基于TaqMan的实时聚合酶链反应与传统检测方法用于检测阴道毛滴虫的比较。

Comparison of a TaqMan-based real-time polymerase chain reaction with conventional tests for the detection of Trichomonas vaginalis.

作者信息

Pillay A, Radebe F, Fehler G, Htun Y, Ballard R C

机构信息

Centers for Disease Control and Prevention, Division of STD Prevention, Laboratory Reference and Research Branch, 1600 Clifton Road, MS-G39, Atlanta, GA 30333, USA.

出版信息

Sex Transm Infect. 2007 Apr;83(2):126-9. doi: 10.1136/sti.2006.022376. Epub 2006 Nov 7.

DOI:10.1136/sti.2006.022376

PMID:17090567

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2598620/

Abstract

OBJECTIVE

To compare a TaqMan-based real-time polymerase chain reaction (PCR) with conventional PCR, culture, and wet-mount microscopy for the diagnosis of trichomoniasis in women.

METHODS

Vaginal swabs from 119 women were tested for Trichomonas vaginalis by wet mount and culture. Paired vaginal lavage and urine specimens were tested by conventional and real-time PCR.

RESULTS

Using an expanded "gold standard", defined as a positive culture result using vaginal swabs and/or a positive PCR test using TVK3/7 primers, the overall prevalence of T vaginalis in the study population was 65.5% (78/119). The detection rate of T vaginalis was 65.5% (78/119) and 36.9% (44/119) by conventional PCR using vaginal washings and urine specimens, respectively; 68.9% (82/119) by real-time PCR using vaginal washings and 61.3% (73/119) by real-time PCR using urine specimens. The sensitivities of conventional PCR using vaginal washings and urine and real-time PCR using vaginal washings and urine, compared with the gold standard were 100%, 56.4%, 100% and 76.7%, and the specificities of these tests were 100%, 97.6%, 82.9% and 97%, respectively.

CONCLUSIONS

The real-time PCR test proved to be significantly more sensitive than culture and wet-mount microscopy, although its specificity was slightly lower than these tests. In addition, it was more sensitive, rapid and less time consuming than conventional PCR for the detection of T vaginalis.

摘要

目的

比较基于TaqMan的实时聚合酶链反应（PCR）与传统PCR、培养法及湿片显微镜检查法在诊断女性滴虫病中的应用。

方法

对119名女性的阴道拭子进行湿片检查和培养以检测阴道毛滴虫。对配对的阴道灌洗液和尿液标本进行传统PCR和实时PCR检测。

结果

采用扩展的“金标准”，即阴道拭子培养结果阳性和/或使用TVK3/7引物的PCR检测结果阳性，研究人群中阴道毛滴虫的总体患病率为65.5%（78/119）。使用阴道灌洗液和尿液标本进行传统PCR检测阴道毛滴虫的检出率分别为65.5%（78/119）和36.9%（44/119）；使用阴道灌洗液进行实时PCR的检出率为68.9%（82/119），使用尿液标本进行实时PCR的检出率为61.3%（73/119）。与金标准相比，使用阴道灌洗液和尿液进行传统PCR以及使用阴道灌洗液和尿液进行实时PCR的敏感性分别为100%、56.4%、100%和76.7%，这些检测方法的特异性分别为100%、97.6%、82.9%和97%。

结论

实时PCR检测法的敏感性明显高于培养法和湿片显微镜检查法，尽管其特异性略低于这些检测方法。此外，在检测阴道毛滴虫方面，它比传统PCR更敏感、快速且耗时更少。

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