Etude des Interactions Hôte-Parasite, UPRES-EA 3142, Laboratoire de Parasitologie-Mycologie, Centre Hospitalier Universitaire, 4 rue Larrey, 49933 Angers Cedex 9, France. Phone: 33 02 41 35 34 72. Fax: 33 02 41 35 36 16. E-mail: Patrick.Vandeputte{at}etud.univ-angers.fr.

Antimicrobial Agents and Chemotherapy, November 2005, p. 4608-4615, Vol. 49, No. 11
0066-4804/05/$08.00+0 doi:10.1128/AAC.49.11.4608-4615.2005
Copyright © 2005, American Society for Microbiology. All Rights Reserved.

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