Detection of heterogeneous vancomycin intermediate resistance in MRSA isolates from Latin America

Author:

Castro Betsy E1,Berrio Maritza2,Vargas Monica L1,Carvajal Lina P1,Millan Lina V1,Rios Rafael1,Hernandez Angie K1,Rincon Sandra1,Cubides Paola1,Forero Erika1,Dinh An3,Seas Carlos4,Munita Jose M356,Arias Cesar A1378,Reyes Jinnethe13,Diaz Lorena136

Affiliation:

1. Molecular Genetics and Antimicrobial Resistance Unit, International Center for Microbial Genomics, Universidad El Bosque, Bogotá, Colombia

2. Instituto Nacional de Salud, Bogotá, Colombia

3. Center for Antimicrobial Resistance and Microbial Genomics, McGovern Medical School, University of Texas Health Science Center, Houston, Texas, USA

4. Universidad Peruana Cayetano Heredia, Lima, Peru

5. Genomics and Resistant Microbes (GeRM) Group, Clínica Alemana de Santiago, Universidad del Desarrollo School of Medicine, Santiago, Chile

6. Millennium Initiative for Collaborative Research On Bacterial Resistance (MICROB-R), Santiago, Chile

7. Division of Infectious Diseases, Department of Internal Medicine, McGovern Medical School, University of Texas Health Science Center, Houston, Texas, USA

8. Center for Infectious Diseases, School of Public Health, University of Texas McGovern Medical School at Houston, Houston, Texas, USA

Abstract

AbstractBackgroundVancomycin is a common first-line option for MRSA infections. The heterogeneous vancomycin-intermediate Staphylococcus aureus (hVISA) phenotype is associated with therapeutic failure. However, hVISA isolates are usually reported as vancomycin susceptible by routine susceptibility testing procedures.ObjectivesTo detect and characterize the hVISA phenotype in MRSA isolates causing infections in nine Latin American countries.MethodsWe evaluated a total of 1189 vancomycin-susceptible MRSA isolates recovered during 2006–08 and 2011–14. After an initial screening of hVISA using glycopeptide-supplemented agar strategies, the detection of hVISA was performed by Etest (GRD) and Macro-method (MET). Isolates deemed to be hVISA were subjected to population analysis profile/AUC (PAP/AUC) and WGS for further characterization. Finally, we interrogated alterations in predicted proteins associated with the development of the VISA phenotype in both hVISA and vancomycin-susceptible S. aureus (VSSA) genomes.ResultsA total of 39 MRSA isolates (3.3%) were classified as hVISA (1.4% and 5.6% in MRSA recovered from 2006–08 and 2011–14, respectively). Most of the hVISA strains (95%) belonged to clonal complex (CC) 5. Only 6/39 hVISA isolates were categorized as hVISA by PAP/AUC, with 6 other isolates close (0.87–0.89) to the cut-off (0.9). The majority of the 39 hVISA isolates exhibited the Leu-14→Ile (90%) and VraT Glu-156→Gly (90%) amino acid substitutions in WalK. Additionally, we identified 10 substitutions present only in hVISA isolates, involving WalK, VraS, RpoB and RpoC proteins.ConclusionsThe hVISA phenotype exhibits low frequency in Latin America. Amino acid substitutions in proteins involved in cell envelope homeostasis and RNA synthesis were commonly identified. Our results suggest that Etest-based methods are an important alternative for the detection of hVISA clinical isolates.

Funder

Departamento Administrativo de Ciencia, Tecnología e Innovación COLCIENCIAS

NIH

NIAID

FONDECYT

Publisher

Oxford University Press (OUP)

Subject

Infectious Diseases,Pharmacology (medical),Pharmacology,Microbiology (medical)

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