Biodereplication of antiplasmodial extracts: application of the amazonian medicinal plant piper coruscans kunth

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Improved methodological tools to hasten antimalarial drug discovery remain of interest, especially when considering natural products as a source of drug candidates. We propose a biodereplication method combining the classical dereplication approach with the early detection of potential antiplasmodia...

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Detalles Bibliográficos
Autores: Vásquez Ocmín, Pedro, Gallard, Jean François, Van Baelen, Anne Cécile, Leblane, Karine, Cojean, Sandrine, Mouray, Elisabeth, Grellier, Philippe, Amasifuen Guerra, Carlos Alberto, Beniddir, Mehdi A., Evanno, Laurent, Figadère, Bruno, Maciuk, Alexandre
Formato: artículo
Fecha de Publicación:2022
Institución:Instituto Nacional de Innovación Agraria
Repositorio:INIA-Institucional
Lenguaje:inglés
OAI Identifier:oai:null:20.500.12955/1975
Enlace del recurso:https://hdl.handle.net/20.500.12955/1975
https://doi.org/10.3390/molecules27217638
Nivel de acceso:acceso abierto
Materia:Piper coruscans Kunth (Piperaceae)
Biodereplication
Heme binding
Mass Spectrometry
Plasmodium
https://purl.org/pe-repo/ocde/ford#4.05.00
Piperaceae
Replication
Spectrometry
Descripción
Sumario:Improved methodological tools to hasten antimalarial drug discovery remain of interest, especially when considering natural products as a source of drug candidates. We propose a biodereplication method combining the classical dereplication approach with the early detection of potential antiplasmodial compounds in crude extracts. Heme binding is used as a surrogate of the antiplasmodial activity and is monitored by mass spectrometry in a biomimetic assay. Molecular networking and automated annotation of targeted mass through data mining were followed by mass-guided compound isolation by taking advantage of the versatility and finely tunable selectivity offered by centrifugal partition chromatography. This biodereplication workflow was applied to an ethanolic extract of the Amazonian medicinal plant Piper coruscans Kunth (Piperaceae) showing an IC50 of 1.36 ug/mL on the 3D7 Plasmodium falciparum strain. It resulted in the isolation of twelve compounds designated as potential antiplasmodial compounds by the biodereplication workflow. Two chalcones, aurentiacin (1) and cardamonin (3), with IC50 values of 2.25 and 5.5 uM, respectively, can be considered to bear the antiplasmodial activity of the extract, with the latter not relying on a heme-binding mechanism. This biodereplication method constitutes a rapid, efficient, and robust technique to identify potential antimalarial compounds in complex extracts such as plant extracts.
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