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基于核酸序列扩增与寡色层分析用于检测临床样本中的布氏锥虫

Nucleic acid sequence-based amplification with oligochromatography for detection of Trypanosoma brucei in clinical samples.

作者信息

Mugasa Claire M, Laurent Thierry, Schoone Gerard J, Kager Piet A, Lubega George W, Schallig Henk D F H

机构信息

Department of Veterinary Parasitology and Microbiology, Faculty of Veterinary Medicine, Makerere University, Kampala, Uganda.

出版信息

J Clin Microbiol. 2009 Mar;47(3):630-5. doi: 10.1128/JCM.01430-08. Epub 2008 Dec 30.

Abstract

Molecular tools, such as real-time nucleic acid sequence-based amplification (NASBA) and PCR, have been developed to detect Trypanosoma brucei parasites in blood for the diagnosis of human African trypanosomiasis (HAT). Despite good sensitivity, these techniques are not implemented in HAT control programs due to the high cost of the equipment, which is unaffordable for laboratories in developing countries where HAT is endemic. In this study, a simplified technique, oligochromatography (OC), was developed for the detection of amplification products of T. brucei 18S rRNA by NASBA. The T. brucei NASBA-OC test has analytical sensitivities of 1 to 10 parasites/ml on nucleic acids extracted from parasite culture and 10 parasites/ml on spiked blood. The test showed no reaction with nontarget pathogens or with blood from healthy controls. Compared to the composite standard applied in the present study, i.e., parasitological confirmation of a HAT case by direct microscopy or by microscopy after concentration of parasites using either a microhematocrit centrifugation technique or a mini-anion-exchange centrifugation technique, NASBA-OC on blood samples had a sensitivity of 73.0% (95% confidence interval, 60 to 83%), while standard expert microscopy had a sensitivity of 57.1% (95% confidence interval, 44 to 69%). On cerebrospinal fluid samples, NASBA-OC had a sensitivity of 88.2% (95% confidence interval, 75 to 95%) and standard microscopy had a sensitivity of 86.2% (95% confidence interval, 64 to 88%). The T. brucei NASBA-OC test developed in this study can be employed in field laboratories, because it does not require a thermocycler; a simple heat block or a water bath maintained at two different temperatures is sufficient for amplification.

摘要

已开发出分子工具,如基于实时核酸序列的扩增技术(NASBA)和聚合酶链反应(PCR),用于检测血液中的布氏锥虫寄生虫,以诊断人类非洲锥虫病(HAT)。尽管这些技术灵敏度较高,但由于设备成本高昂,发展中国家流行HAT地区的实验室无力承担,因此未在HAT防控项目中应用。在本研究中,开发了一种简化技术——寡色层分析法(OC),用于检测NASBA扩增的布氏锥虫18S rRNA产物。布氏锥虫NASBA-OC检测对从寄生虫培养物中提取的核酸的分析灵敏度为每毫升1至10个寄生虫,对加样血液的分析灵敏度为每毫升10个寄生虫。该检测对非目标病原体或健康对照者的血液无反应。与本研究采用的复合标准(即通过直接显微镜检查或使用微量血细胞比容离心技术或微型阴离子交换离心技术浓缩寄生虫后进行显微镜检查对HAT病例进行寄生虫学确诊)相比,血液样本的NASBA-OC检测灵敏度为73.0%(95%置信区间为60%至83%),而标准专家显微镜检查的灵敏度为57.1%(95%置信区间为44%至69%)。对于脑脊液样本,NASBA-OC检测的灵敏度为88.2%(95%置信区间为75%至95%),标准显微镜检查的灵敏度为86.2%(95%置信区间为64%至88%)。本研究开发的布氏锥虫NASBA-OC检测可用于现场实验室,因为它不需要热循环仪;一个简单的加热块或保持在两个不同温度的水浴就足以进行扩增。

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