Affiliation:
1. Department of Microbiology, University College Cork, Cork, Ireland
2. Alimentary Pharmabiotic Centre, Cork, Ireland
3. Teagasc, Moorepark Food Research Centre, Fermoy, County Cork, Ireland
Abstract
ABSTRACT
Due to the severity of the food-borne infection listeriosis, strict legislation governs the detectable and permissible limits at which
Listeria monocytogenes
is permitted in foods. These requirements, coupled with the ubiquitous nature of
L. monocytogenes
strains and the potential for epidemic outbreaks, mean that the pathogen can devastate affected sectors of the food industry. Although almost all
L. monocytogenes
strains have the potential to cause listeriosis, those implicated in the vast majority of epidemics belong to a subset of strains belonging to evolutionary lineage I. It has been established that a significant proportion of these strains, including those implicated in the majority of outbreaks, produce an additional hemolysin, designated listeriolysin S (LLS), which may be responsible for the enhanced virulence of these strains. In order to ultimately establish this definitively, it is important to first be able to rapidly discriminate between LLS-positive and -negative strains. Here, after essential genes within the LLS-encoding cluster,
Listeria
pathogenicity island 3, were identified by deletion mutagenesis, a real-time PCR assay which targets one such gene,
llsX
, was developed as a means of identifying LLS-positive
L. monocytogenes
. The specificity of the assay was validated against a panel of 40
L. monocytogenes
strains (20 of which were LLS positive) and 25 strains representative of other
Listeria
species. Furthermore, 1 CFU of an LLS-positive strain per 25 g/ml of spiked foods was detected in less than 30 h when the assay was coupled with culture enrichment. The detection limit of this assay was 10 genome equivalents.
Publisher
American Society for Microbiology
Subject
Ecology,Applied Microbiology and Biotechnology,Food Science,Biotechnology
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