Literature DB >> 29016335

Performance of Loop-Mediated Isothermal Amplification for the Identification of Submicroscopic Plasmodium falciparum Infection in Uganda.

Shereen Katrak1, Maxwell Murphy1, Patience Nayebare2, John Rek2, Mary Smith3, Emmanuel Arinaitwe4,2, Joaniter I Nankabirwa5,2, Moses Kamya5,2, Grant Dorsey1, Philip J Rosenthal1, Bryan Greenhouse1.   

Abstract

Accurately identifying and targeting the human reservoir of malaria parasitemia is critical for malaria control, and requires a reliable and sensitive diagnostic method. Loop-mediated isothermal amplification (LAMP) is increasingly used to diagnose submicroscopic parasitemia. Although most published studies report the sensitivity of LAMP compared with nested polymerase chain reaction (PCR) as ≥ 80%, they have failed to use a consistent, sensitive diagnostic as a comparator. We used cross-sectional samples from children and adults in Tororo, Uganda, a region with high but declining transmission due to indoor residual spraying, to characterize the sensitivity and specificity of pan-Plasmodium LAMP for detecting submicroscopic infections. We compared LAMP results targeting a mitochondrial DNA sequence conserved in all Plasmodium species, performed on DNA extracted from dried blood spots, to those of a gold standard quantitative PCR assay targeting the var gene acidic terminal sequence of Plasmodium falciparum (varATS qPCR), performed on DNA extracted from 200 µL of whole blood. Using LAMP and varATS qPCR increased the detection of parasitemia 2- to 5-fold, compared with microscopy. Among microscopy-negative samples, the sensitivity of LAMP was 81.5% for detecting infection ≥ 1 parasites/µL. However, low density infections were common, and LAMP failed to identify more than half of all infections diagnosed by varATS qPCR, performing with an overall sensitivity of 44.7% for detecting submicroscopic infections ≥ 0.01 parasites/µL. Thus, although the LAMP assay is more sensitive than microscopy, it missed a significant portion of the submicroscopic reservoir. These findings have important implications for malaria control, particularly in settings where low-density infections predominate.

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Year:  2017        PMID: 29016335      PMCID: PMC5805042          DOI: 10.4269/ajtmh.17-0225

Source DB:  PubMed          Journal:  Am J Trop Med Hyg        ISSN: 0002-9637            Impact factor:   2.345


  32 in total

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5.  The effect of indoor residual spraying on malaria and anemia in a high-transmission area of northern Uganda.

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3.  Persistent Parasitemia Despite Dramatic Reduction in Malaria Incidence After 3 Rounds of Indoor Residual Spraying in Tororo, Uganda.

Authors:  Joaniter I Nankabirwa; Jessica Briggs; John Rek; Emmanuel Arinaitwe; Patience Nayebare; Shereen Katrak; Sarah G Staedke; Philip J Rosenthal; Isabel Rodriguez-Barraquer; Moses R Kamya; Grant Dorsey; Bryan Greenhouse
Journal:  J Infect Dis       Date:  2019-03-15       Impact factor: 5.226

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Authors:  Jimmy Vareta; Andrea G Buchwald; Angelica Barrall; Lauren M Cohee; Jenny A Walldorf; Jenna E Coalson; Karl Seydel; Alick Sixpence; Don P Mathanga; Terrie E Taylor; Miriam K Laufer
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5.  Limitations of rapid diagnostic tests in malaria surveys in areas with varied transmission intensity in Uganda 2017-2019: Implications for selection and use of HRP2 RDTs.

Authors:  Agaba B Bosco; Joaniter I Nankabirwa; Adoke Yeka; Sam Nsobya; Karryn Gresty; Karen Anderson; Paul Mbaka; Christiane Prosser; David Smith; Jimmy Opigo; Rhoda Namubiru; Emmanuel Arinaitwe; John Kissa; Samuel Gonahasa; Sungho Won; Bora Lee; Chae Seung Lim; Charles Karamagi; Qin Cheng; Joan K Nakayaga; Moses R Kamya
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6.  Microscopic and submicroscopic infection by Plasmodium falciparum: Immunoglobulin M and A profiles as markers of intensity and exposure.

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7.  Rapid diagnosis of Plasmodium falciparum malaria using a point-of-care loop-mediated isothermal amplification device.

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