Combined DNA extraction and antibody elution from filter papers for the assessment of malaria transmission intensity in epidemiological studies

被引:53
作者
Baidjoe, Amrish [1 ]
Stone, Will [1 ]
Ploemen, Ivo [1 ]
Shagari, Shehu [2 ,3 ]
Grignard, Lynn [5 ]
Osoti, Victor [2 ,3 ]
Makori, Euniah [2 ,3 ]
Stevenson, Jennifer [4 ]
Kariuki, Simon [2 ,3 ]
Sutherland, Colin [5 ]
Sauerwein, Robert [1 ]
Cox, Jonathan [4 ]
Drakeley, Chris [5 ]
Bousema, Teun [1 ,5 ]
机构
[1] Radboud Univ Nijmegen, Med Ctr, Dept Med Microbiol, NL-6525 ED Nijmegen, Netherlands
[2] Kenya Govt Med Res Ctr, Ctr Global Hlth Res, Kisumu, Kenya
[3] Ctr Dis Control & Prevent, Kisumu, Kenya
[4] London Sch Hyg & Trop Med, Fac Infect & Trop Dis, Dept Dis Control, London WC1E 7HT, England
[5] London Sch Hyg & Trop Med, Fac Infect & Trop Dis, Dept Immunol & Infect, London WC1E 7HT, England
关键词
Plasmodium; Malaria; Antibodies; IgG; DNA; Submicroscopic; Extraction; Transmission; PCR; ELISA; DRIED BLOOD SPOTS; PLASMODIUM-FALCIPARUM; PARASITES; ELIMINATION; BURDEN; AREA; INFECTIONS; PROVINCE; IMPACT; TERM;
D O I
10.1186/1475-2875-12-272
中图分类号
R51 [传染病];
学科分类号
100401 ;
摘要
Background: Informing and evaluating malaria control efforts relies on knowledge of local transmission dynamics. Serological and molecular tools have demonstrated great sensitivity to quantify transmission intensity in low endemic settings where the sensitivity of traditional methods is limited. Filter paper blood spots are commonly used a source of both DNA and antibodies. To enhance the operational practicability of malaria surveys, a method is presented for combined DNA extraction and antibody elution. Methods: Filter paper blood spots were collected as part of a large cross-sectional survey in the Kenyan highlands. DNA was extracted using a saponin/chelex method. The eluate of the first wash during the DNA extraction process was used for antibody detection and compared with previously validated antibody elution procedures. Antibody elution efficiency was assessed by total IgG ELISA for malaria antigens apical membrane antigen-1 (AMA-1) and merozoite-surface protein-1 (MSP-1(42)). The sensitivity of nested 18S rRNA and cytochrome b PCR assays and the impact of doubling filter paper material for PCR sensitivity were determined. The distribution of cell material and antibodies throughout filter paper blood spots were examined using luminescent and fluorescent reporter assays. Results: Antibody levels measured after the combined antibody/DNA extraction technique were strongly correlated to those measured after standard antibody elution (p < 0.0001). Antibody levels for both AMA-1 and MSP-142 were generally slightly lower (11.3-21.4%) but age-seroprevalence patterns were indistinguishable. The proportion of parasite positive samples ranged from 12.9% to 19.2% in the different PCR assays. Despite strong agreement between outcomes of different PCR assays, none of the assays detected all parasite-positive individuals. For all assays doubling filter paper material for DNA extraction increased sensitivity. The concentration of cell and antibody material was not homogenously distributed throughout blood spots. Conclusion: Combined DNA extraction and antibody elution is an operationally attractive approach for high throughput assessment of cumulative malaria exposure and current infection prevalence in endemic settings. Estimates of antibody prevalence are unaffected by the combined extraction and elution procedure. The choice of target gene and the amount and source of filter paper material for DNA extraction can have a marked impact on PCR sensitivity.
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