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Genome-wide diversity and differentiation in New World populations of the human malaria parasite Plasmodium vivax

Identifieur interne : 000098 ( Hal/Curation ); précédent : 000097; suivant : 000099

Genome-wide diversity and differentiation in New World populations of the human malaria parasite Plasmodium vivax

Auteurs : Thais De Oliveira [Brésil] ; Priscila Rodrigues [Brésil] ; Maria Menezes [Brésil] ; Raquel Gonçalves-Lopes [Brésil] ; Melissa Bastos [Brésil] ; Nathália Lima [Brésil] ; Susana Barbosa [Brésil] ; Alexandra Gerber [Brésil] ; Guilherme Loss De Morais [Brésil] ; Luisa Berná [Uruguay] ; Jody Phelan [Royaume-Uni] ; Carlos Robello [Uruguay] ; Ana De Vasconcelos [Brésil] ; João Alves [Brésil] ; Marcelo Ferreira [Brésil]

Source :

RBID : Hal:pasteur-02046467

Abstract

BACKGROUND: The Americas were the last continent colonized by humans carrying malaria parasites. Plasmodium falciparum from the New World shows very little genetic diversity and greater linkage disequilibrium, compared with its African counterparts, and is clearly subdivided into local, highly divergent populations. However, limited available data have revealed extensive genetic diversity in American populations of another major human malaria parasite, P. vivax.METHODS: We used an improved sample preparation strategy and next-generation sequencing to characterize 9 high-quality P. vivax genome sequences from northwestern Brazil. These new data were compared with publicly available sequences from recently sampled clinical P. vivax isolates from Brazil (BRA, total n = 11 sequences), Peru (PER, n = 23), Colombia (COL, n = 31), and Mexico (MEX, n = 19).PRINCIPAL FINDINGS/CONCLUSIONS: We found that New World populations of P. vivax are as diverse (nucleotide diversity π between 5.2 × 10-4 and 6.2 × 10-4) as P. vivax populations from Southeast Asia, where malaria transmission is substantially more intense. They display several non-synonymous nucleotide substitutions (some of them previously undescribed) in genes known or suspected to be involved in antimalarial drug resistance, such as dhfr, dhps, mdr1, mrp1, and mrp-2, but not in the chloroquine resistance transporter ortholog (crt-o) gene. Moreover, P. vivax in the Americas is much less geographically substructured than local P. falciparum populations, with relatively little between-population genome-wide differentiation (pairwise FST values ranging between 0.025 and 0.092). Finally, P. vivax populations show a rapid decline in linkage disequilibrium with increasing distance between pairs of polymorphic sites, consistent with very frequent outcrossing. We hypothesize that the high diversity of present-day P. vivax lineages in the Americas originated from successive migratory waves and subsequent admixture between parasite lineages from geographically diverse sites. Further genome-wide analyses are required to test the demographic scenario suggested by our data.


