Genetic diversity of msp3α and msp1 _b5 markers of Plasmodium vivax in French Guiana

Abstract Background Reliable molecular typing tools are required for a better understanding of the molecular epidemiology of Plasmodium vivax . The genes msp3a and msp1 _block5 are highly polymorphic and have been used as markers in many P. vivax population studies. These markers were used to assess...

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Bibliographic Details
Published in:Malaria Journal
Main Authors: Carme Bernard, Simon Stéphane, Volney Béatrice, Yrinesi Joséphine, Legrand Eric, Véron Vincent
Format: Article in Journal/Newspaper
Language:English
Published: BMC 2009
Subjects:
Arctic medicine. Tropical medicine
RC955-962
Infectious and parasitic diseases
RC109-216
Arctic
Online Access:https://doi.org/10.1186/1475-2875-8-40
https://doaj.org/article/97e779a8eb834871a17e5e47a05f3525
Description
Summary:Abstract Background Reliable molecular typing tools are required for a better understanding of the molecular epidemiology of Plasmodium vivax . The genes msp3a and msp1 _block5 are highly polymorphic and have been used as markers in many P. vivax population studies. These markers were used to assess the genetic diversity of P. vivax strains from French Guiana (South America) and to develop a molecular typing protocol. Methods A total of 120 blood samples from 109 patients (including 10 patients suffered from more than one malaria episode, samples were collected during each episode) with P. vivax infection were genotyped. All samples were analysed by msp3a PCR-RFLP and msp1 _b5 gene sequencing was performed on 57 samples. Genotyping protocol applied to distinguish between new infection or relapse from heterologus hypnozoites and treatment failure or relapse from homologus hypnozoites was based on analysing first msp3a by PCR-RFLP and secondly, only if the genotypes of the two samples are identical, on sequencing the msp1 _b5 gene. Results msp3a alleles of three sizes were amplified by PCR: types A, B and C. Eleven different genotypes were identified among the 109 samples analysed by msp3a PCR-RFLP. In 13.8% of cases, a mixed genotype infection was observed. The sequence of msp1_ b5 gene revealed 22 unique genotypes and 12.3% of cases with mixed infection. In the 57 samples analysed by both methods, 45 genotypes were found and 21% were mixed. Among ten patients with two or three malaria episodes, the protocol allowed to identify five new infections or relapses from heterologous hypnozoites and six treatment failures of relapses from homologous hypnozoites. Conclusion The study showed a high diversity of msp3a and msp1_ b5 genetic markers among P. vivax strains in French Guiana with a low polyclonal infection rate. These results indicated that the P. vivax genotyping protocol presented has a good discrimination power and can be used in clinical drug trials or epidemiological studies.

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