Evaluating the Prevalence of Malaria Parasite Infection among Adults in Wetlands Using Nested PCR and High Resolution Melting Analysis

F. Ogbole, Chidi Uzoma Igwe, Henrietta Chinyere Onuoha, Chiamaka Perpetua Nzebude
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Abstract

Background: Wetlands serve as breeding grounds for mosquitoes, the vector of malaria Plasmodium. Effective detection of Plasmodium infection requires a very sensitive                        method. Aim: The aim of the present study was to evaluate the prevalence of malaria parasite infection in Sagbama LGA, Bayelsa State using nested PCR and high resolution melting analysis (HRMA) technique in comparison with microscopy. Methods: A community based cross sectional study design was employed to randomly select 206 study participants. DNA was extracted from 200 ⴗl of whole blood of each participant and a set of primers was used to target and amplify the 18S rRNA gene of Plasmodium falciparum in both molecular methods. Result: The prevalence of Plasmodium falciparum infection by microscopy was 33.01% (5.8% asymptomatic, 17% mild and 10.2% severe malaria).The prevalence of malaria parasite infection by nested genomic PCR was 71.36% (asymptomatic, 42.20% mild, 18.93%and severe malaria, 10.19%). Prevalence of malaria parasite infection by high resolution melting analysis 92.71% (asymptomatic, 63.59%, mild, 18.93% and severe, 10.19%). All the study participants that were positive for microscopy and nested genomic PCR were also positive for high resolution melting analysis. There were 59.71% and 21.36% false negatives by microscopy and nested PCR respectively. McNemar`s test for pair-wise performance comparisons among the different methods was statistically significant (p < 0.001). High parasite density (19927 ± 749 parasites/µl blood) and hyper parasite density (103667 ± 5214 parasites/ⴗl of blood) were found among asymptomatic and severe malaria subjects (P < 0.000). Conclusion: In conclusion, a high malaria parasite infection prevalence of 92.72% was found in Sagbama LGA. This requires urgent attention especially asymptomatic malaria. HRMA was the most sensitive molecular method and is therefore recommended for future molecular detection of malaria infection.
利用巢式PCR和高分辨率融化分析评估湿地成人疟疾寄生虫感染流行情况
背景:湿地是蚊子的繁殖地,蚊子是疟疾疟原虫的传播媒介。有效地检测疟原虫感染需要一种非常灵敏的方法。目的:采用巢式PCR和高分辨率熔融分析(HRMA)技术,比较巴耶尔萨州Sagbama LGA地区疟疾寄生虫感染的流行情况。方法:采用基于社区的横断面研究设计,随机抽取206名研究对象。从每个参与者的200ⴗl全血中提取DNA,使用一套引物,用两种分子方法靶向扩增恶性疟原虫18S rRNA基因。结果:镜检恶性疟原虫感染率为33.01%,其中无症状者5.8%,轻度者17%,重度者10.2%。巢式基因组PCR检测结果显示,无症状人群疟疾感染率为71.36%,其中轻度疟疾占42.20%,18.93%,重度疟疾占10.19%。高分辨率融解分析疟疾寄生虫感染率为92.71%(无症状者为63.59%,轻度者为18.93%,重度者为10.19%)。所有在显微镜和巢式基因组PCR中呈阳性的研究参与者在高分辨率熔化分析中也呈阳性。镜检和巢式PCR假阴性检出率分别为59.71%和21.36%。不同方法间两两性能比较的McNemar检验具有统计学意义(p < 0.001)。无症状和重度疟疾患者的疟原虫高密度(19927±749只/ μ l血)和高密度(103667±5214只/ⴗl血)(P < 0.000)。结论:Sagbama地区疟疾感染率较高,为92.72%。这需要紧急关注,特别是无症状疟疾。HRMA是最敏感的分子方法,因此推荐用于未来疟疾感染的分子检测。
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