Optimizing the HRP-2 in vitro malaria drug susceptibility assay using a reference clone to improve comparisons of Plasmodium falciparum field isolates

Wiriya Rutvisuttinunt; Suwanna Chaorattanakawee; Stuart D Tyner; Paktiya Teja-Isavadharm; Youry Se; Kritsanai Yingyuen; Panjaporn Chaichana; Delia Bethell; Douglas S Walsh; Chanthap Lon; Mark Fukuda; Duong Socheat; Harald Noedl; Kurt Schaecher; David L Saunders

doi:10.1186/1475-2875-11-325

Optimizing the HRP-2 in vitro malaria drug susceptibility assay using a reference clone to improve comparisons of Plasmodium falciparum field isolates

Malar J. 2012 Sep 13:11:325. doi: 10.1186/1475-2875-11-325.

Authors

Wiriya Rutvisuttinunt¹, Suwanna Chaorattanakawee, Stuart D Tyner, Paktiya Teja-Isavadharm, Youry Se, Kritsanai Yingyuen, Panjaporn Chaichana, Delia Bethell, Douglas S Walsh, Chanthap Lon, Mark Fukuda, Duong Socheat, Harald Noedl, Kurt Schaecher, David L Saunders

Affiliation

¹ Department of Immunology and Medicine, US Army Medical Corps, Armed Forces Research Institute of Medical Sciences (USAMC-AFRIMS), Bangkok, Thailand.

Abstract

Background: Apparent emerging artemisinin-resistant Plasmodium falciparum malaria in Southeast Asia requires development of practical tools to monitor for resistant parasites. Although in vitro anti-malarial susceptibility tests are widely used, uncertainties remain regarding interpretation of P. falciparum field isolate values.

Methods: Performance parameters of the W2 P. falciparum clone (considered artemisinin "sensitive") were evaluated as a reference for the HRP-2 immediate ex vivo assay. Variability in W2 IC50s was assessed, including intra- and inter-assay variability among and between technicians in multiple experiments, over five freeze-thaw cycles, over five months of continuous culture, and before and after transport of drug-coated plates to remote field sites. Nominal drug plate concentrations of artesunate (AS) and dihydroartemisinin (DHA) were verified by LC-MS analysis. Plasmodium falciparum field isolate IC50s for DHA from subjects in an artemisinin-resistant area in Cambodia were compared with W2 susceptibility.

Results: Plate drug concentrations and day-to-day technical assay performance among technicians were important sources of variability for W2 IC50s within and between assays. Freeze-thaw cycles, long-term continuous culture, and transport to and from remote sites had less influence. Despite variability in W2 susceptibility, the median IC50s for DHA for Cambodian field isolates were higher (p <0.0001) than the W2 clone (3.9 nM), both for subjects with expected (less than 72 hours; 6.3 nM) and prolonged (greater or equal to 72 hours; 9.6 nM) parasite clearance times during treatment with artesunate monotherapy.

Conclusion: The W2 reference clone improved the interpretability of field isolate susceptibility from the immediate ex vivo HRP-2 assay from areas of artemisinin resistance. Methods to increase the reproducibility of plate coating may improve overall assay interpretability and utility.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Antigens, Protozoan / analysis*
Antimalarials / pharmacology*
Artemisinins / pharmacology
Artesunate
Chromatography, Liquid
Culture Media / chemistry
Humans
Inhibitory Concentration 50
Malaria, Falciparum / parasitology*
Mass Spectrometry
Parasitic Sensitivity Tests / methods*
Parasitic Sensitivity Tests / standards*
Plasmodium falciparum / drug effects*
Plasmodium falciparum / isolation & purification
Protozoan Proteins / analysis*

Substances

Antigens, Protozoan
Antimalarials
Artemisinins
Culture Media
HRP-2 antigen, Plasmodium falciparum
Protozoan Proteins
Artesunate
artenimol