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Characterization of Metabolically Quiescent Leishmania Parasites in Murine Lesions Using Heavy Water Labeling

Information on the growth rate and metabolism of microbial pathogens that cause long-term chronic infections is limited, reflecting the absence of suitable tools for measuring these parameters in vivo. Here, we have measured the replication and physiological state of Leishmania mexicana parasites in...

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Autores principales: Kloehn, Joachim, Saunders, Eleanor C., O’Callaghan, Sean, Dagley, Michael J., McConville, Malcolm J.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2015
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4340956/
https://www.ncbi.nlm.nih.gov/pubmed/25714830
http://dx.doi.org/10.1371/journal.ppat.1004683
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author Kloehn, Joachim
Saunders, Eleanor C.
O’Callaghan, Sean
Dagley, Michael J.
McConville, Malcolm J.
author_facet Kloehn, Joachim
Saunders, Eleanor C.
O’Callaghan, Sean
Dagley, Michael J.
McConville, Malcolm J.
author_sort Kloehn, Joachim
collection PubMed
description Information on the growth rate and metabolism of microbial pathogens that cause long-term chronic infections is limited, reflecting the absence of suitable tools for measuring these parameters in vivo. Here, we have measured the replication and physiological state of Leishmania mexicana parasites in murine inflammatory lesions using (2)H(2)O labeling. Infected BALB/c mice were labeled with (2)H(2)O for up to 4 months, and the turnover of parasite DNA, RNA, protein and membrane lipids estimated from the rate of deuterium enrichment in constituent pentose sugars, amino acids, and fatty acids, respectively. We show that the replication rate of parasite stages in these tissues is very slow (doubling time of ~12 days), but remarkably constant throughout lesion development. Lesion parasites also exhibit markedly lower rates of RNA synthesis, protein turnover and membrane lipid synthesis than parasite stages isolated from ex vivo infected macrophages or cultured in vitro, suggesting that formation of lesions induces parasites to enter a semi-quiescent physiological state. Significantly, the determined parasite growth rate accounts for the overall increase in parasite burden indicating that parasite death and turnover of infected host cells in these lesions is minimal. We propose that the Leishmania response to lesion formation is an important adaptive strategy that minimizes macrophage activation, providing a permissive environment that supports progressive expansion of parasite burden. This labeling approach can be used to measure the dynamics of other host-microbe interactions in situ.
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spelling pubmed-43409562015-03-04 Characterization of Metabolically Quiescent Leishmania Parasites in Murine Lesions Using Heavy Water Labeling Kloehn, Joachim Saunders, Eleanor C. O’Callaghan, Sean Dagley, Michael J. McConville, Malcolm J. PLoS Pathog Research Article Information on the growth rate and metabolism of microbial pathogens that cause long-term chronic infections is limited, reflecting the absence of suitable tools for measuring these parameters in vivo. Here, we have measured the replication and physiological state of Leishmania mexicana parasites in murine inflammatory lesions using (2)H(2)O labeling. Infected BALB/c mice were labeled with (2)H(2)O for up to 4 months, and the turnover of parasite DNA, RNA, protein and membrane lipids estimated from the rate of deuterium enrichment in constituent pentose sugars, amino acids, and fatty acids, respectively. We show that the replication rate of parasite stages in these tissues is very slow (doubling time of ~12 days), but remarkably constant throughout lesion development. Lesion parasites also exhibit markedly lower rates of RNA synthesis, protein turnover and membrane lipid synthesis than parasite stages isolated from ex vivo infected macrophages or cultured in vitro, suggesting that formation of lesions induces parasites to enter a semi-quiescent physiological state. Significantly, the determined parasite growth rate accounts for the overall increase in parasite burden indicating that parasite death and turnover of infected host cells in these lesions is minimal. We propose that the Leishmania response to lesion formation is an important adaptive strategy that minimizes macrophage activation, providing a permissive environment that supports progressive expansion of parasite burden. This labeling approach can be used to measure the dynamics of other host-microbe interactions in situ. Public Library of Science 2015-02-25 /pmc/articles/PMC4340956/ /pubmed/25714830 http://dx.doi.org/10.1371/journal.ppat.1004683 Text en © 2015 Kloehn et al http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Kloehn, Joachim
Saunders, Eleanor C.
O’Callaghan, Sean
Dagley, Michael J.
McConville, Malcolm J.
Characterization of Metabolically Quiescent Leishmania Parasites in Murine Lesions Using Heavy Water Labeling
title Characterization of Metabolically Quiescent Leishmania Parasites in Murine Lesions Using Heavy Water Labeling
title_full Characterization of Metabolically Quiescent Leishmania Parasites in Murine Lesions Using Heavy Water Labeling
title_fullStr Characterization of Metabolically Quiescent Leishmania Parasites in Murine Lesions Using Heavy Water Labeling
title_full_unstemmed Characterization of Metabolically Quiescent Leishmania Parasites in Murine Lesions Using Heavy Water Labeling
title_short Characterization of Metabolically Quiescent Leishmania Parasites in Murine Lesions Using Heavy Water Labeling
title_sort characterization of metabolically quiescent leishmania parasites in murine lesions using heavy water labeling
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4340956/
https://www.ncbi.nlm.nih.gov/pubmed/25714830
http://dx.doi.org/10.1371/journal.ppat.1004683
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