Affiliation:
1. School of Animal and Microbial Sciences, University of Reading, Reading, England,1 and
2. SOAEFD Marine Laboratory, Aberdeen, Scotland2
Abstract
ABSTRACT
The importance of the two major extracellular enzymes of
Aeromonas salmonicida
, glycerophospholipid:cholesterol acyltransferase (GCAT) and a serine protease (AspA), to the pathology and mortality of salmonid fish with furunculosis had been indicated in toxicity studies. In this study, the genes encoding GCAT (
satA
) and AspA (
aspA
) have been cloned and mutagenized by marker replacement of internal deletions, and the constructs have been used for the creation of isogenic
satA
and
aspA
mutants of
A. salmonicida
. A pSUP202 derivative (pSUP202sac) carrying the
sacRB
genes was constructed to facilitate the selection of mutants. The requirement of serine protease for processing of pro-GCAT was demonstrated. Processing involved the removal of a short internal fragment. Surprisingly, pathogenicity trials revealed no major decrease in virulence of the
A. salmonicida ΔsatA
::
kan
or
A. salmonicida ΔaspA
::
kan
mutants compared to the wild-type parent strains when Atlantic salmon (
Salmo salar
L.) were challenged by intraperitoneal injection. Moreover, using a cohabitation model, which more closely mimics the natural disease, there was also no significant decrease in the relative cumulative mortality following infection with either of the deletion mutants compared to the parent strain. Thus, although these two toxins may confer some competitive advantage to
A. salmonicida
, neither toxin is essential for the very high virulence of
A. salmonicida
in Atlantic salmon. This first report of defined deletion mutations within any proposed extracellular virulence factor of
A. salmonicida
raises crucial questions about the pathogenesis of this important fish pathogen.
Publisher
American Society for Microbiology
Subject
Infectious Diseases,Immunology,Microbiology,Parasitology
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