2012
DOI: 10.1002/jobm.201100466
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Carbohydrate binding and gene expression by in vitro and in vivo propagated Campylobacter jejuni after Immunomagnetic Separation

Abstract: Campylobacter jejuni is an important human food‐borne intestinal pathogen, however relatively little is known about its mechanisms of pathogenesis or pathogen‐host interactions. To monitor changes in gene expression and glycan binding of C. jejuni within a common avian host, an immunomagnetic separation technique (IMS) was utilised to directly isolate infecting C. jejuni 81116 from a chicken host. An average of 105 cells/g was re‐isolated from chicken caecal samples by IMS technique. The in vivo passaged strai… Show more

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Cited by 7 publications
(10 citation statements)
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“…The cdtA gene expression by ccaA isogenic mutant cells isolated from chickens was up-regulated as was the expression of cdtB in the mutant cells isolated from the mouse. This was in agreement with a previous study showing that in chickens the cdtA/C subunits could be up-regulated 34 . Therefore, while it may be a contributing pathogenicity factor, it is possible to speculate that they are unlikely to account for the observed pathology.…”
Section: Discussionsupporting
confidence: 94%
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“…The cdtA gene expression by ccaA isogenic mutant cells isolated from chickens was up-regulated as was the expression of cdtB in the mutant cells isolated from the mouse. This was in agreement with a previous study showing that in chickens the cdtA/C subunits could be up-regulated 34 . Therefore, while it may be a contributing pathogenicity factor, it is possible to speculate that they are unlikely to account for the observed pathology.…”
Section: Discussionsupporting
confidence: 94%
“…jejuni 11168-GS and 11168-O isolated from the caecal content of chicks at day 5p.i. by IMS 34 . The binding specificities of 11168-O and 11168-O ΔccaA::cat were compared and only statistically significant differences (p < 0.05) are described in Table 1 .…”
Section: Resultsmentioning
confidence: 99%
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“…Cultures for RNA analysis were grown under the following conditions: Cultures that mimic environmental conditions were performed as previously described [ 12 ]. Cultures grown for laboratory conditions were grown at either 37 or 42°C as described in Day et al (2009) and processed to minimise effects on RNA expression as per King et al (2012) [ 12 , 21 ].…”
Section: Methodsmentioning
confidence: 99%
“…Moreover, more and more proteins have been sequenced without knowledge of their function(s) due to increasingly inexpensive sequencing techniques. Although there is one high‐throughput technique (glycan arrays) for detecting novel CBPs and investigating their binding specificity, it is challenging to construct a sizeable, diverse glycan array because of difficulty in synthesis and isolation of carbohydrates. Here, we focus on a complementary approach: prediction of CBPs and their binding amino acid residues by computational techniques.…”
Section: Introductionmentioning
confidence: 99%