An innovative tool for moving malaria PCR detection of parasite reservoir into the field

Lydie Canier; Nimol Khim; Saorin Kim; Vincent Sluydts; Somony Heng; Dany Dourng; Rotha Eam; Sophy Chy; Chanra Khean; Kaknika Loch; Malen Ken; Hokkean Lim; Sovannaroath Siv; Tho Sochantha; Pascal Masse-Navette; Charlotte Gryseels; Sambunny Uk; Karel Van Roey; Koen Peeters Grietens; Mao Sokny; Boukheng Thavrin; Char Meng Chuor; Vincent Deubel; Lies Durnez; Marc Coosemans; Didier Ménard

doi:10.1186/1475-2875-12-405

An innovative tool for moving malaria PCR detection of parasite reservoir into the field

Lydie Canier(Institut Pasteur du Cambodge), Nimol Khim(Institut Pasteur du Cambodge), Saorin Kim(Institut Pasteur du Cambodge), Vincent Sluydts(Instituut voor Tropische Geneeskunde), Somony Heng(Institut Pasteur du Cambodge), Dany Dourng(Institut Pasteur du Cambodge), Rotha Eam(Institut Pasteur du Cambodge), Sophy Chy(Institut Pasteur du Cambodge), Chanra Khean(Institut Pasteur du Cambodge), Kaknika Loch(Institut Pasteur du Cambodge), Malen Ken(Institut Pasteur du Cambodge), Hokkean Lim(Institut Pasteur du Cambodge), Sovannaroath Siv(Cambodia National Malaria Center), Tho Sochantha(Cambodia National Malaria Center), Pascal Masse-Navette(Institut Pasteur du Cambodge), Charlotte Gryseels(Instituut voor Tropische Geneeskunde), Sambunny Uk(Cambodia National Malaria Center), Karel Van Roey(Instituut voor Tropische Geneeskunde), Koen Peeters Grietens(Instituut voor Tropische Geneeskunde), Mao Sokny(Cambodia National Malaria Center), Boukheng Thavrin(Cambodia National Malaria Center), Char Meng Chuor(Cambodia National Malaria Center), Vincent Deubel(Institut Pasteur du Cambodge), Lies Durnez(Instituut voor Tropische Geneeskunde), Marc Coosemans(University of Antwerp), Didier Ménard(Institut Pasteur du Cambodge)

Malaria Journal

November 9, 2013

10.1186/1475-2875-12-405

Cited by 155Open Access

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Abstract

BACKGROUND: To achieve the goal of malaria elimination in low transmission areas such as in Cambodia, new, inexpensive, high-throughput diagnostic tools for identifying very low parasite densities in asymptomatic carriers are required. This will enable a switch from passive to active malaria case detection in the field. METHODS: DNA extraction and real-time PCR assays were implemented in an "in-house" designed mobile laboratory allowing implementation of a robust, sensitive and rapid malaria diagnostic strategy in the field. This tool was employed in a survey organized in the context of the MalaResT project (NCT01663831). RESULTS: The real-time PCR screening and species identification assays were performed in the mobile laboratory between October and November 2012, in Rattanakiri Province, to screen approximately 5,000 individuals in less than four weeks and treat parasite carriers within 24-48 hours after sample collection. An average of 240 clinical samples (and 40 quality control samples) was tested every day, six/seven days per week. Some 97.7% of the results were available <24 hours after the collection. A total of 4.9% were positive for malaria. Plasmodium vivax was present in 61.1% of the positive samples, Plasmodium falciparum in 45.9%, Plasmodium malariae in 7.0% and Plasmodium ovale in 2.0%. CONCLUSIONS: The operational success of this diagnostic set-up proved that molecular testing and subsequent treatment is logistically achievable in field settings. This will allow the detection of clusters of asymptomatic carriers and to provide useful epidemiological information. Fast results will be of great help for staff in the field to track and treat asymptomatic parasitaemic cases. The concept of the mobile laboratory could be extended to other countries for the molecular detection of malaria or other pathogens, or to culture vivax parasites, which does not support long-time delay between sample collection and culture.

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