PCR-based detection of Plasmodium falciparum in saliva using mitochondrial cox3 and varATS primers

Abstract Background Sampling of saliva for diagnosing Plasmodium falciparum infections is a safe, non-invasive alternative to sampling of blood. However, the use of saliva presents a challenge because lower concentrations of parasite DNA are present in saliva compared to peripheral blood. Therefore,...

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Bibliographic Details
Published in:Tropical Medicine and Health
Main Authors: Yukie M. Lloyd, Livo F. Esemu, Jovikka Antallan, Bradley Thomas, Samuel Tassi Yunga, Bekindaka Obase, Nana Christine, Rose G. F. Leke, Richard Culleton, Kenji Obadiah Mfuh, Vivek R. Nerurkar, Diane Wallace Taylor
Format: Article in Journal/Newspaper
Language:English
Published: BMC 2018
Subjects:
Malaria diagnosis
Saliva-based assays
Detection
Cameroon
Plasmodium falciparum
Malaria surveillance
Arctic medicine. Tropical medicine
RC955-962
Arctic
Online Access:https://doi.org/10.1186/s41182-018-0100-2
https://doaj.org/article/8d6cc5c71be54b6bbfaa70dcf2290553
Description
Summary:Abstract Background Sampling of saliva for diagnosing Plasmodium falciparum infections is a safe, non-invasive alternative to sampling of blood. However, the use of saliva presents a challenge because lower concentrations of parasite DNA are present in saliva compared to peripheral blood. Therefore, a sensitive method is needed for detection of parasite DNA in saliva. This study utilized two recently reported “ultra-sensitive” PCR assays based on detection of the P. falciparum mitochondrial cox3 gene and the multi-copy nuclear varATS gene. The ultra-sensitive assays have an advantage over standard 18S rRNA gene-based PCR assay as they target genes with higher copy numbers per parasite genome. Stored saliva DNA samples from 60 Cameroonian individuals with infections previously confirmed by 18S rRNA gene PCR in peripheral blood were tested with assays targeting the cox3 and varATS genes. Results Overall, the standard 18S rRNA gene-based PCR assay detected P. falciparum DNA in 62% of the stored saliva DNA samples, whereas 77 and 68% of the samples were positive with assays that target the cox3 and varATS genes, respectively. Interestingly, the ultra-sensitive assays detected more P. falciparum infections in stored saliva samples than were originally detected by thick-film microscopy (41/60 = 68%). When stratified by number of parasites in the blood, the cox3 assay successfully detected more than 90% of infections using saliva when individuals had > 1000 parasites/μl of peripheral blood, but sensitivity was reduced at submicroscopic parasitemia levels. Bands on electrophoresis gels were distinct for the cox3 assay, whereas faint or non-specific bands were sometimes observed for varATS and 18S rRNA that made interpretation of results difficult. Assays could be completed in 3.5 and 3 h for the cox3 and varATS assays, respectively, whereas the 18S rRNA gene assays required at least 7 h. Conclusions This study demonstrates that a PCR assay targeting the cox3 gene detected P. falciparum DNA in more saliva samples than ...

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