Evaluation of Etest and MICRONAUT-AM Assay for Antifungal Susceptibility Testing of Candida auris: Underestimation of Fluconazole Resistance by MICRONAUT-AM and Overestimation of Amphotericin B Resistance by Etest

Author:

Asadzadeh Mohammad1ORCID,Ahmad Suhail1ORCID,Alfouzan Wadha12ORCID,Al-Obaid Inaam3,Spruijtenburg Bram45ORCID,Meijer Eelco F. J.45,Meis Jacques F.56ORCID,Mokaddas Eiman17

Affiliation:

1. Department of Microbiology, Faculty of Medicine, Kuwait University, Safat 13110, Kuwait

2. Microbiology Department, Farwaniya Hospital, Farwaniya 81004, Kuwait

3. Microbiology Department, Al-Sabah Hospital, Shuwaikh 70031, Kuwait

4. Canisius Wilhelmina Hospital (CWZ)/Dicoon, 6532 Nijmegen, The Netherlands

5. Radboudumc-CWZ Center of Expertise for Mycology, 6500 Nijmegen, The Netherlands

6. Institute of Translational Research, Cologne Excellence Cluster on Cellular Stress Responses in Aging-Associated Diseases (CECAD) and Excellence Center for Medical Mycology, University of Cologne, 50923 Cologne, Germany

7. Microbiology Department, Ibn-Sina Hospital, Shuwaikh 70031, Kuwait

Abstract

Multidrug-resistant Candida auris has recently caused major outbreaks in healthcare facilities. Rapid and accurate antifungal susceptibility testing (AST) of C. auris is crucial for proper management of invasive infections. The Commercial Sensititre Yeast One and Vitek 2 methods underestimate or overestimate the resistance of C. auris to fluconazole and amphotericin B (AMB). This study evaluated the AST results of C. auris against fluconazole and AMB by gradient-MIC-strip (Etest) and broth microdilution-based MICRONAUT-AM-EUCAST (MCN-AM) assays. Clinical C. auris isolates (n = 121) identified by phenotypic and molecular methods were tested. Essential agreement (EA, ±1 two-fold dilution) between the two methods and categorical agreement (CA) based on the Centers for Disease Control and Prevention’s (CDC’s) tentative resistance breakpoints were determined. Fluconazole resistance-associated mutations were detected by PCR-sequencing of ERG11. All isolates identified as C. auris belonged to South Asian clade I and contained the ERG11 Y132F or K143R mutation. The Etest–MCN-AM EA was poor (33%) for fluconazole and moderate (76%) for AMB. The CA for fluconazole was higher (94.2%, 7 discrepancies) than for AMB (91.7%, 10 discrepancies). Discrepancies were reduced when an MCN-AM upper-limit value of 4 µg/mL for fluconazole-susceptible C. auris and an Etest upper-limit value of 8 µg/mL for the wild type for AMB were used. Our data show that resistance to fluconazole was underestimated by MCN-AM, while resistance to AMB was overestimated by Etest when using the CDC’s tentative resistance breakpoints of ≥32 µg/mL for fluconazole and ≥2 µg/mL for AMB. Method-specific resistance breakpoints should be devised for accurate AST of clinical C. auris isolates for proper patient management.

Publisher

MDPI AG

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