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Rapid fluoroquinolone resistance detection in using mismatch amplification mutation assay-based real-time PCR. | LitMetric

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Article Abstract

Antimicrobial resistance (AMR) is an ever-increasing global health concern. One crucial facet in tackling the AMR epidemic is earlier and more accurate AMR diagnosis, particularly in the dangerous and highly multi-drug-resistant ESKAPE pathogen, . We aimed to develop two SYBR Green-based mismatch amplification mutation assays (SYBR-MAMAs) targeting GyrA T83I (248) and GyrA D87N, D87Y and D87H (259). Together, these variants cause the majority of fluoroquinolone (FQ) AMR in . Following assay validation, the 248 and 259 SYBR-MAMAs were tested on 84 Australian clinical isolates, 46 of which demonstrated intermediate/full ciprofloxacin resistance according to antimicrobial susceptibility testing. Our two SYBR-MAMAs correctly predicted an AMR phenotype in the majority (83%) of isolates with intermediate/full FQ resistance. All FQ-sensitive strains were predicted to have a sensitive phenotype. Whole-genome sequencing confirmed 100 % concordance with SYBR-MAMA genotypes. Our GyrA SYBR-MAMAs provide a rapid and cost-effective method for same-day identification of FQ AMR in . An additional SYBR-MAMA targeting the GyrB S466Y/S466F variants would increase FQ AMR prediction to 91 %. Clinical implementation of our assays will permit more timely treatment alterations in cases where decreased FQ susceptibility is identified, leading to improved patient outcomes and antimicrobial stewardship.

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http://dx.doi.org/10.1099/jmm.0.001593DOI Listing

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