Sensitive and specific assay for the simultaneous detection of Mycoplasma genitalium and macrolide resistance-associated mutations

被引:9
作者
Braam, Joyce F. [1 ]
van Marm, Sebastian [1 ]
Severs, Tim T. [1 ]
Belousov, Yevgeniy [2 ]
Mahoney, Walt [2 ]
Kusters, Johannes G. [1 ]
机构
[1] Univ Med Ctr Utrecht, Dept Med Microbiol, Heidelberglaan 100, NL-3584 CX Utrecht, Netherlands
[2] ELITechGrp Inc, Bothell, WA USA
关键词
Azithromycin resistance; qPCR; Mycoplasma genitalium; 23S rRNA; A2058T; REAL-TIME PCR; POLYMERASE-CHAIN-REACTION; NONGONOCOCCAL URETHRITIS; CLINICAL SPECIMENS; HIGH PREVALENCE; AZITHROMYCIN; DISEASE; IDENTIFICATION; METAANALYSIS; STRAINS;
D O I
10.1007/s10096-018-3350-3
中图分类号
R51 [传染病];
学科分类号
100401 ;
摘要
Patients infected by Mycoplasma genitalium are often treated empirically with the macrolide azithromycin. Macrolide resistance is becoming quite common; empirical treatment is compromised. Sequencing was initially used to detected azithromycin resistance-associated mutations. As this was laborious, qPCRs have been developed for their detection. In the present study, we describe a fast, sensitive, and specific qPCR assay that enables routine testing of M. genitalium and macrolide resistance-associated mutations in a single assay. M. genitalium positive clinical samples were used to compare (i) the commonly used MgPa assay for the detection of M. genitalium infections (MgPa qPCR), (ii) a combined 23S rRNA gene PCR/sequencing assay (Mg23S qPCR/Sequencing) to identify macrolide resistance-associated mutations, and (iii) our newly developed probe-based melt curve qPCR for simultaneous detection of M. genitalium and macrolide resistance-associated mutations (Macrolide-R/MG ELITe MGB Kit, Elitech Bothel USA in short Mg Macrolide(R) qPCR). Specificity of the qPCR was tested using urogenital samples that were tested positive for a range of other micro-organisms. M. genitalium was detected in 196/236 (83.1%) samples by the MgPa qPCR, versus 172/236 (72.9%) by the combined Mg23S qPCR/Sequencing, and 202/236 (85.6%) by the Mg Macrolide(R) qPCR. The Mg Macrolide(R) qPCR showed high concordance to the Mg23S qPCR/Sequencing assay (201 vs 202 could be genotyped, respectively) for the detection of the macrolide resistant mutations. None of the other urogenital pathogens were tested positive in the Mg Macrolide(R) qPCR, indicating specificity. The Mg Macrolide(R) qPCR is fast, sensitive, specific, and can easily be implemented in the routine diagnostics.
引用
收藏
页码:2137 / 2144
页数:8
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