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Featured researches published by Indira Berrio.


Journal of Clinical Microbiology | 2017

Rapid and Accurate Molecular Identification of the Emerging Multidrug-Resistant Pathogen Candida auris

Milena Kordalewska; Yanan Zhao; Shawn R. Lockhart; Anuradha Chowdhary; Indira Berrio; David S. Perlin

ABSTRACT Candida auris is an emerging multidrug-resistant fungal pathogen causing nosocomial and invasive infections associated with high mortality. C. auris is commonly misidentified as several different yeast species by commercially available phenotypic identification platforms. Thus, there is an urgent need for a reliable diagnostic method. In this paper, we present fast, robust, easy-to-perform and interpret PCR and real-time PCR assays to identify C. auris and related species: Candida duobushaemulonii, Candida haemulonii, and Candida lusitaniae. Targeting rDNA region nucleotide sequences, primers specific for C. auris only or C. auris and related species were designed. A panel of 140 clinical fungal isolates was used in both PCR and real-time PCR assays followed by electrophoresis or melting temperature analysis, respectively. The identification results from the assays were 100% concordant with DNA sequencing results. These molecular assays overcome the deficiencies of existing phenotypic tests to identify C. auris and related species.


Revista Iberoamericana De Micologia | 2018

Single-tube classical PCR for Candida auris and Candida haemulonii identification

Laura Theill; Catiana Dudiuk; Soraya E. Morales-López; Indira Berrio; José Yesid Rodríguez; Adriana Marin; Soledad Gamarra; Guillermo Garcia-Effron

BACKGROUND Candida auris and Candida haemulonii are emerging and multiresistant pathogens. C. auris has produced hospital outbreaks and is misidentified by phenotypic-based methods. The only reliable identification methods are DNA sequencing and MALDI-TOF. AIMS To develop a classical-PCR method capable of rapidly and accurately identify C. auris and C. haemulonii. METHODS A multiplex PCR was carried out in one tube that included an internal control and oligonucleotides that specifically hybridize to the ITS2 region of C. auris and C. haemulonii. The usefulness of the new method was verified by testing a collection of 50 strains of 20 different species (previously identified by ITS sequencing). The selection of species was made in order to emulate the C. auris panel used by the CDC to validate diagnostic tools. In addition, other yeast species not included in the aforementioned panel were incorporated based on reported identification errors. RESULTS The results obtained with the proposed protocol were in total agreement with those obtained by ITS sequencing. CONCLUSIONS We present a PCR method able to unequivocally identify C. auris and differentiate it from C. haemulonii. It is inexpensive, fast and it could be a useful tool to reduce the chances of a C. auris outbreak.


Clinical Infectious Diseases | 2018

Molecular Epidemiology of Candida auris in Colombia Reveals a Highly Related, Countrywide Colonization With Regional Patterns in Amphotericin B Resistance

Patricia Escandón; Nancy A. Chow; Diego H. Cáceres; Lalitha Gade; Elizabeth L. Berkow; Paige Armstrong; Sandra Rivera; Elizabeth Misas; Carolina Duarte; Heather Moulton-Meissner; Rory M. Welsh; Claudia Parra; Luz Angela Pescador; Nohora Villalobos; Soraya Salcedo; Indira Berrio; Carmen Varón; Andres Espinosa-Bode; Shawn R. Lockhart; Brendan R. Jackson; Anastasia P. Litvintseva; Mauricio Beltrán; Tom Chiller

Background Candida auris is a multidrug-resistant yeast associated with hospital outbreaks worldwide. During 2015-2016, multiple outbreaks were reported in Colombia. We aimed to understand the extent of contamination in healthcare settings and to characterize the molecular epidemiology of C. auris in Colombia. Methods We sampled patients, patient contacts, healthcare workers, and the environment in 4 hospitals with recent C. auris outbreaks. Using standardized protocols, people were swabbed at different body sites. Patient and procedure rooms were sectioned into 4 zones and surfaces were swabbed. We performed whole-genome sequencing (WGS) and antifungal susceptibility testing (AFST) on all isolates. Results Seven of the 17 (41%) people swabbed were found to be colonized. Candida auris was isolated from 37 of 322 (11%) environmental samples. These were collected from a variety of items in all 4 zones. WGS and AFST revealed that although isolates were similar throughout the country, isolates from the northern region were genetically distinct and more resistant to amphotericin B (AmB) than the isolates from central Colombia. Four novel nonsynonymous mutations were found to be significantly associated with AmB resistance. Conclusions Our results show that extensive C. auris contamination can occur and highlight the importance of adherence to appropriate infection control practices and disinfection strategies. Observed genetic diversity supports healthcare transmission and a recent expansion of C. auris within Colombia with divergent AmB susceptibility.


