Evaluation of peptide nucleic acid-mediated multiplex real-time PCR kits for rapid detection of carbapenemase genes in gram-negative clinical isolates
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Jeong, Seri
[1
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Kim, Jung Ok
[2
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Jeong, Seok Hoon
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Yonsei Univ, Coll Med, Res Inst Bacterial Resistance, Dept Lab Med, Seoul 120749, South KoreaKosin Univ, Coll Med, Dept Lab Med, Busan, South Korea
Jeong, Seok Hoon
[2
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Bae, Il Kwon
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Shilla Univ, Coll Med & Life Sci, Dept Dent Hyg, Busan, South KoreaKosin Univ, Coll Med, Dept Lab Med, Busan, South Korea
Bae, Il Kwon
[3
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Song, Wonkeun
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Hallym Univ, Kangnam Sacred Heart Hosp, Coll Med, Dept Lab Med, Seoul 150950, South KoreaKosin Univ, Coll Med, Dept Lab Med, Busan, South Korea
Song, Wonkeun
[4
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[1] Kosin Univ, Coll Med, Dept Lab Med, Busan, South Korea
[2] Yonsei Univ, Coll Med, Res Inst Bacterial Resistance, Dept Lab Med, Seoul 120749, South Korea
[3] Shilla Univ, Coll Med & Life Sci, Dept Dent Hyg, Busan, South Korea
[4] Hallym Univ, Kangnam Sacred Heart Hosp, Coll Med, Dept Lab Med, Seoul 150950, South Korea
The emergence of clinical isolates of carbapenemase-producing microbes confers multidrug-resistance to these bacteria and renders them difficult to treat. This study was performed to evaluate peptide nucleic acid (PNA) probe-based multiplex real-time PCR kits used to detect carbapenemase genes. In total, 324 carbapenemase genes, collected from 318 gram-negative clinical isolates in 36 different hospital laboratories, were assayed to evaluate multiplex real-time PCR kits (PANAGENE; Daejeon, Korea). The nine most prevalent carbapenemase genes (KPC, OXA-48, GES, IMP, VIM, NDM, ISAba1-OXA-51, OXA-23, and OXA-58) were included in this study. The sensitivity and specificity of the multiplex real-time PCR assay to all of the carbapenemase genes were above 99.0%, except for ISAba1-OXA-51. The detection limit of the assay was 100 target copies per 25 mu L of reaction volume for all of the nine genetic types of carbapenemases, and-the genes were all detected in a single three-hour PCR. The assay also showed considerable efficiency (above 80.0%), stable reproducibility (coefficient of variation, below 5.0%) and a long shelf-life (more than eight months) with no cross reactivity. The developed PNA-mediated multiplex real-time PCR assay was useful for the rapid, accurate and simultaneous identification of nine carbapenemase genes in gram-negative clinical isolates, suggesting its potential to help choose the appropriate antibiotics and aid the control of carbapenemase genes. (C) 2015 Elsevier B.V. All rights reserved.
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Univ Western Australia, Queen Elizabeth II Med Ctr, Dept Microbiol, PathWest Lab Med WA, Nedlands, WA 6009, AustraliaUniv Western Australia, Queen Elizabeth II Med Ctr, Dept Microbiol, PathWest Lab Med WA, Nedlands, WA 6009, Australia
Pereira, Lynette A.
Harnett, Gerald B.
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Univ Western Australia, Queen Elizabeth II Med Ctr, Dept Microbiol, PathWest Lab Med WA, Nedlands, WA 6009, AustraliaUniv Western Australia, Queen Elizabeth II Med Ctr, Dept Microbiol, PathWest Lab Med WA, Nedlands, WA 6009, Australia
Harnett, Gerald B.
Hodge, Meredith M.
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Univ Western Australia, Queen Elizabeth II Med Ctr, Dept Microbiol, PathWest Lab Med WA, Nedlands, WA 6009, AustraliaUniv Western Australia, Queen Elizabeth II Med Ctr, Dept Microbiol, PathWest Lab Med WA, Nedlands, WA 6009, Australia
Hodge, Meredith M.
Cattell, Julia A.
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Univ Western Australia, Queen Elizabeth II Med Ctr, Dept Microbiol, PathWest Lab Med WA, Nedlands, WA 6009, AustraliaUniv Western Australia, Queen Elizabeth II Med Ctr, Dept Microbiol, PathWest Lab Med WA, Nedlands, WA 6009, Australia
Cattell, Julia A.
Speers, David J.
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Univ Western Australia, Queen Elizabeth II Med Ctr, Dept Microbiol, PathWest Lab Med WA, Nedlands, WA 6009, Australia
Univ Western Australia, Sch Med & Pharmacol, Nedlands, WA 6009, AustraliaUniv Western Australia, Queen Elizabeth II Med Ctr, Dept Microbiol, PathWest Lab Med WA, Nedlands, WA 6009, Australia