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首页> 外文期刊>Journal of Clinical Microbiology >Molecular Characterization of Syphilis in Patients in Canada: Azithromycin Resistance and Detection of Treponema pallidum DNA in Whole-Blood Samples versus Ulcerative Swabs
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Molecular Characterization of Syphilis in Patients in Canada: Azithromycin Resistance and Detection of Treponema pallidum DNA in Whole-Blood Samples versus Ulcerative Swabs

机译:加拿大患者梅毒的分子特征:阿奇霉素抗性和全血样品与溃疡拭子中梅毒螺旋体DNA的检测

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Although detection of Treponema pallidum DNA in whole-blood specimens of syphilis patients has been reported, it is uncertain at what stage of the disease such specimens are most suitable for the molecular diagnosis of syphilis. Also, few studies have directly compared the different gene targets for routine laboratory diagnostic usage in PCR assays. We examined 87 specimens from 68 patients attending two urban sexually transmitted disease clinics in Alberta, Canada. PCR was used to amplify the T. pallidum tpp47, bmp, and polA genes as well as a specific region of the 23S rRNA gene linked to macrolide antibiotic susceptibility. In primary syphilis cases, PCR was positive exclusively (75% sensitivity rate) in ulcerative swabs but not in blood specimens, while in secondary syphilis cases, 50% of the blood specimens were positive by PCR. Four out of 14 (28.6%) of our PCR-positive syphilis cases were found to be caused by an azithromycin-resistant strain(s). Our results confirmed that swabs from primary ulcers are the specimens of choice for laboratory diagnostic purposes. However, further research is required to determine what specimen(s) would be most appropriate for molecular investigation of syphilis in secondary and latent syphilis.
机译:尽管已经报道了梅毒患者全血标本中的梅毒螺旋体DNA的检测,但是尚不确定在哪种疾病的标本中最适合梅毒的分子诊断。同样,很少有研究直接比较不同基因靶点在PCR分析中的常规实验室诊断用途。我们检查了来自加拿大艾伯塔省两家城市性传播疾病诊所的68名患者的87个标本。 PCR用于扩增 T。 pallidum tpp47, bmp polA 基因以及与大环内酯类抗生素敏感性相关的23S rRNA基因的特定区域。在原发性梅毒病例中,溃疡拭子PCR仅呈阳性(敏感性为75%),而在血液样本中则呈阳性,而在继发性梅毒病例中,PCR则有50%的血液样本呈阳性。在我们的PCR阳性梅毒病例中,有14例(28.6%)中有4例是由耐阿奇霉素的菌株引起的。我们的结果证实,原发性溃疡拭子是用于实验室诊断的首选标本。但是,需要进一步的研究来确定哪种标本最适合继发性和潜在性梅毒的梅毒分子研究。

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