4.7 Article

Pfhrp2-Deleted Plasmodium falciparum Parasites in the Democratic Republic of the Congo: A National Cross-sectional Survey

期刊

JOURNAL OF INFECTIOUS DISEASES
卷 216, 期 1, 页码 36-44

出版社

OXFORD UNIV PRESS INC
DOI: 10.1093/infdis/jiw538

关键词

rapid diagnostic tests; false-negative; diagnostic resistance; histidine-rich protein 2; pfhrp3; hrp2; hrp3; RDT; deletion; malaria

资金

  1. National Institutes of Allergy and Infectious Diseases [5T32AI007151, 5R01AI107949]
  2. Population Research Infrastructure Program through Eunice Kennedy Shriver National Institute of Child Health and Human Development [P2C HD050924]
  3. National Science Foundation [BCS-1339949]
  4. UK Medical Research Council (MRC)
  5. Department for International Development (DfID) under the MRC/DfID concordat
  6. Division Of Behavioral and Cognitive Sci
  7. Direct For Social, Behav & Economic Scie [1339949] Funding Source: National Science Foundation
  8. MRC [MR/N01507X/1] Funding Source: UKRI
  9. Medical Research Council [MR/K010174/1B, MR/N01507X/1] Funding Source: researchfish

向作者/读者索取更多资源

Background. Rapid diagnostic tests (RDTs) account for more than two-thirds of malaria diagnoses in Africa. Deletions of the Plasmodium falciparum hrp2 (pfhrp2) gene cause false-negative RDT results and have never been investigated on a national level. Spread of pfhrp2-deleted P. falciparum mutants, resistant to detection by HRP2-based RDTs, would represent a serious threat to malaria elimination efforts. Methods. Using a nationally representative cross-sectional study of 7,137 children under five years of age from the Democratic Republic of Congo (DRC), we tested 783 subjects with RDT-/PCR+ results using PCR assays to detect and confirm deletions of the pfhrp2 gene. Spatial and population genetic analyses were employed to examine the distribution and evolution of these parasites. Results. We identified 149 pfhrp2-deleted parasites, representing 6.4% of all P. falciparum infections country-wide (95% confidence interval 5.1-8.0%). Bayesian spatial analyses identified statistically significant clustering of pfhrp2 deletions near Kinshasa and Kivu. Population genetic analysis revealed significant genetic differentiation between wild-type and pfhrp2-deleted parasite populations (G(ST)=.046, p <=.00001). Conclusions. Pfhrp2-deleted P. falciparum is a common cause of RDT-/ PCR+ malaria among asymptomatic children in the DRC and appears to be clustered within select communities. Surveillance for these deletions is needed, and alternatives to HRP2specific RDTs may be necessary.

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