Affiliation:
1. Cooperative Research Centre for Diagnostics, Institute of Health and Biomedical Innovation, Queensland University of Technology, Brisbane, Australia
Abstract
ABSTRACT
The aim of this investigation was to exploit the vast comparative data generated by comparative genome hybridization (CGH) studies of
Campylobacter jejuni
in developing a genotyping method. We examined genes in
C. jejuni
that exhibit binary status (present or absent between strains) within known plasticity regions, in order to identify a minimal subset of gene targets that provide high-resolution genetic fingerprints. Using CGH data from three studies as input, binary gene sets were identified with “Minimum SNPs” software. “Minimum SNPs” selects for the minimum number of targets required to obtain a predefined resolution, based on Simpson's index of diversity (
D
). After implementation of stringent criteria for gene presence/absence, eight binary genes were found that provided 100% resolution (
D
= 1) of 20
C. jejuni
strains. A real-time PCR assay was developed and tested on 181
C. jejuni
and
Campylobacter coli
isolates, a subset of which have previously been characterized by multilocus sequence typing,
flaA
short variable region sequencing, and pulsed-field gel electrophoresis. In addition to the binary gene real-time PCR assay, we refined the seven-member single nucleotide polymorphism (SNP) real-time PCR assay previously described for
C. jejuni
and
C. coli
. By normalizing the SNP assay with the respective
C. jejuni
and
C. coli
ubiquitous genes,
mapA
and
ceuE
, the polymorphisms at each SNP could be determined without separate reactions for every polymorphism. We have developed and refined a rapid, highly discriminatory genotyping method for
C. jejuni
and
C. coli
that uses generic technology and is amenable to high-throughput analyses.
Publisher
American Society for Microbiology
Subject
Ecology,Applied Microbiology and Biotechnology,Food Science,Biotechnology
Cited by
29 articles.
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