In vitro and ex vivo activity of an Azadirachta indica A.Juss. seed kernel extract on early sporogonic development of Plasmodium in comparison with azadirachtin A, its most abundant constituent

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• 作者：Nisha Dahiya^a ; ^{nisha.dahiya@unicam.it} ; ^{nisha_072@hotmail.com} ; Giuseppina Chianese^b ; ^{g.chianese@unina.it} ; Solomon Mequanente Abay^a ; ^c ; ^{solomonabay@gmail.com} ; Orazio Taglialatela-Scafati^b ; ^{scatagli@unina.it} ; Fulvio Esposito^a ; ^{fulvio.esposito@unicam.it} ; Giulio Lupidi^a ; ^{giulio.lupidi@unicam.it} ; Massimo Bramucci^a ; ^{massimo.bramucci@unicam.it} ; Luana Quassinti^a ; ^{luana.quassinti@unicam.it} ; George Christophides^d ; ^{g.christophides@imperial.ac.uk} ; Annette Habluetzel^a ; ^{annette.habluetzel@unicam.it} ; Leonardo Lucantoni^a ; ^e ; ^{l.lucantoni@griffith.edu.au}
• 关键词：NeemAzal® ; Azadirachtin A ; Pharmacodynamics ; Exflagellation ; Plasmodium
• 刊名：Phytomedicine
• 出版年：2016
• 出版时间：15 December 2016
• 年：2016
• 卷：23
• 期：14
• 页码：1743-1752
• 全文大小：1787 K
• 卷排序：23

文摘

NeemAzal® (NA) is a quantified extract from seed kernels of neem, Azadirachta indica A.Juss. (Meliaceae), with a wide spectrum of biological properties, classically ascribed to its limonoid content. NA contains several azadirachtins (A to L), azadirachtin A (AzaA) being its main constituent. AzaA has been shown to inhibit microgamete formation of the rodent malaria parasite Plasmodium berghei, and NA was found to completely inhibit the transmission of Plasmodium berghei to Anopheles stephensi mosquitoes when administered to gametocytemic mice at a corresponding AzaA dose of 50 mg/kg before exposure to mosquitoes.PurposeThe present study was aimed at i) assessing the pharmacodynamics and duration of action of NA and AzaA against P. berghei exflagellation in systemic circulation in mice and ii) elucidating the transmission blocking activity (TBA) of the main NA constituents.Study designThe NA and AzaA pharmacodynamics on exflagellation were assessed through ex vivo exflagellation assays, while TBA of NA constituents was evaluated through in vitro ookinete development assay.MethodsPharmacodynamics experiments: Peripheral blood from P. berghei infected BALB/c mice with circulating mature gametocytes, were treated i.p. with 50 mg/kg and 100 mg/kg pure AzaA and with NeemAzal® (Trifolio-M GmbH) at the corresponding AzaA concentrations. The effect magnitude and duration of action of compounds was estimated by counting exflagellation centers, formed by microgametocytes in process of releasing flagellated gametes, at various time points after treatment in ex vivo exflagellation tests. Ookinete Development Assay: The direct effects of NeemAzal® and AzaA on ookinete development were measured by fluorescence microscopy after incubation of gametocytemic blood with various concentrations of test substances in microplates for 24 h.ResultsThe exflagellation tests revealed an half-life of NA anti-plasmodial compounds of up to 7 h at a NA dose corresponding to 100 mg/kg equivalent dose of AzaA. The ookinete development assay showed an increased activity of NA against early sporogonic stages compared to that of AzaA. The IC50 value determined for NA was 6.8 µg/ml (CI95: 5.95–7.86), about half of the AzaA IC50 (12.4 µg/ml; CI95: 11.0–14.04).ConclusionThe stronger activity of NA, when compared to AzaA, could not be explained by an additive or synergistic effect by other azadirachtins (B, D and I) present in NA. In fact, the addition of these compounds at 50 µM concentration to AzaA did not evidence any decrease of the IC50 against early sporogonic stages to that obtained with AzaA alone. It is likely that other non-limonoid compounds present in NA may contribute to AzaA activity and enhanced pharmacodynamics against exflagellation both in vitro and in vivo.