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MOLECULAR CHARACTERISATION AND DIAGNOSIS |
Institute of Veterinary, Animal and Biomedical Sciences, Massey University, Palmerston North and *Wakefield Gastroenterology Research Centre, Wakefield Hospital, Wellington, New Zealand
Corresponding author: Dr A. Murray.
Received 18 July 1999; revised version received 12 Nov. 1999; accepted 18 Nov. 1999.
Abstract
The use of alkaline phosphatase fusion methodology to identify Helicobacter pylori exported proteins enabled the identification of an open reading frame (ORF) encoding a highly immunogenic, previously uncharacterised exported protein. The predicted amino-acid sequence displays a typical N-terminal signal peptide and contains regions of C-terminal hydrophobicity consistent with a membrane-associated protein. Southern blot analysis revealed that the gene encoding the protein was absent in several Helicobacter spp. and a combination of PCR and sequence analysis of the amplified gene showed that it is highly conserved amongst isolates of H. pylori. To obtain pure recombinant protein, the gene encoding the protein was cloned and expressed as a ß-galactosidase (ß-gal) fusion in Escherichia coli and the protein was purified by affinity chromatography and proteolytic cleavage of the ß-gal portion. The purified protein, which has an apparent mol. wt of 18 kDa, was recognised by antibody present in 71% of sera from patients infected with H. pylori, but in only 16% of sera from patients with unrelated or no gastrointestinal disease, by Western blot assays. These results indicate that the 18-kDa protein from H. pylori is immunogenic and is expressed in vivo.
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