Poor Diagnostic Performance of a Species-Specific Loop-Mediated Isothermal Amplification (LAMP) Platform for Malaria.

European Journal of Microbiology & Immunology Pub Date : 2018-09-28 eCollection Date: 2018-12-23 DOI:10.1556/1886.2018.00020
Hans Kollenda, Ralf Matthias Hagen, Miriam Hanke, Sandra Rojak, Rebecca Hinz, Lars Wassill, Sven Poppert, Egbert Tannich, Hagen Frickmann
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引用次数: 12

Abstract

Background: The objective of this study was to assess an in-house loop-mediated isothermal amplification (LAMP) platform for malaria parasite detection and identification on species level.

Methods: LAMP primers specific for the human Plasmodium spp., namely, P. falciparum, P. vivax, P. ovale, P. malariae, and P. knowlesi, as well as genus-specific primers, were tested against a composite gold standard comprising microscopy from thick and thin blood films, commercial genus-specific Meridian illumigene Malaria LAMP, in-house real-time polymerase chain reaction (PCR), and commercial fast-track diagnostics (FTD) Malaria differentiation PCR.

Results: Of the 523 blood samples analyzed, the composite gold standard indicated 243 Plasmodium-species-DNA-containing samples (46.5%). Sensitivity and specificity of the analyzed genus- and species-specific LAMP primers were 71.0%-100.0% and 90.8%-100.0%, respectively. The influence of parasitemia was best documented for P. falciparum-specific LAMP with sensitivity values of 35.5% (22/62) for microscopically negative samples containing P. falciparum DNA, 50% (19/38) for parasitemia ≤50/μL, 84% (21/25) for parasitemia ≤500/μL, and 100% (92/92) for parasitemia >500/μL.

Conclusions: In our hands, performance characteristics of species-specific in-house LAMP for malaria lack reliability required for diagnostic laboratories. The use of the easy-to-apply technique for surveillance purposes may be considered.

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疟疾物种特异性环介导等温扩增(LAMP)平台诊断性能差。
背景:本研究的目的是评估一个内部环介导的等温扩增(LAMP)平台,用于疟疾寄生虫的检测和物种水平鉴定。方法:对人类疟原虫(即恶性疟原虫、间日疟原虫、卵形疟原虫、疟疾疟原虫和诺氏疟原虫)特异性LAMP引物以及属特异性引物进行复合金标准检测,包括厚、薄血膜显微镜、商业属特异性子午线光照疟疾LAMP、室内实时聚合酶链反应(PCR)和商业快速诊断(FTD)疟疾分化PCR。结果:523份血样中,含疟原虫dna的243份(46.5%)为复合金标准品。所分析的属特异性和种特异性LAMP引物的敏感性和特异性分别为71.0% ~ 100.0%和90.8% ~ 100.0%。恶性疟原虫特异性LAMP对疟原虫DNA镜检阴性样品的敏感性为35.5%(22/62),对≤50/μL敏感性为50%(19/38),对≤500/μL敏感性为84%(21/25),对>500/μL敏感性为100%(92/92)。结论:在我们手中,针对特定物种的疟疾内部LAMP的性能特征缺乏诊断实验室所需的可靠性。可以考虑为监视目的使用易于应用的技术。
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