18S rDNA多聚酶链反应和测序在甲真菌病诊断中的应用

来源 :世界核心医学期刊文摘(皮肤病学分册) | 被引量 : 0次 | 上传用户：xia226

【摘要】

：

Diagnostic approaches to onychomycosis have traditionally been based on a combination of culture and microscopy. In the present study clinical specimens from 34

【作者】

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Walberg M Moφrk C. Sandven P. 冯义国

【机构】

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Institute of Medical Microbiology Rikshospitalet University Hospital NO- 0027Oslo Norway,

【出处】

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世界核心医学期刊文摘(皮肤病学分册)

【发表日期】

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2006年09期

【关键词】

：

甲真菌病多聚酶链反应测序标本培养须癣毛癣菌标本数阴性琼脂数据库检索镜检

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论文部分内容阅读

Diagnostic approaches to onychomycosis have traditionally been based on a combination of culture and microscopy. In the present study clinical specimens from 346 patients with suspected onychomycosis were analysed by 18S polymerase chain reaction (detection) followed by sequencing and subsequent database search (identification) in parallel with routine culture on agar (detection and identification). In 49 samples Trichophyton rubrum was identified by culture and sequencing. In 67 additional culture negative samples, a positive dermatophyte sequence was obtained (T. rubrum in 54, T. mentagrophytes in 5, and T. species in 8 samples). Fifteen samples cultured positive while no sequence was obtained. Two hundred and seven samples were negative by culture as well as by sequencing. Nails from 10 healthy controls were negative by culture and sequencing. In conclusion, the number of specimens that were positive by polymerase chain reaction was more than double the number that were positive by culture alone. Diagnostic approaches to onychomycosis have traditionally been based on a combination of culture and microscopy. In the present study clinical specimens from 346 patients with suspected onychomycosis were analysed by 18S polymerase chain reaction (detection) followed by sequencing and subsequent database search (identification) in parallel With routine culture on agar (detection and identification). In 49 additional culture negative samples, a positive dermatophyte sequence was obtained (T. rubrum in 54, T. mentagrophytes in 5, and Two species and seven samples were negative by culture as well by sequencing. In conclusion, the number of specimens that were positive by polymerase chain reaction was more than double the number that were positive by culture alone.

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18S rDNA多聚酶链反应和测序在甲真菌病诊断中的应用

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