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Clinical Evaluation of Three Commercial PCR Assays for the Detection of Macrolide Resistance in Mycoplasma Genitalium

Overview
Specialty Microbiology
Date 2019 Dec 6
PMID 31801835
Citations 14
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Abstract

As macrolide resistance in is increasing worldwide, macrolide resistance-associated mutations should be assessed in -positive specimens. New commercial kits are available for detection of macrolide resistance concurrently with We prospectively evaluated the handling and clinical performances of three commercial kits for detection of macrolide resistance in Between August and December 2018, remnants of all urogenital specimens determined to be positive using an in-house real-time PCR assay were prospectively collected at the French National Reference Center for Bacterial Sexually Transmitted Infections, Bordeaux University Hospital, Bordeaux, France. The internal control of each kit was added to the primary specimen before DNA extraction, and the absence of amplification inhibition associated with the addition of the three internal controls was assessed. Specimens were evaluated with four assays: the ResistancePlus MG assay (SpeeDx), the S-DiaMGRes assay (Diagenode), the RealAccurate TVMGres assay (PathoFinder), and amplification and sequencing of the 23S rRNA gene (the reference assay). Overall, 195 -positive specimens were assessed. The positive agreement of detection for each kit ranged between 94.8% and 96.4%. Among 154 specimens with positivity as detected by the three commercial kits and 23S rRNA sequencing data, the clinical sensitivity and specificity ranges of the three commercial kits for detecting macrolide resistance-associated mutations were 95 to 100% and 94.6 to 97.3%, respectively. The sensitivity and specificity values were similar among the kits. The launch of three easy-to-use sensitive and specific commercial kits for simultaneous detection of and macrolide resistance will be useful for resistance-guided therapy.

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