Characterisation of Campylobacter jejuni genes potentially involved in phosphonate degradation

doi:10.1186/1757-4749-1-13

Gut Pathogens

Volume 1

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Hartley LE
Kaakoush NO
Ford JL
Korolik V
Mendz GL

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Kaakoush NO
Ford JL
Korolik V
Mendz GL
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Characterisation of Campylobacter jejuni genes potentially involved in phosphonate degradation

Lauren E Hartley¹ , Nadeem O Kaakoush² , Justin L Ford² , Victoria Korolik¹ and George L Mendz²

¹Institute for Glycomics, Griffith University, Gold Coast, Australia

²School of Medicine, Sydney, The University of Notre Dame Australia, Darlinghurst NSW 2010, Australia

author email corresponding author email

Gut Pathogens 2009, 1:13doi:10.1186/1757-4749-1-13


Published:	25 June 2009

Abstract

Potential biological roles of the Campylobacter jejuni genes cj0641, cj0774c and cj1663 were investigated. The proteins encoded by these genes showed sequence similarities to the phosphonate utilisation PhnH, K and L gene products of Escherichia coli. The genes cj0641, cj0774c and cj1663 were amplified from the pathogenic C. jejuni strain 81116, sequenced, and cloned into pGEM-T Easy vectors. Recombinant plasmids were used to disrupt each one of the genes by inserting a kanamycin resistance (Km^R) cassette employing site-directed mutagenesis or inverse PCR. Campylobacter jejuni 81116 isogenic mutants were generated by integration of the mutated genes into the genome of the wild-type strain. The C. jejuni mutants grew on primary isolation plates, but they could not be purified by subsequent passages owing to cell death. The mutant C. jejuni strains survived and proliferated in co-cultures with wild-type bacteria or in media in which wild-type C. jejuni had been previously grown. PCR analyses of mixed wild-type/mutant cultures served to verify the presence of the mutated gene in the genome of a fraction of the total bacterial population. The data suggested that each mutation inactivated a gene essential for survival. Rates of phosphonate catabolism in lysates of E. coli strain DH5α were determined using proton nuclear magnetic resonance spectroscopy. Whole-cell lysates of the wild-type degraded phosphonoacetate, phenylphosphonate and aminomethylphosphonate. Significant differences in the rates of phosphonate degradation were observed between lysates of wild-type E. coli, and of bacteria transformed with each one of the vectors carrying one of the C. jejuni genes, suggesting that these genes were involved in phosphonate catabolism.