Assessing drug efficacy against Plasmodium falciparum liver stages in vivo
Erika L. Flannery, … , Stefan H.I. Kappe, Sebastian A. Mikolajczak
Erika L. Flannery, … , Stefan H.I. Kappe, Sebastian A. Mikolajczak
Published January 11, 2018
Citation Information: JCI Insight. 2018;3(1):e92587. https://doi.org/10.1172/jci.insight.92587.
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Resource and Technical Advance Infectious disease Microbiology

Assessing drug efficacy against Plasmodium falciparum liver stages in vivo

Abstract

Malaria eradication necessitates new tools to fight the evolving and complex Plasmodium pathogens. These tools include prophylactic drugs that eliminate Plasmodium liver stages and consequently prevent clinical disease, decrease transmission, and reduce the propensity for resistance development. Currently, the identification of these drugs relies on in vitro P. falciparum liver stage assays or in vivo causal prophylaxis assays using rodent malaria parasites; there is no method to directly test in vivo liver stage activity of candidate antimalarials against the human malaria–causing parasite P. falciparum. Here, we use a liver-chimeric humanized mouse (FRG huHep) to demonstrate in vivo P. falciparum liver stage development and describe the efficacy of clinically used and candidate antimalarials with prophylactic activity. We show that daily administration of atovaquone-proguanil (ATQ-PG; ATQ, 30 mg/kg, and PG, 10 mg/kg) protects 5 of 5 mice from liver stage infection, consistent with the use in humans as a causal prophylactic drug. Single-dose primaquine (60 mg/kg) has similar activity to that observed in humans, demonstrating the activity of this drug (and its active metabolites) in FRG huHep mice. We also show that DSM265, a selective Plasmodial dihydroorotate dehydrogenase inhibitor with causal prophylactic activity in humans, reduces liver stage burden in FRG huHep mice. Finally, we measured liver stage–to–blood stage transition of the parasite, the ultimate readout of prophylactic activity and measurement of infective capacity of parasites in the liver, to show that ATQ-PG reduces blood stage patency to below the limit of quantitation by quantitative PCR (qPCR). The FRG huHep model, thus, provides a platform for preclinical evaluation of drug candidates for liver stage causal prophylactic activity, pharmacokinetic/pharmacodynamics studies, and biological studies to investigate the mechanism of action of liver stage active antimalarials.

Authors

Erika L. Flannery, Lander Foquet, Vorada Chuenchob, Matthew Fishbaugher, Zachary Billman, Mary Jane Navarro, William Betz, Tayla M. Olsen, Joshua Lee, Nelly Camargo, Thao Nguyen, Carola Schafer, Brandon K. Sack, Elizabeth M. Wilson, Jessica Saunders, John Bial, Brice Campo, Susan A. Charman, Sean C. Murphy, Margaret A. Phillips, Stefan H.I. Kappe, Sebastian A. Mikolajczak

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Figure 6

Experimental design for testing liver stage efficacy of antimalarials against P. falciparum.

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Experimental design for testing liver stage efficacy of antimalarials ag...
Mature, luciferase-expressing P. falciparum (Pf NF54 GFP-luc) gametocytes are produced in vitro in hRBC culture. Mosquitoes are infected with mature stage V gametocytes using a standard membrane feeding assay. Fourteen days after feeding, FRG huHep mice are infected by mosquito bite or i.v. injection with freshly dissected salivary gland sporozoites. P. falciparum liver parasite burden is quantified 4–6 days after infection by live in vivo bioluminescence imaging or liver harvest and Plasmodium 18S rRNA qPCR. Optionally, injection of hRBCs on day 5 after infection and subsequent days captures the liver stage–to–blood stage transition on days 7–9.