Malaria surveillance from both ends: concurrent detection of Plasmodium falciparum in saliva and excreta harvested from Anopheles mosquitoes

Ramirez, AL; van den Hurk, AF; Mackay, IM; Yang, ASP; Hewitson, GR; McMahon, JL; Boddey, JA; Ritchie, SA; Erickson, SM

Author(s): Ramirez, AL; van den Hurk, AF; Mackay, IM; Yang, ASP; Hewitson, GR; McMahon, JL; Boddey, JA; Ritchie, SA; Erickson, SM;
Details: Publication Year 2019-07-18,Volume 12,Issue #1,Page 355
Journal Title: Parasites & Vectors
Publication Type: Journal Article
Abstract: BACKGROUND: Malaria is the most important vector-borne disease in the world. Epidemiological and ecological studies of malaria traditionally utilize detection of Plasmodium sporozoites in whole mosquitoes or salivary glands by microscopy or serological or molecular assays. However, these methods are labor-intensive, and can over- or underestimate mosquito transmission potential. To overcome these limitations, alternative sample types have been evaluated for the study of malaria. It was recently shown that Plasmodium could be detected in saliva expectorated on honey-soaked cards by Anopheles stephensi, providing a better estimate of transmission risk. We evaluated whether excretion of Plasmodium falciparum nucleic acid by An. stephensi correlates with expectoration of parasites in saliva, thus providing an additional sample type for estimating transmission potential. Mosquitoes were exposed to infectious blood meals containing cultured gametocytes, and excreta collected at different time points post-exposure. Saliva was collected on honey-soaked filter paper cards, and salivary glands were dissected and examined microscopically for sporozoites. Excreta and saliva samples were tested by real time polymerase chain reaction (RT-rtPCR). RESULTS: Plasmodium falciparum RNA was detected in mosquito excreta as early as four days after ingesting a bloodmeal containing gametocytes. Once sporogony (the development of sporozoites) occurred, P. falciparum RNA was detected concurrently in both excreta and saliva samples. In the majority of cases, no difference was observed between the Ct values obtained from matched excreta and saliva samples, suggesting that both samples provide equally sensitive results. A positive association was observed between the molecular detection of the parasites in both samples and the proportion of mosquitoes with sporozoites in their salivary glands from each container. No distinguishable parasites were observed when excreta samples were stained and microscopically analyzed. CONCLUSIONS: Mosquito saliva and excreta are easily collected and are promising for surveillance of malaria-causing parasites, especially in low transmission settings or in places where arboviruses co-circulate.
Publisher: BMC
Research Division(s): Infectious Diseases And Immune Defence
PubMed ID: 31319880
Publisher's Version: https://doi.org/10.1186/s13071-019-3610-9
Open Access at Publisher's Site: https://doi.org/10.1186/s13071-019-3610-9
NHMRC Grants: NHMRC/1123727,
Terms of Use/Rights Notice: Refer to copyright notice on published article.
Documents: Ramirez et al_Parasites Vectors_2019.pdf - (1.88MB, application/pdf)

Creation Date: 2019-07-26 09:44:16

Last Modified: 2019-08-13 01:09:12