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用于检测生殖支原体的不同生殖标本类型的转录介导扩增法与聚合酶链反应检测结果的比较。

Comparison of transcription-mediated amplification and PCR assay results for various genital specimen types for detection of Mycoplasma genitalium.

作者信息

Wroblewski Jennifer K H, Manhart Lisa E, Dickey Kathleen A, Hudspeth Marie K, Totten Patricia A

机构信息

Department of Medicine, Harborview Medical Center, University of Washington, Box 359779, 325 9th Ave., Seattle, 98104, USA.

出版信息

J Clin Microbiol. 2006 Sep;44(9):3306-12. doi: 10.1128/JCM.00553-06.

Abstract

Mycoplasma genitalium is now recognized as a possible cause of several idiopathic sexually transmitted disease (STD) syndromes. However, due to the difficulty of culture of this fastidious bacterium, nucleic acid amplification tests (NAATs) are necessary for its detection in patient specimens. In the current study we compared a newly developed research-only transcription-mediated amplification (TMA) assay (Gen-Probe Incorporated) to our in-house DNA-based PCR assay for detection of M. genitalium. The relative performance characteristics of these two NAATs were assessed with genital specimens from 284 women and 352 men reporting to an STD clinic in Seattle, WA. Among the women, M. genitalium was detected by the TMA and PCR assays in 36 (13%) and 39 (14%) vaginal swab specimens, respectively (kappa = 0.923); 26 (9%) and 23 (8%) cervical swab specimens, respectively (kappa = 0.843); and 25 (9%) and 28 (10%) urine specimens, respectively (kappa = 0.687). Among the M. genitalium-positive women, the relative sensitivities of detection for the TMA and PCR assays were 84% and 91%, respectively, for vaginal swab specimens; 60% and 53%, respectively, for cervical swab specimens; and 58% and 65%, respectively, for urine specimens. By using an infected patient (a woman positive at any site by TMA assay and at any site by PCR) as a proxy for a "gold standard," the specificities of detection were >99.5% for both the TMA and the PCR assays. Among the men, M. genitalium was detected in 24 urine specimens (6.8%) by the TMA assay, 26 (7.4%) urine specimens by PCR assay, and 32 urine specimens (9%) by either test (kappa = 0.791). We conclude that the M. genitalium TMA and PCR assays are highly specific and that vaginal swab specimens are the most sensitive specimen type for the detection of M. genitalium in women.

摘要

生殖支原体现已被认为是多种特发性性传播疾病(STD)综合征的可能病因。然而,由于这种苛求菌培养困难,核酸扩增检测(NAATs)对于在患者标本中检测它是必要的。在本研究中,我们将一种新开发的仅用于研究的转录介导扩增(TMA)检测法(Gen-Probe公司)与我们内部基于DNA的PCR检测法进行比较,以检测生殖支原体。使用来自华盛顿州西雅图一家STD诊所的284名女性和352名男性的生殖器标本评估这两种NAATs的相对性能特征。在女性中,通过TMA检测法和PCR检测法分别在36份(13%)和39份(14%)阴道拭子标本中检测到生殖支原体(kappa = 0.923);分别在26份(9%)和23份(8%)宫颈拭子标本中检测到(kappa = 0.843);以及分别在25份(9%)和28份(10%)尿液标本中检测到(kappa = 0.687)。在生殖支原体阳性的女性中,对于阴道拭子标本,TMA检测法和PCR检测法的相对检测灵敏度分别为84%和91%;对于宫颈拭子标本,分别为60%和53%;对于尿液标本,分别为58%和65%。通过将一名感染患者(一名通过TMA检测法在任何部位呈阳性且通过PCR检测法在任何部位呈阳性的女性)作为“金标准”的替代物,TMA检测法和PCR检测法的检测特异性均>99.5%。在男性中,通过TMA检测法在24份尿液标本(6.8%)中检测到生殖支原体,通过PCR检测法在26份(7.4%)尿液标本中检测到,通过任一检测法在32份尿液标本(9%)中检测到(kappa = 0.791)。我们得出结论,生殖支原体TMA检测法和PCR检测法具有高度特异性,并且阴道拭子标本是女性中检测生殖支原体最敏感的标本类型。

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