The early response of Atlantic salmon (Salmo salar) macrophages exposed in vitro to Aeromonas salmonicida cultured in broth and in fish

Aeromonas salmonicida is a fish pathogen that causes furunculosis. Virulent strains of this bacterium are able to infect salmonid macrophages and survive within them, although mechanisms favouring intracellular survival are not completely understood. It is known that A. salmonicida cultured in vivo...

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Bibliographic Details
Main Authors: Ewart, K. Vanya, Williams, Jason, Richards, Robert C., Gallant, Jeffrey W., Melville, Krista, Douglas, Susan E.
Format: Article in Journal/Newspaper
Language:English
Published: Elsevier 2007
Subjects:
inflammation
acute phase response
fish
microarray
qPCR
Atlantic salmon
Salmo salar
Online Access:https://nrc-publications.canada.ca/eng/view/object/?id=f29fc1f2-3e48-4dfa-8001-12d683a20318
https://nrc-publications.canada.ca/fra/voir/objet/?id=f29fc1f2-3e48-4dfa-8001-12d683a20318
Description
Summary:Aeromonas salmonicida is a fish pathogen that causes furunculosis. Virulent strains of this bacterium are able to infect salmonid macrophages and survive within them, although mechanisms favouring intracellular survival are not completely understood. It is known that A. salmonicida cultured in vivo in the peritoneal cavity of the host undergoes changes in gene expression and surface architecture compared with cultures grown in vitro in broth. Therefore, in this study, the early macrophage responses to A. salmonicida grown in vivo and in vitro were compared. Macrophage-enriched cell preparations from head kidney of Atlantic salmon (Salmo salar) were infected in vitro in 96-well microtitre dishes and changes in gene expression during the infection process were monitored using a custom Atlantic salmon cDNA microarray. A. salmonicida cultures grown in tryptic soy broth and in peritoneal implants were used to infect the macrophages. The macrophages were harvested at 0.5, 1.0 and 2.0 h after addition of the bacteria to the medium. Significant changes in gene expression were evident by microarray analysis at 2.0 h post-infection in macrophages infected with broth-grown and implant-grown bacteria; however, qPCR analysis revealed earlier up-regulation of JunB and TNF-α in macrophages exposed to the implant-grown bacteria. Up-regulation of those genes and others is consistent with the effects of extracellular products of aeromonad bacteria on macrophages and also suggests initiation of the innate immune response. Peer reviewed: Yes NRC publication: Yes

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