Serveur d'exploration Chloroquine

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Adaptive evolution of malaria parasites in French Guiana: Reversal of chloroquine resistance by acquisition of a mutation in pfcrt.

Identifieur interne : 000010 ( Hal/Curation ); précédent : 000009; suivant : 000011

Adaptive evolution of malaria parasites in French Guiana: Reversal of chloroquine resistance by acquisition of a mutation in pfcrt.

Auteurs : Stéphane Pelleau ; Eli L. Moss [États-Unis] ; Satish K. Dhingra [États-Unis] ; Béatrice Volney ; Jessica Casteras ; Stanislaw J. Gabryszewski [États-Unis] ; Sarah K. Volkman [États-Unis] ; Dyann F. Wirth [États-Unis] ; Eric Legrand ; David A. Fidock [États-Unis] ; Daniel E. Neafsey [États-Unis] ; Lise Musset

Source :

RBID : Hal:pasteur-01229321

English descriptors

Abstract

In regions with high malaria endemicity, the withdrawal of chloroquine (CQ) as first-line treatment of Plasmodium falciparum infections has typically led to the restoration of CQ susceptibility through the reexpansion of the wild-type (WT) allele K76 of the chloroquine resistance transporter gene (pfcrt) at the expense of less fit mutant alleles carrying the CQ resistance (CQR) marker K76T. In low-transmission settings, such as South America, drug resistance mutations can attain 100% prevalence, thereby precluding the return of WT parasites after the complete removal of drug pressure. In French Guiana, despite the fixation of the K76T allele, the prevalence of CQR isolates progressively dropped from >90% to <30% during 17 y after CQ withdrawal in 1995. Using a genome-wide association study with CQ-sensitive (CQS) and CQR isolates, we have identified a single mutation in pfcrt encoding a C350R substitution that is associated with the restoration of CQ susceptibility. Genome editing of the CQR reference strain 7G8 to incorporate PfCRT C350R caused a complete loss of CQR. A retrospective molecular survey on 580 isolates collected from 1997 to 2012 identified all C350R mutant parasites as being CQS. This mutation emerged in 2002 and rapidly spread throughout the P. falciparum population. The C350R allele is also associated with a significant decrease in piperaquine susceptibility in vitro, suggesting that piperaquine pressure in addition to potential fitness costs associated with the 7G8-type CQR pfcrt allele may have selected for this mutation. These findings have important implications for understanding the evolutionary dynamics of antimalarial drug resistance.


