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首页> 外文期刊>Journal of Clinical Microbiology >Prevalence and Density-Related Concordance of Three Diagnostic Tests for Malaria in a Region of Tanzania with Hypoendemic Malaria
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Prevalence and Density-Related Concordance of Three Diagnostic Tests for Malaria in a Region of Tanzania with Hypoendemic Malaria

机译:坦桑尼亚地区低流行性疟疾的三项疟疾诊断测试的患病率和与密度相关的一致性

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摘要

Accurate malaria diagnosis has dual roles in identification of symptomatic persons for effective malaria treatment and also enumeration of asymptomatic persons who contribute to the epidemiologic determinants of transmission. Three currently used diagnostic tests, microscopy, rapid diagnostic tests (RDTs), and real-time PCR, all have different sensitivities and specificities, which are parasite density dependent. Here, we compare their concordance among 451 febrile episodes in a cohort of 2,058 children and adults followed over 6 months in a region in central Tanzania with hypoendemic malaria. Microscopy, a histidine-rich protein-based RDT, and two different real-time PCR gene probes detected Plasmodium falciparum in 20, 54, 41, and 78 episodes of fever, respectively. They had complete concordance in only 9 episodes. Real-time PCR with an 18S probe was more sensitive than with a mitochondrial probe for cytochrome b despite higher copy numbers of mitochondrial DNA. Both PCR yields were increased 4-fold by glycogen/acetate precipitation with low-speed centrifugation. Duplicate PCR increases low-density malaria detection. RDT had the highest number of unique positives, presumably from persistent antigen despite the absence of parasites, although RDT did not detect 3 parasitemias with over 1,000 parasites/μl. In a latent class analysis, real-time PCR had significantly higher sensitivity than did microscopy or RDT. Agreement between real-time PCR, RDT, and microscopy was highest in March and April, when both the P. falciparum parasite rate and parasite densities are highest. Real-time PCR is more sensitive and specific than RDT and microscopy in low-prevalence, low-parasite-density settings.
机译:准确的疟疾诊断在识别有症状的人以进行有效的疟疾治疗以及列举无症状的人(其对传播的流行病学决定因素有贡献)方面起着双重作用。当前使用的三种诊断测试,显微镜检查,快速诊断测试(RDT)和实时PCR都具有不同的敏感性和特异性,这取决于寄生虫的密度。在这里,我们比较了坦桑尼亚中部地区发生低流行性疟疾的2058名儿童和成人队列中的451次高热发作的一致性,随访了6个月以上。显微镜检查,富含组氨酸的基于蛋白质的RDT和两种不同的实时PCR基因探针分别在20、54、41和78次发烧中检测出恶性疟原虫。他们只有9集完全一致。尽管线粒体DNA的拷贝数更高,但使用18S探针的实时PCR对细胞色素 b 的敏感性比用线粒体探针更高。通过糖原/乙酸盐的低速离心沉淀,两种PCR的产量都提高了4倍。重复PCR可提高低密度疟疾的检测率。尽管没有寄生虫,RDT的独特阳性数量最多,大概是来自持久性抗原,尽管RDT并未检测到3种寄生虫病,每株寄生虫超过1,000个。在潜在类别分析中,实时PCR的灵敏度明显高于显微镜或RDT。实时PCR,RDT和显微镜检查在3月和4月之间的一致性最高,而恶性疟原虫的寄生虫发生率和寄生虫密度最高。在低流行,低寄生虫密度的环境中,实时PCR比RDT和显微镜检查更灵敏,更具特异性。

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