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梅毒的检测方法:定量聚合酶链反应有助于更好地了解早期感染情况。

Getting the measure of syphilis: qPCR to better understand early infection.

机构信息

Imperial College London, Jefferiss Trust Laboratories, Wright-Fleming Institute, London W2 1PG, UK.

出版信息

Sex Transm Infect. 2011 Oct;87(6):479-85. doi: 10.1136/sti.2011.049494. Epub 2011 Jul 12.

DOI:10.1136/sti.2011.049494
PMID:21752804
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3252622/
Abstract

OBJECTIVES

Until recently, PCR had been used to detect but not quantify Treponema pallidum. To understand infection kinetics of this uncultivable organism, a real-time PCR assay was developed to quantify 47 kDa membrane lipoprotein gene DNA (tpp47).

METHODS

Assay specificity was determined against DNA from humans, skin organisms and sexually transmitted pathogens. tpp47 DNA (Nichols strain) was used to construct a standard curve for T pallidum quantification. Blood and ulcer samples were obtained from 99 patients being investigated or screened for syphilis and tpp47 was quantified.

RESULTS

The assay was specific, not cross-reactive with other organisms tested and sensitive, with a detection limit of a single copy of tpp47 DNA. For ulcer samples, the assay was 100% sensitive and 97.14% specific. Sensitivity fell to 34.1% for blood samples but specificity remained high (100%). tpp47 DNA was more commonly detected, and at a higher copy number, in blood of patients with secondary infection (sensitivity 57.89%) compared with primary infection. Quantity of tpp47 DNA was higher in primary infection ulcers, especially in HIV-1-positive patients, than in ulcers persisting into secondary disease.

CONCLUSIONS

Quantifying T pallidum provides insight into syphilis infection kinetics: Ulcers of primary disease in HIV-1-positive patients are perhaps more infectious and the presence and load of T pallidum bacteraemia is variable, with a peak in the secondary stage. Quantitative PCR has the potential to map T pallidum infection and to highlight the impact of HIV on syphilis.

摘要

目的

直到最近,聚合酶链反应(PCR)一直用于检测梅毒螺旋体,但无法对其进行定量。为了解这种不可培养微生物的感染动力学,开发了一种实时PCR检测方法来定量47 kDa膜脂蛋白基因DNA(tpp47)。

方法

针对来自人类、皮肤微生物和性传播病原体的DNA测定检测方法的特异性。使用tpp47 DNA(Nichols菌株)构建梅毒螺旋体定量的标准曲线。从99名正在接受梅毒调查或筛查的患者中采集血液和溃疡样本,并对tpp47进行定量。

结果

该检测方法具有特异性,与其他测试微生物无交叉反应且灵敏,tpp47 DNA单拷贝的检测限。对于溃疡样本,该检测方法的灵敏度为100%,特异性为97.14%。血液样本的灵敏度降至34.1%,但特异性仍然很高(100%)。与一期感染相比,二期感染患者血液中更常检测到tpp47 DNA,且拷贝数更高(灵敏度57.89%)。一期感染溃疡中tpp47 DNA的量高于持续到二期疾病的溃疡,尤其是在HIV-1阳性患者中。

结论

梅毒螺旋体定量有助于了解梅毒感染动力学:HIV-1阳性患者一期疾病的溃疡可能更具传染性,梅毒螺旋体菌血症的存在和负荷是可变的,在二期达到峰值。定量PCR有可能绘制梅毒螺旋体感染图谱,并突出HIV对梅毒的影响。

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