首页> 外文期刊>Journal of the European Academy of Dermatology and Venereology: JEADV >Comparison of fungal fluorescent staining and ITS rDNA PCR ITS rDNA PCR ‐based sequencing with conventional methods for the diagnosis of onychomycosis
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Comparison of fungal fluorescent staining and ITS rDNA PCR ITS rDNA PCR ‐based sequencing with conventional methods for the diagnosis of onychomycosis

机译:真菌荧光染色及其RDNA PCR其RDNA PCR的测序与常规方法进行测序,用于诊断甲癣的诊断

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Abstract Background The current gold standard for diagnosing onychomycosis is direct microscopic examination and culturing. Fungal culture is a time‐consuming procedure, while direct microscopy of potassium hydroxide ( KOH ) mounts suffers from low sensitivity. More rapid and sensitive methods for the diagnosis of onychomycosis are in high demand. Objective To establish an effective method for the diagnosis of onychomycosis by assessing the efficacies of fungal fluorescent staining and internal transcribed spacer ( ITS ) ribosomal DNA ( rDNA ) polymerase chain reaction ( PCR )‐based sequencing. Methods A total of 204 clinical specimens from patients with suspected onychomycosis were analysed. The gold standard for a true positive sample was positive by KOH , culturing or both methods. All specimens were also tested by fungal fluorescent staining and ITS rDNA PCR ‐based sequencing. We compared the detection, sensitivity and specificity for these two methods with conventional methods. Results In total, 126 (62%) and 102 (50%) were detected by fluorescent staining and PCR ‐based sequencing, respectively. According to the conventional diagnostic standard, the sensitivity of fluorescent staining and PCR ‐based sequencing was 97% and 78%, respectively, and specificities of 89% and 90%, respectively. Use of fluorescence enhanced the sensitivity of direct examination by 12% compared with KOH . PCR ‐based sequencing increased the sensitivity by 6% compared with culturing. Conclusions Fluorescence microscopy has a higher sensitivity for the detection of fungi in nail specimens compared with KOH and can be used as a rapid screening tool. PCR ‐based sequencing was faster and more sensitive compared with culture and when used in conjunction with fluorescence microscopy resulted in higher efficiency.
机译:摘要背景诊断甲癣的当前金标准是直接显微镜检查和培养。真菌培养是一种耗时的程序,而氢氧化钾(KOH)安装的直接显微镜患者患有低灵敏度。对甲癣诊断的更快速和敏感的方法都有很高的需求。目的通过评估真菌荧光染色和内转录的间隔(ITS)核糖体DNA(RDNA)聚合酶链反应(PCR)的测序的测序来建立诊断甲癣病的有效方法。方法分析了来自疑似甲氧闭虫病患者的204例临床标本。真正阳性样品的金标准由KOH,培养或两种方法阳性。所有标本也通过真菌荧光染色及其RDNA PCR基测序测试。我们将这两种方法的检测,敏感性和特异性与传统方法进行了比较。通过分别通过荧光染色和PCR基测序检测总共126(62%)和102(50%)。根据常规的诊断标准,荧光染色和PCR的敏感性分别为97%和78%,分别为89%和90%的特异性。与KOH相比,使用荧光增强了12%的直接检查的敏感性。与培养相比,PCR基于碱的测序增加了6%的敏感性。结论与KOH相比,荧光显微镜对钉子标本中真菌的检测具有更高的灵敏度,并且可以用作快速筛选工具。与培养相比,PCR基于碱的测序比培养更快,更敏感,并且与荧光显微镜结合使用导致效率更高。

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    Shandong Provincial Hospital for Skin DiseasesShandong UniversityJinan Shandong China;

    Department of Toxicological and Functional TestShandong Centers for Disease Control and;

    Shandong Provincial Institute of Dermatology and VenereologyShandong Academy of Medical;

    Shandong Provincial Institute of Dermatology and VenereologyShandong Academy of Medical;

    Shandong Provincial Institute of Dermatology and VenereologyShandong Academy of Medical;

    Shandong Provincial Institute of Dermatology and VenereologyShandong Academy of Medical;

    Shandong Provincial Hospital for Skin DiseasesShandong UniversityJinan Shandong China;

    Shandong Provincial Hospital for Skin DiseasesShandong UniversityJinan Shandong China;

    Shandong Provincial Hospital for Skin DiseasesShandong UniversityJinan Shandong China;

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  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 皮肤病学与性病学;
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