Multiplex-RT-PCR-ELISA panel for detecting mosquito-borne pathogens : Plasmodium sp. preserved and eluted from dried blood spots on sample cards

dc.contributor.authorKoliopoulos, Philip
dc.contributor.authorKayange, Neema Mathias
dc.contributor.authorDaniel, Tim
dc.contributor.authorHuth, Florian
dc.contributor.authorGröndahl, Britta
dc.contributor.authorMedina-Montaño, Grey Carolina
dc.contributor.authorPretsch, Leah
dc.contributor.authorKlüber, Julia
dc.contributor.authorSchmidt, Christian
dc.contributor.authorZüchner, Antke
dc.contributor.authorUlbert, Sebastian
dc.contributor.authorMshana, Steven E.
dc.contributor.authorAddo, Marylyn
dc.contributor.authorGehring, Stephan
dc.date.accessioned2021-09-24T09:11:01Z
dc.date.available2021-09-24T09:11:01Z
dc.date.issued2021
dc.description.abstractBACKGROUND Children are the most vulnerable group affected by malaria and other tropical, vector-borne diseases in low-resource countries. Infants presenting with acute onset fever represent a major sector of outpatient care in the Lake Victoria region. Misclassification and overuse of antibiotics and anti-malarial medications are consistent problems. Identifying the prevalent mosquito-borne pathogens in the region will reduce the prescription of non-indicated medicines. METHODS The literature was reviewed focusing on the mosquito-borne pathogens most prevalent in sub-Saharan Africa. Accordingly, an assay comprised of a multiplex-reverse transcriptase-polymerase chain reaction and an enzyme-linked immunosorbent assay (multiplex-RT-PCR-ELISA) was designed and validated in its ability to identify and differentiate nine human mosquito-borne pathogens including eight arboviruses and Plasmodium sp., the aetiologic agents of malaria. Blood samples obtained from 132 children suspected of having malaria were spotted and preserved on Whatman® 903 protein sample cards. Multiplex-RT-PCR-ELISA analysis was assessed and compared to results obtained by blood smear microscopy and the malaria rapid diagnostic test (RDT). RESULTS Nine out of nine pathogens were amplified specifically by the multiplex-RT-PCR-ELISA panel. Twenty-seven out of 132 paediatric patients presenting with acute fever were infected with Plasmodium sp., confirmed by multiplex-RT-PCR. The results of blood smear microscopy were only 40% sensitive and 92.8% specific. The malaria RDT, on the other hand, detected acute Plasmodium infections with 96.3% sensitivity and 98.1% specificity. The preservation of Plasmodium sp. in clinical sera and whole blood samples spotted on sample cards was evaluated. The duration of successful, sample card storage was 186 to 312 days. CONCLUSIONS Reliable, easy-to-use point of care diagnostic tests are a powerful alternative to laboratory-dependent gold standard tests. The multiplex-RT-PCR-ELISA amplified and identified nine vector-borne pathogens including Plasmodium sp. with great accuracy. Translation of improved diagnostic approaches, i.e., multiplex-RT-PCR-ELISA, into effective treatment options promises to reduce childhood mortality and non-indicated prescriptions.en_GB
dc.identifier.doihttp://doi.org/10.25358/openscience-6365
dc.identifier.urihttps://openscience.ub.uni-mainz.de/handle/20.500.12030/6375
dc.language.isoengde
dc.rightsCC-BY-4.0*
dc.rights.urihttps://creativecommons.org/licenses/by/4.0/*
dc.subject.ddc610 Medizinde_DE
dc.subject.ddc610 Medical sciencesen_GB
dc.titleMultiplex-RT-PCR-ELISA panel for detecting mosquito-borne pathogens : Plasmodium sp. preserved and eluted from dried blood spots on sample cardsen_GB
dc.typeZeitschriftenaufsatzde
jgu.journal.titleMalaria journalde
jgu.journal.volume20de
jgu.organisation.departmentFB 04 Medizinde
jgu.organisation.nameJohannes Gutenberg-Universität Mainz
jgu.organisation.number2700
jgu.organisation.placeMainz
jgu.organisation.rorhttps://ror.org/023b0x485
jgu.pages.alternative66de
jgu.publisher.doi10.1186/s12936-021-03595-4
jgu.publisher.issn1475-2875de
jgu.publisher.nameBioMed Centralde
jgu.publisher.placeLondonde
jgu.publisher.urihttps://doi.org/10.1186/s12936-021-03595-4de
jgu.publisher.year2021
jgu.rights.accessrightsopenAccess
jgu.subject.ddccode610de
jgu.type.dinitypeArticleen_GB
jgu.type.resourceTextde
jgu.type.versionPublished versionde

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