Url:
DOI: 10.1371/journal.pntd.0005824

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<date type="datePub">2017-07-31</date>
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<p>BACKGROUND: The Americas were the last continent colonized by humans carrying malaria parasites. Plasmodium falciparum from the New World shows very little genetic diversity and greater linkage disequilibrium, compared with its African counterparts, and is clearly subdivided into local, highly divergent populations. However, limited available data have revealed extensive genetic diversity in American populations of another major human malaria parasite, P. vivax.METHODS: We used an improved sample preparation strategy and next-generation sequencing to characterize 9 high-quality P. vivax genome sequences from northwestern Brazil. These new data were compared with publicly available sequences from recently sampled clinical P. vivax isolates from Brazil (BRA, total n = 11 sequences), Peru (PER, n = 23), Colombia (COL, n = 31), and Mexico (MEX, n = 19).PRINCIPAL FINDINGS/CONCLUSIONS: We found that New World populations of P. vivax are as diverse (nucleotide diversity π between 5.2 × 10-4 and 6.2 × 10-4) as P. vivax populations from Southeast Asia, where malaria transmission is substantially more intense. They display several non-synonymous nucleotide substitutions (some of them previously undescribed) in genes known or suspected to be involved in antimalarial drug resistance, such as dhfr, dhps, mdr1, mrp1, and mrp-2, but not in the chloroquine resistance transporter ortholog (crt-o) gene. Moreover, P. vivax in the Americas is much less geographically substructured than local P. falciparum populations, with relatively little between-population genome-wide differentiation (pairwise FST values ranging between 0.025 and 0.092). Finally, P. vivax populations show a rapid decline in linkage disequilibrium with increasing distance between pairs of polymorphic sites, consistent with very frequent outcrossing. We hypothesize that the high diversity of present-day P. vivax lineages in the Americas originated from successive migratory waves and subsequent admixture between parasite lineages from geographically diverse sites. Further genome-wide analyses are required to test the demographic scenario suggested by our data.</p>
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<title xml:lang="en">Genome-wide diversity and differentiation in New World populations of the human malaria parasite Plasmodium vivax</title>
<author role="aut">
<persName>
<forename type="first">Thais</forename>
<forename type="middle">C</forename>
<surname>de Oliveira</surname>
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<author role="aut">
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<forename type="first">Priscila</forename>
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<surname>Rodrigues</surname>
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<forename type="first">Maria</forename>
<forename type="middle">José</forename>
<surname>Menezes</surname>
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<forename type="first">Raquel</forename>
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<surname>Gonçalves-Lopes</surname>
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<forename type="first">Melissa</forename>
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<surname>Bastos</surname>
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<forename type="first">Nathália</forename>
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<surname>Lima</surname>
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<forename type="first">Susana</forename>
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<email type="md5">7ca65118dc270c8d0d21da1dc0049493</email>
<email type="domain">liv.ac.uk</email>
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<author role="aut">
<persName>
<forename type="first">Alexandra</forename>
<forename type="middle">L</forename>
<surname>Gerber</surname>
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<forename type="first">Guilherme</forename>
<surname>LOSS DE MORAIS</surname>
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<forename type="first">Luisa</forename>
<surname>Berná</surname>
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<idno type="halauthorid">1522096</idno>
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<persName>
<forename type="first">Jody</forename>
<surname>Phelan</surname>
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<persName>
<forename type="first">Carlos</forename>
<surname>Robello</surname>
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<author role="aut">
<persName>
<forename type="first">Ana</forename>
<forename type="middle">Tereza Ribeiro</forename>
<surname>De Vasconcelos</surname>
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<email type="md5">22a5c460c18402ea83c4fd3b354f5e11</email>
<email type="domain">lncc.br</email>
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<persName>
<forename type="first">João</forename>
<forename type="middle">Marcelo P</forename>
<surname>Alves</surname>
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<forename type="first">Marcelo</forename>
<surname>Ferreira</surname>
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<surname>Ben Hassine</surname>
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<funder>Research was supported by research grants from the Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq), Brazil (590106/2011-2 to MUF), the Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP), Brazil (2010/51835-7 to MUF), and the National Institute of Allergy and Infectious Diseases (NIAID), National Institutes of Health (NIH), USA (International Centers of Excellence in Malaria Research [ICEMR] program, U19 AI089681 to Joseph M. Vinetz, University of California, San Diego); PTR was supported by a scholarship from CNPq, which also provided a senior researcher scholarship to MUF. RMG-L (2010/51938-0), NFL (2013/26928-0), and SB (2013/23770-6) were supported by scholarships from FAPESP and TCO was supported by a scholarship from the Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES), Brazil.</funder>
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<forename type="first">Thais</forename>
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<forename type="first">Alexandra</forename>
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<forename type="first">Ana</forename>
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<abstract xml:lang="en">
<p>BACKGROUND: The Americas were the last continent colonized by humans carrying malaria parasites. Plasmodium falciparum from the New World shows very little genetic diversity and greater linkage disequilibrium, compared with its African counterparts, and is clearly subdivided into local, highly divergent populations. However, limited available data have revealed extensive genetic diversity in American populations of another major human malaria parasite, P. vivax.METHODS: We used an improved sample preparation strategy and next-generation sequencing to characterize 9 high-quality P. vivax genome sequences from northwestern Brazil. These new data were compared with publicly available sequences from recently sampled clinical P. vivax isolates from Brazil (BRA, total n = 11 sequences), Peru (PER, n = 23), Colombia (COL, n = 31), and Mexico (MEX, n = 19).PRINCIPAL FINDINGS/CONCLUSIONS: We found that New World populations of P. vivax are as diverse (nucleotide diversity π between 5.2 × 10-4 and 6.2 × 10-4) as P. vivax populations from Southeast Asia, where malaria transmission is substantially more intense. They display several non-synonymous nucleotide substitutions (some of them previously undescribed) in genes known or suspected to be involved in antimalarial drug resistance, such as dhfr, dhps, mdr1, mrp1, and mrp-2, but not in the chloroquine resistance transporter ortholog (crt-o) gene. Moreover, P. vivax in the Americas is much less geographically substructured than local P. falciparum populations, with relatively little between-population genome-wide differentiation (pairwise FST values ranging between 0.025 and 0.092). Finally, P. vivax populations show a rapid decline in linkage disequilibrium with increasing distance between pairs of polymorphic sites, consistent with very frequent outcrossing. We hypothesize that the high diversity of present-day P. vivax lineages in the Americas originated from successive migratory waves and subsequent admixture between parasite lineages from geographically diverse sites. Further genome-wide analyses are required to test the demographic scenario suggested by our data.</p>
</abstract>
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<org type="consortium">We thank all sample donors for their participation in this study; Kézia K. G. Scopel for help in field work; Danielle S. Menchaca Vega for laboratory support; and Daniel E. Neafsey for a critical reading of the manuscript. This publication uses sequence data generated by the Wellcome Trust Sanger Institute (Hinxton, UK) as part of the MalariaGEN P. vivax Genome Variation project and by the Broad Institute of MIT and Harvard (Cambridge, MA), as part of the International Centers of Excellence for Malaria Research (ICEMR) program of the National Institute of Allergy and Infectious Diseases (NIAID) of the National Institutes of Health (NIH), United States.</org>
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