Optimization and Clinical Evaluation of an Automated Commercial Analyte-Specific Reagent Assay for Mycoplasmoides genitalium Macrolide Resistance Detection in Primary Clinical Specimens

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creativework.keywords - en
Automation
commercial assay
resistance
macrolide
creativework.keywords - other
Mycoplasmoides genitalium
dc.contributor.author
Munson, Erik
Zapp, Amanda
Moore, Josephine
Munson, Kimber L.
Lavey, Stephen C.
Russell, Hunter
Martin, Irene
dc.date.accessioned
2023-11-21T01:19:11Z
dc.date.available
2023-11-21T01:19:11Z
dc.date.issued
2023-07-20
dc.description.abstract - en
With improvement in laboratory diagnosis of Mycoplasmoides genitalium infection through molecular diagnostics, macrolide resistance determination within M. genitalium-positive patients is necessary. In this study, we report baseline parameters for an analyte-specific reagent (ASR) macrolide resistance real-time reverse transcriptase PCR on an open access analyzer and evaluated detection of macrolide resistance-mediated mutation (MRM) within 23S rRNA in a clinical specimen set. Initial use of 1.2 μM M. genitalium primer and 0.8 μM M. genitalium detection probe concentrations yielded an 80% false-positive detection rate when challenged with 10,000 copies of wild-type RNA. Optimization experiments showed that lowering primer/detection probe and MgCl2 concentrations minimized these false-detections of wild-type 23S rRNA, while higher levels of KCl increased rates of MRM detection with concomitant lower cycle threshold values and higher fluorescence emission. Lower limit of A2058G mutation detection was 5000 copies/mL (180 copies/reaction; 20/20 detections). Utilization of a baseline correction slope limit of 250 units further mitigated false-detection from wild-type 23S rRNA at challenges up to 3.3 billion copies/mL. MRM was detected in 583/866 (67.3%) clinical specimens initially positive for M. genitalium by commercial transcription-mediated amplification. These data included 392/564 detections (69.5%) from M. genitalium-positive swab specimens and 191/302 (63.2%) from M. genitalium-positive-positive first-void urine specimens (P = 0.06). Overall resistance detection rates did not vary by gender (P = 0.76). Specificity of the M. genitalium macrolide resistance ASR was 100% (141 urogenital determinations). MRM detection by the ASR was confirmed at a concordance rate of 90.9% by Sanger sequencing of a clinical specimen subset.
dc.identifier.citation
Munson, E., Zapp, A., Moore, J., Lavey, S. C., Russell, H., Munson, K. L., & Martin, I. (2023). Optimization and Clinical Evaluation of an Automated Commercial Analyte-Specific Reagent Assay for Mycoplasmoides genitalium Macrolide Resistance Detection in Primary Clinical Specimens. Journal of clinical microbiology, 61(7), e0033523. https://doi.org/10.1128/jcm.00335-23
dc.identifier.doi
https://doi.org/10.1128/jcm.00335-23
dc.identifier.govdoc
PMC10358159
dc.identifier.issn
1098-660X
dc.identifier.pubmedID
37341596
dc.identifier.uri
https://open-science.canada.ca/handle/123456789/1309
dc.language.iso
en
dc.publisher
American Society for Microbiology
dc.rights - en
Creative Commons Attribution 4.0 International (CC BY 4.0)
dc.rights - fr
Creative Commons Attribution 4.0 International (CC BY 4.0)
dc.rights.openaccesslevel - en
Gold
dc.rights.openaccesslevel - fr
Or
dc.rights.uri - en
https://creativecommons.org/licenses/by/4.0/
dc.rights.uri - fr
https://creativecommons.org/licenses/by/4.0/deed.fr
dc.subject - en
Health
dc.subject - fr
Santé
dc.subject.en - en
Health
dc.subject.fr - fr
Santé
dc.title - en
Optimization and Clinical Evaluation of an Automated Commercial Analyte-Specific Reagent Assay for Mycoplasmoides genitalium Macrolide Resistance Detection in Primary Clinical Specimens
dc.type - en
Article
dc.type - fr
Article
local.acceptedmanuscript.articlenum
e0033523
local.article.journalissue
7
local.article.journaltitle
Journal of clinical microbiology
local.article.journalvolume
61
local.peerreview - en
Yes
local.peerreview - fr
Oui
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