Multiplex real-time PCR with high-resolution melting analysis for rapid identification of carbapenem and colistin resistance genes in clinical Enterobacterales isolates

Luk-In S.; Phopin K.; Bangmuangngam S.; Chatsuwan T.; Wannigama D.L.; Shein A.M.S.; Lawung R.; Tantimongcolwat T.

Multiplex real-time PCR with high-resolution melting analysis for rapid identification of carbapenem and colistin resistance genes in clinical Enterobacterales isolates

Issued Date

2026-12-01

Resource Type

Article

eISSN

20452322

DOI

10.1038/s41598-026-41530-2

Scopus ID

2-s2.0-105035200511

Journal Title

Scientific Reports

Volume

16

Issue

1

Rights Holder(s)

SCOPUS

Bibliographic Citation

Scientific Reports Vol.16 No.1 (2026)

Suggested Citation

Luk-In S., Phopin K., Bangmuangngam S., Chatsuwan T., Wannigama D.L., Shein A.M.S., Lawung R., Tantimongcolwat T. Multiplex real-time PCR with high-resolution melting analysis for rapid identification of carbapenem and colistin resistance genes in clinical Enterobacterales isolates. Scientific Reports Vol.16 No.1 (2026). doi:10.1038/s41598-026-41530-2 Retrieved from: https://repository.li.mahidol.ac.th/handle/123456789/116207

Title

Multiplex real-time PCR with high-resolution melting analysis for rapid identification of carbapenem and colistin resistance genes in clinical Enterobacterales isolates

Author(s)

Luk-In S.
Phopin K.
Bangmuangngam S.
Chatsuwan T.
Wannigama D.L.
Shein A.M.S.
Lawung R.
Tantimongcolwat T.

Author's Affiliation

The University of Sheffield
Mahidol University
Yamagata University Faculty of Medicine
Faculty of Medicine, Chulalongkorn University
Yamagata Prefectural Central Hospital
Yamagata Prefectural University of Health Sciences

Corresponding Author(s)

Luk-In S.

Other Contributor(s)

Mahidol University

Abstract

Conventional susceptibility testing requires 18–48 h and often delays therapy, whereas existing molecular assays are costly and limited. Real-time PCR’s ubiquity in hospitals offers a rapid multiplex screening platform. We established a single-tube multiplex real-time PCR assay coupled with high-resolution melting analysis to detect seven resistance genes (bla<inf>KPC</inf>, bla<inf>NDM</inf>, bla<inf>OXA-48-like</inf>, bla<inf>VIM</inf>, bla<inf>IMP</inf>, mcr-1, and mcr-3). Validated on 577 clinical Enterobacterales isolates and a standard strain, the assay exhibited distinct melt peaks for each target, with intra- and inter-run CVs < 0.1%. Compared with reference PCR, the assay offered overall sensitivity of 97.3%, the specificity of 99.5%, the PPV of 99.7%, and the NPV of 95.4%, yielding a kappa coefficient of 0.936 (95% CI 0.913–0.958) with “high concordance”. Codetection of the bla<inf>NDM</inf> and bla<inf>OXA-48-like</inf> genes improved the sensitivity from 82.7% to 92.9% when precision melt analysis software was used. The assay demonstrated good quantitative analytical performance, with efficiencies ranging from 91 to 114% (R<sup>2</sup> = 0.96–0.99), and a minimum of 10<sup>2</sup> copies required to confidently detect all targets. In under 4 h, this cost-effective assay leverages existing platforms for comprehensive surveillance of carbapenem and colistin resistance, enabling timely antimicrobial stewardship and infection control.

Keyword(s)

Multidisciplinary

URI

https://repository.li.mahidol.ac.th/handle/123456789/116207

Collections

Scopus 2026

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