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应用直接聚合酶链反应检测浅部和甲真菌病的红色毛癣菌:快速和敏感。

Fast and sensitive detection of Trichophyton rubrum in superficial tinea and onychomycosis by use of a direct polymerase chain reaction assay.

机构信息

Department of Dermatology, University Hospitals of Schleswig-Holstein, Campus Kiel, Kiel, Germany.

出版信息

Mycoses. 2011 Sep;54(5):e313-7. doi: 10.1111/j.1439-0507.2010.01904.x. Epub 2010 May 19.

Abstract

Detection of Trichophyton rubrum in superficial skin infections by conventional methods is time consuming and not always successful. However, with modern molecular methods, an alternative is in sight. The aim of this study was to compare the detection of T. rubrum by conventional methods and by a direct specific PCR assay under routine conditions. Skin scrapings (n = 464) and nail samples (n = 230) collected from suspected tinea lesions were equally divided for KOH-mounts, cultures and PCR-analysis. For the latter, DNA was extracted and PCR was performed with T. rubrum-specific primers. Of the scale samples, 16% were positive for T. rubrum in the culture and PCR as well, 9% were positive in the PCR only and 3% in the culture only, whereas 5% were only KOH-positive. The corresponding results for nail samples were 17%, 20%, 3% and 7%. PCR results were available after 2-5 days, culture results after 2-3 weeks. Our results show that a specific PCR assay can successfully be used to detect T. rubrum directly in samples collected from superficial skin lesions and nails under routine conditions. Compared with conventional methods, it is faster and more sensitive. We recommend its complementary use.

摘要

传统方法检测浅部皮肤感染的红色毛癣菌既费时又不总是成功。然而,随着现代分子方法的出现,一种替代方法已经在望。本研究的目的是比较常规条件下传统方法和直接特异性 PCR 检测法对红色毛癣菌的检测。从疑似癣病病变处采集的皮肤刮屑(n=464)和指甲样本(n=230)等量分为 KOH 载玻片、培养物和 PCR 分析。对于后者,提取 DNA 并使用红色毛癣菌特异性引物进行 PCR。在鳞屑样本中,16%的样本在培养和 PCR 中均为红色毛癣菌阳性,9%的样本仅在 PCR 中阳性,3%的样本仅在培养中阳性,而 5%的样本仅在 KOH 中阳性。指甲样本的相应结果分别为 17%、20%、3%和 7%。PCR 结果可在 2-5 天后获得,培养结果在 2-3 周后获得。我们的结果表明,特定的 PCR 检测法可成功地在常规条件下直接从浅部皮肤病变和指甲样本中检测到红色毛癣菌。与传统方法相比,它更快、更敏感。我们建议互补使用。

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