Journal of global antimicrobial resistance | 2017

Comparative study for 147 Candida spp. identification and echinocandins susceptibility in isolates obtained from blood cultures in 15 hospitals, Medellin, Colombia

Indira Berrio; Natalia Maldonado; Catalina de Bedout; Karen Arango; Luz Elena Cano; Yorlady Valencia; Cristina Jiménez-Ortigosa; David S. Perlin; Beatriz L. Gómez; Carlos Robledo; Jaime Robledo

OBJECTIVES Invasive candidiasis has a high impact on morbidity and mortality in hospitalised patients. Accurate and timely methods for identification of Candida spp. and determination of echinocandin susceptibility have become a priority for clinical microbiology laboratories. METHODS This study was performed to compare matrix-assisted laser desorption/ionisation time-of-flight mass spectrometry (MALDI-TOF/MS) identification with sequencing of the D1/D2 region of the rRNA gene complex 28 subunit in 147 Candida spp. isolates obtained from patients with candidaemia. Antimicrobial susceptibility testing was performed by broth microdilution (BMD) and Etest. Sequencing of the FKS1 and FKS2 genes was performed. RESULTS The most common species isolated were Candida albicans (40.8%), followed by Candida parapsilosis (23.1%) and Candida tropicalis (17.0%). Overall agreement between the results of identification by MALDI-TOF/MS and molecular identification was 99.3%. Anidulafungin and caspofungin susceptibility by the BMD method was 98.0% and 88.4%, respectively. Susceptibility to anidulafungin and caspofungin by Etest was 93.9% and 98.6%, respectively. Categorical agreement between Etest and BMD was 91.8% for anidulafungin and 89.8% for caspofungin, with lower agreements in C. parapsilosis for anidulafungin (76.5%) and C. glabrata for caspofungin (40.0%). No mutations related to resistance were found in the FKS genes, although 54 isolates presented synonymous polymorphisms in the hotspots sequenced. CONCLUSIONS MALDI-TOF/MS is a good alternative for routine identification of Candida spp. isolates. DNA sequencing of the FKS genes suggested that the isolates analysed were susceptible to echinocandins; alternatively, unknown resistance mechanisms or limitations related to antifungal susceptibility tests may explain the resistance found in a few isolates.


Enfermedades Infecciosas Y Microbiologia Clinica | 2017

Resistencia a ertapenem en 2 instituciones hospitalarias de alto nivel de complejidad: microbiología, epidemiología y factores de riesgo

Natalia Maldonado; Bibiana Castro; Indira Berrio; Miguel Manjarrés; Carlos Robledo; Jaime Robledo

INTRODUCTION Carbapenems resistance is a growing phenomenon and a threat to public health because of the reduced therapeutic options for resistant infections. METHODS A retrospective case-control study was conducted in 2 tertiary-care hospitals in Medellín, Colombia. Fifty patients infected with ertapenem-resistant enterobacteriaceae were compared with a control group consisting of 100 patients with infections caused by ertapenem susceptible enterobacteriaceae. A multivariate logistic regression model was used to identify factors that best explain ertapenem-resistant enterobacteriaceae infections. RESULTS The factors associated with ertapenem-resistant enterobacteriaceae infections were prior exposure to carbapenems (adjusted OR 3.43; 95% IC 1.08-10.87) and prior exposure to cefepime (adjusted OR 6.46; 95% IC 1.08-38.38). CONCLUSION Prior exposure to antibiotics is the factor that best explains the ertapenem-resistant enterobacteriaceae infection in this population, highlighting the importance of antimicrobial stewardship programs in hospitals.


Antimicrobial Agents and Chemotherapy | 2018

Understanding Echinocandin Resistance in the Emerging Pathogen Candida auris

Milena Kordalewska; Annie Lee; Steven Park; Indira Berrio; Anuradha Chowdhary; Yanan Zhao; David S. Perlin


Enfermedades Infecciosas Y Microbiologia Clinica | 2017

[Ertapenem resistance in 2 tertiary-care hospitals: Microbiology, epidemiology, and risk factors].

Natalia Maldonado; Bibiana Castro; Indira Berrio; Miguel Manjarrés; Carlos Robledo; Jaime Robledo


Archive | 2018

Limited mutations identified in isolates of directly contribute to reduced azole susceptibility.

Kelley R. Healey; Milena Kordalewska; Cristina Jiménez Ortigosa; Ashutosh Singh; Indira Berrio; Anuradha Chowdhary; David S. Perlin


Archive | 2018

Understanding echinocandin resistance in the emerging pathogen .

Milena Kordalewska; Annie Lee; Steven Park; Indira Berrio; Anuradha Chowdhary; Yanan Zhao; David S. Perlin


Antimicrobial Agents and Chemotherapy | 2018

Limited ERG11 Mutations Identified in Isolates of Candida auris Directly Contribute to Reduced Azole Susceptibility

Kelley R. Healey; Milena Kordalewska; Cristina Jiménez Ortigosa; Ashutosh Kumar Singh; Indira Berrio; Anuradha Chowdhary; David S. Perlin

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David S. Perlin

Rutgers Biomedical and Health Sciences

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Milena Kordalewska

Rutgers Biomedical and Health Sciences

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Jaime Robledo

Pontifical Bolivarian University

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Cristina Jiménez Ortigosa

Public Health Research Institute

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Diego H. Cáceres

Centers for Disease Control and Prevention

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