Background <p>Antimicrobial resistance (AMR) is a growing threat to public health, especially in low- and middle-income countries. This study aimed to identify multidrug-resistant (MDR) pathogens in clinical samples from a tertiary hospital in Ecuador, evaluate their phenotypic antibiotic susceptibility, and compare these findings with genotypic resistance patterns.</p> Methods <p>Clinical samples were collected from an Ecuadorian reference hospital from September 2022 to September 2023. Bacterial identification and susceptibility testing were performed using the VITEK-2 system. After genomic DNA extraction, key resistance genes (<i>bla</i><sub>KPC</sub>, <i>bla</i><sub>NDM</sub>, <i>bla</i><sub>VIM</sub>, <i>bla</i><sub>OXA−48</sub>, <i>bla</i><sub>CTX−M</sub> and <i>bla</i><sub>IMP−1</sub>) were identified via multiplex PCR with TaqMan probes. Phenotypic and genotypic data were integrated using bioinformatics tools.</p> Results <p>The 216 bacterial isolates analyzed exhibited resistance phenotypes, primarily to carbapenems and third-generation cephalosporins. <i>Klebsiella pneumoniae</i> was the most prevalent resistant species (59.7%), followed by <i>Pseudomonas aeruginosa</i> (11.6%) and <i>Serratia marcescens</i> (8.3%). However, 20.8% of the isolates phenotypically resistant to carbapenems did not carry any of the targeted carbapenemase genes. The <i>bla</i><sub>KPC</sub> gene was most common (70.8%), followed by <i>bla</i><sub>NDM</sub> (9.7%) and <i>bla</i><sub>VIM</sub> (2.8%). Ten isolates harbored gene combinations, including, to our knowledge, the first reported co-occurrence of <i>bla</i><sub>KPC</sub> and <i>bla</i><sub>OXA−48</sub> in <i>K. pneumoniae</i> in Ecuador.Neither <i>bla</i><sub>IMP−1</sub> nor <i>bla</i><sub>CTX−M</sub> was detected in any of the evaluated isolates.</p> Conclusions <p>There is strong concordance between carbapenemase genes and the MDR phenotype, some of which are newly reported in Ecuador. However, the absence of gene detection in some resistant isolates suggests the presence of alternative resistance mechanisms. Integrating phenotypic and molecular methods that target locally prevalent resistance genes improves the accuracy of AMR detection and supports better diagnosis and infection control in hospital settings.</p>

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Co-occurrence of blaKPC and blaOXA−48 genes in Klebsiella pneumoniae isolates from a tertiary-care hospital in Ecuador and evidence of emerging genotypic–phenotypic AMR inconsistencies

  • David Fernández-Salvatierra,
  • Carmen María González-Domenech,
  • Gabriel Morey-León,
  • Juan Carlos Fernández-Cadena

摘要

Background

Antimicrobial resistance (AMR) is a growing threat to public health, especially in low- and middle-income countries. This study aimed to identify multidrug-resistant (MDR) pathogens in clinical samples from a tertiary hospital in Ecuador, evaluate their phenotypic antibiotic susceptibility, and compare these findings with genotypic resistance patterns.

Methods

Clinical samples were collected from an Ecuadorian reference hospital from September 2022 to September 2023. Bacterial identification and susceptibility testing were performed using the VITEK-2 system. After genomic DNA extraction, key resistance genes (blaKPC, blaNDM, blaVIM, blaOXA−48, blaCTX−M and blaIMP−1) were identified via multiplex PCR with TaqMan probes. Phenotypic and genotypic data were integrated using bioinformatics tools.

Results

The 216 bacterial isolates analyzed exhibited resistance phenotypes, primarily to carbapenems and third-generation cephalosporins. Klebsiella pneumoniae was the most prevalent resistant species (59.7%), followed by Pseudomonas aeruginosa (11.6%) and Serratia marcescens (8.3%). However, 20.8% of the isolates phenotypically resistant to carbapenems did not carry any of the targeted carbapenemase genes. The blaKPC gene was most common (70.8%), followed by blaNDM (9.7%) and blaVIM (2.8%). Ten isolates harbored gene combinations, including, to our knowledge, the first reported co-occurrence of blaKPC and blaOXA−48 in K. pneumoniae in Ecuador.Neither blaIMP−1 nor blaCTX−M was detected in any of the evaluated isolates.

Conclusions

There is strong concordance between carbapenemase genes and the MDR phenotype, some of which are newly reported in Ecuador. However, the absence of gene detection in some resistant isolates suggests the presence of alternative resistance mechanisms. Integrating phenotypic and molecular methods that target locally prevalent resistance genes improves the accuracy of AMR detection and supports better diagnosis and infection control in hospital settings.