Url:
DOI: 10.1073/pnas.1507142112

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Hal:pasteur-01229321

Curation

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Stéphane Pelleau
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Béatrice Volney
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Jessica Casteras
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Eric Legrand
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<title xml:lang="en">Adaptive evolution of malaria parasites in French Guiana: Reversal of chloroquine resistance by acquisition of a mutation in pfcrt.</title>
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<title level="j">Proceedings of the National Academy of Sciences of the United States of America </title>
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<p>In regions with high malaria endemicity, the withdrawal of chloroquine (CQ) as first-line treatment of Plasmodium falciparum infections has typically led to the restoration of CQ susceptibility through the reexpansion of the wild-type (WT) allele K76 of the chloroquine resistance transporter gene (pfcrt) at the expense of less fit mutant alleles carrying the CQ resistance (CQR) marker K76T. In low-transmission settings, such as South America, drug resistance mutations can attain 100% prevalence, thereby precluding the return of WT parasites after the complete removal of drug pressure. In French Guiana, despite the fixation of the K76T allele, the prevalence of CQR isolates progressively dropped from >90% to <30% during 17 y after CQ withdrawal in 1995. Using a genome-wide association study with CQ-sensitive (CQS) and CQR isolates, we have identified a single mutation in pfcrt encoding a C350R substitution that is associated with the restoration of CQ susceptibility. Genome editing of the CQR reference strain 7G8 to incorporate PfCRT C350R caused a complete loss of CQR. A retrospective molecular survey on 580 isolates collected from 1997 to 2012 identified all C350R mutant parasites as being CQS. This mutation emerged in 2002 and rapidly spread throughout the P. falciparum population. The C350R allele is also associated with a significant decrease in piperaquine susceptibility in vitro, suggesting that piperaquine pressure in addition to potential fitness costs associated with the 7G8-type CQR pfcrt allele may have selected for this mutation. These findings have important implications for understanding the evolutionary dynamics of antimalarial drug resistance.</p>
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<title xml:lang="en">Adaptive evolution of malaria parasites in French Guiana: Reversal of chloroquine resistance by acquisition of a mutation in pfcrt.</title>
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<forename type="first">Stéphane</forename>
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<funder>This work was supported by European Commission Grant REGPOT-CT-2011-285837-430 STRonGer (to S.P.), AgenceNationale de la Recherche Investissements d’Avenir Grant ANR-10-LABX-25-01(to S.P. and L.M.), NIH Grants R01AI50234 (to D.A.F.) and R01AI109023 (to D.A.F.),and the Institut de Veille Sanitaire. Sequencing was supported, in part, byNational Institute of Allergy and Infectious Diseases, NIH, Department ofHealth and Human Services Contract HHSN272200900018C.</funder>
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<note type="commentary">Comment in : Fusion of field studies and the laboratory solves a puzzle in antimalarial resistance. [Proc Natl Acad Sci U S A. 2015]</note>
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<idno type="halJournalId" status="VALID">7969</idno>
<idno type="issn">0027-8424</idno>
<idno type="eissn">1091-6490</idno>
<title level="j">Proceedings of the National Academy of Sciences of the United States of America </title>
<imprint>
<publisher>National Academy of Sciences</publisher>
<biblScope unit="volume">112</biblScope>
<biblScope unit="issue">37</biblScope>
<biblScope unit="pp">11672-11677</biblScope>
<date type="datePub">2015-09-15</date>
<date type="dateEpub">2015-08-10</date>
</imprint>
</monogr>
<idno type="doi">10.1073/pnas.1507142112</idno>
<idno type="pubmed">26261345</idno>
<idno type="pubmedcentral">PMC4577156</idno>
</biblStruct>
</sourceDesc>
<profileDesc>
<langUsage>
<language ident="en">English</language>
</langUsage>
<textClass>
<keywords scheme="author">
<term xml:lang="en">Plasmodium falciparum</term>
<term xml:lang="en">PfCRT</term>
<term xml:lang="en">malaria</term>
<term xml:lang="en">evolution</term>
<term xml:lang="en">drug resistance</term>
</keywords>
<classCode scheme="mesh">Alleles</classCode>
<classCode scheme="mesh">Chloroquine/therapeutic use*</classCode>
<classCode scheme="mesh">Principal Component Analysis</classCode>
<classCode scheme="mesh">Protozoan Proteins/genetics*</classCode>
<classCode scheme="mesh">Drug Resistance/genetics*</classCode>
<classCode scheme="mesh">Quinolines/chemistry</classCode>
<classCode scheme="mesh">Retrospective Studies</classCode>
<classCode scheme="mesh">Evolution, Molecular*</classCode>
<classCode scheme="mesh">French Guiana</classCode>
<classCode scheme="mesh">Genetic Markers</classCode>
<classCode scheme="mesh">Genome</classCode>
<classCode scheme="mesh">Genotype</classCode>
<classCode scheme="mesh">Inhibitory Concentration 50</classCode>
<classCode scheme="mesh">Haplotypes</classCode>
<classCode scheme="mesh">Humans</classCode>
<classCode scheme="mesh">Malaria/drug therapy</classCode>
<classCode scheme="mesh">Membrane Transport Proteins/genetics*</classCode>
<classCode scheme="mesh">Mutation*</classCode>
<classCode scheme="mesh">Phenotype</classCode>
<classCode scheme="mesh">Plasmodium falciparum/drug effects</classCode>
<classCode scheme="mesh">Plasmodium falciparum/genetics*</classCode>
<classCode scheme="mesh">Prevalence</classCode>
<classCode scheme="halDomain" n="sdv">Life Sciences [q-bio]</classCode>
<classCode scheme="halDomain" n="sdv.mp.par">Life Sciences [q-bio]/Microbiology and Parasitology/Parasitology</classCode>
<classCode scheme="halDomain" n="sdv.spee">Life Sciences [q-bio]/Santé publique et épidémiologie</classCode>
<classCode scheme="halTypology" n="ART">Journal articles</classCode>
</textClass>
<abstract xml:lang="en">
<p>In regions with high malaria endemicity, the withdrawal of chloroquine (CQ) as first-line treatment of Plasmodium falciparum infections has typically led to the restoration of CQ susceptibility through the reexpansion of the wild-type (WT) allele K76 of the chloroquine resistance transporter gene (pfcrt) at the expense of less fit mutant alleles carrying the CQ resistance (CQR) marker K76T. In low-transmission settings, such as South America, drug resistance mutations can attain 100% prevalence, thereby precluding the return of WT parasites after the complete removal of drug pressure. In French Guiana, despite the fixation of the K76T allele, the prevalence of CQR isolates progressively dropped from >90% to <30% during 17 y after CQ withdrawal in 1995. Using a genome-wide association study with CQ-sensitive (CQS) and CQR isolates, we have identified a single mutation in pfcrt encoding a C350R substitution that is associated with the restoration of CQ susceptibility. Genome editing of the CQR reference strain 7G8 to incorporate PfCRT C350R caused a complete loss of CQR. A retrospective molecular survey on 580 isolates collected from 1997 to 2012 identified all C350R mutant parasites as being CQS. This mutation emerged in 2002 and rapidly spread throughout the P. falciparum population. The C350R allele is also associated with a significant decrease in piperaquine susceptibility in vitro, suggesting that piperaquine pressure in addition to potential fitness costs associated with the 7G8-type CQR pfcrt allele may have selected for this mutation. These findings have important implications for understanding the evolutionary dynamics of antimalarial drug resistance.</p>
</abstract>
</profileDesc>
</hal>
</record>

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