Impact of Plasmodium falciparum gene deletions on malaria rapid diagnostic test performance

Impact of Plasmodium falciparum gene deletions on malaria rapid diagnostic test performance

Malaria rapid diagnostic tests (RDTs) have greatly improved access to diagnosis in endemic countries. Most RDTs detect Plasmodium falciparum histidine-rich protein 2 (HRP2), but their sensitivity is seriously threatened by the emergence of pfhrp2-deleted parasites. RDTs detecting P. falciparum or pa...

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Veröffentlicht in:Malaria journal 2020-11, Vol.19 (1), p.392-392, Article 392
Hauptverfasser: Gatton, Michelle L, Chaudhry, Alisha, Glenn, Jeff, Wilson, Scott, Ah, Yong, Kong, Amy, Ord, Rosalynn L, Rees-Channer, Roxanne R, Chiodini, Peter, Incardona, Sandra, Cheng, Qin, Aidoo, Michael, Cunningham, Jane
Format: Artikel
Sprache:eng
Schlagworte:
Antigens
Clinical isolates
Culture techniques
Diagnosis
Diagnostic tests
Erythrocytes
Gene deletion
Gene mutation
Genetic aspects
Health aspects
Hisidine rich protein 2
Histidine
HRP2
Human diseases
Identification and classification
Innovations
L-Lactate dehydrogenase
Lactate
Lactic acid
Malaria
Medical testing products
Molecular diagnostic techniques
Parasites
Performance assessment
Plasmodium falciparum
Rapid diagnostic tests
Vector-borne diseases
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Zusammenfassung:Malaria rapid diagnostic tests (RDTs) have greatly improved access to diagnosis in endemic countries. Most RDTs detect Plasmodium falciparum histidine-rich protein 2 (HRP2), but their sensitivity is seriously threatened by the emergence of pfhrp2-deleted parasites. RDTs detecting P. falciparum or pan-lactate dehydrogenase (Pf- or pan-LDH) provide alternatives. The objective of this study was to systematically assess the performance of malaria RDTs against well-characterized pfhrp2-deleted P. falciparum parasites. Thirty-two RDTs were tested against 100 wild-type clinical isolates (200 parasites/µL), and 40 samples from 10 culture-adapted and clinical isolates of pfhrp2-deleted parasites. Wild-type and pfhrp2-deleted parasites had comparable Pf-LDH concentrations. Pf-LDH-detecting RDTs were also tested against 18 clinical isolates at higher density (2,000 parasites/µL) lacking both pfhrp2 and pfhrp3. RDT positivity against pfhrp2-deleted parasites was highest (> 94%) for the two pan-LDH-only RDTs. The positivity rate for the nine Pf-LDH-detecting RDTs varied widely, with similar median positivity between double-deleted (pfhrp2/3 negative; 63.9%) and single-deleted (pfhrp2-negative/pfhrp3-positive; 59.1%) parasites, both lower than against wild-type P. falciparum (93.8%). Median positivity for HRP2-detecting RDTs against 22 single-deleted parasites was 69.9 and 35.2% for HRP2-only and HRP2-combination RDTs, respectively, compared to 96.0 and 92.5% for wild-type parasites. Eight of nine Pf-LDH RDTs detected all clinical, double-deleted samples at 2,000 parasites/µL. The pan-LDH-only RDTs evaluated performed well. Performance of Pf-LDH-detecting RDTs against wild-type P. falciparum does not necessarily predict performance against pfhrp2-deleted parasites. Furthermore, many, but not all HRP2-based RDTs, detect pfhrp2-negative/pfhrp3-positive samples, with implications for the HRP2-based RDT screening approach for detection and surveillance of HRP2-negative parasites.
ISSN:1475-2875
1475-2875
DOI:10.1186/s12936-020-03460-w