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

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 de...

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Autores principales: Canier, Lydie, Khim, Nimol, Kim, Saorin, Sluydts, Vincent, Heng, Somony, Dourng, Dany, Eam, Rotha, Chy, Sophy, Khean, Chanra, Loch, Kaknika, Ken, Malen, Lim, Hokkean, Siv, Sovannaroath, Tho, Sochantha, Masse-Navette, Pascal, Gryseels, Charlotte, Uk, Sambunny, Van Roey, Karel, Grietens, Koen Peeters, Sokny, Mao, Thavrin, Boukheng, Chuor, Char Meng, Deubel, Vincent, Durnez, Lies, Coosemans, Marc, Ménard, Didier
Formato: Online Artículo Texto
Lenguaje:English
Publicado: BioMed Central 2013
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3829804/
https://www.ncbi.nlm.nih.gov/pubmed/24206649
http://dx.doi.org/10.1186/1475-2875-12-405
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author Canier, Lydie
Khim, Nimol
Kim, Saorin
Sluydts, Vincent
Heng, Somony
Dourng, Dany
Eam, Rotha
Chy, Sophy
Khean, Chanra
Loch, Kaknika
Ken, Malen
Lim, Hokkean
Siv, Sovannaroath
Tho, Sochantha
Masse-Navette, Pascal
Gryseels, Charlotte
Uk, Sambunny
Van Roey, Karel
Grietens, Koen Peeters
Sokny, Mao
Thavrin, Boukheng
Chuor, Char Meng
Deubel, Vincent
Durnez, Lies
Coosemans, Marc
Ménard, Didier
author_facet Canier, Lydie
Khim, Nimol
Kim, Saorin
Sluydts, Vincent
Heng, Somony
Dourng, Dany
Eam, Rotha
Chy, Sophy
Khean, Chanra
Loch, Kaknika
Ken, Malen
Lim, Hokkean
Siv, Sovannaroath
Tho, Sochantha
Masse-Navette, Pascal
Gryseels, Charlotte
Uk, Sambunny
Van Roey, Karel
Grietens, Koen Peeters
Sokny, Mao
Thavrin, Boukheng
Chuor, Char Meng
Deubel, Vincent
Durnez, Lies
Coosemans, Marc
Ménard, Didier
author_sort Canier, Lydie
collection PubMed
description 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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spelling pubmed-38298042013-11-16 An innovative tool for moving malaria PCR detection of parasite reservoir into the field Canier, Lydie Khim, Nimol Kim, Saorin Sluydts, Vincent Heng, Somony Dourng, Dany Eam, Rotha Chy, Sophy Khean, Chanra Loch, Kaknika Ken, Malen Lim, Hokkean Siv, Sovannaroath Tho, Sochantha Masse-Navette, Pascal Gryseels, Charlotte Uk, Sambunny Van Roey, Karel Grietens, Koen Peeters Sokny, Mao Thavrin, Boukheng Chuor, Char Meng Deubel, Vincent Durnez, Lies Coosemans, Marc Ménard, Didier Malar J Research 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. BioMed Central 2013-11-09 /pmc/articles/PMC3829804/ /pubmed/24206649 http://dx.doi.org/10.1186/1475-2875-12-405 Text en Copyright © 2013 Canier et al.; licensee BioMed Central Ltd. http://creativecommons.org/licenses/by/2.0 This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited. The Creative Commons Public Domain Dedication waiver (http://creativecommons.org/publicdomain/zero/1.0/) applies to the data made available in this article, unless otherwise stated.
spellingShingle Research
Canier, Lydie
Khim, Nimol
Kim, Saorin
Sluydts, Vincent
Heng, Somony
Dourng, Dany
Eam, Rotha
Chy, Sophy
Khean, Chanra
Loch, Kaknika
Ken, Malen
Lim, Hokkean
Siv, Sovannaroath
Tho, Sochantha
Masse-Navette, Pascal
Gryseels, Charlotte
Uk, Sambunny
Van Roey, Karel
Grietens, Koen Peeters
Sokny, Mao
Thavrin, Boukheng
Chuor, Char Meng
Deubel, Vincent
Durnez, Lies
Coosemans, Marc
Ménard, Didier
An innovative tool for moving malaria PCR detection of parasite reservoir into the field
title An innovative tool for moving malaria PCR detection of parasite reservoir into the field
title_full An innovative tool for moving malaria PCR detection of parasite reservoir into the field
title_fullStr An innovative tool for moving malaria PCR detection of parasite reservoir into the field
title_full_unstemmed An innovative tool for moving malaria PCR detection of parasite reservoir into the field
title_short An innovative tool for moving malaria PCR detection of parasite reservoir into the field
title_sort innovative tool for moving malaria pcr detection of parasite reservoir into the field
topic Research
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3829804/
https://www.ncbi.nlm.nih.gov/pubmed/24206649
http://dx.doi.org/10.1186/1475-2875-12-405
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