Cloning and expression of a high-molecular-mass major antigen of Helicobacter pylori: evidence of linkage to cytotoxin production.

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Infect Immun. 1993 May; 61(5): 1799-1809

Cloning and expression of a high-molecular-mass major antigen of Helicobacter pylori: evidence of linkage to cytotoxin production.

M K Tummuru, T L Cover and M J Blaser

Department of Medicine, Vanderbilt Unviersity School of Medicine, Nashville, Tennessee 37232-2605.

ABSTRACT

A high-molecular-mass (120- to 128-kDa) Helicobacter pyloriantigen has been associated with peptic ulcer disease. We createda bank of 40,000 random chromosomal fragments of H. pylori 84-183by using lambda ZapII. Screening of this bank in Escherichiacoli XL1-Blue with absorbed serum from an H. pylori-infectedperson permitted the isolation and purification of a clone witha 3.5-kb insert. Subcloning of this insert (pMC3) permittedthe expression of a recombinant H. pylori protein that had amass of approximately 96 kDa and that was recognized by thehuman serum. Sera that were obtained from H. pylori-infectedpersons and that recognized the native 120- to 128-kDa H. pyloriantigen recognized the recombinant 96-kDa pMC3 protein to asignificantly greater extent than did sera that did not recognizethe native H. pylori antigen. All 19 H. pylori isolates producingthe 120- to 128-kDa antigen hybridized with pMC3; none of 13nonproducers did so (P < 0.001). Because all 15 isolatesproducing the vacuolating cytotoxin hybridized with pMC3, wecalled the gene cagA (cytotoxin-associated gene). Sequence analysisof pMC3 identified an open reading frame of 859 amino acids,without a termination codon. Parallel screening of a lambdagt11 library with human serum revealed positive plaques withidentical 0.6-kb inserts and sequences matching the sequenceof the downstream region of pMC3. To clone the full-length gene,we used the 0.6-kb fragment as a probe and isolated a clonewith a 2.7-kb insert from the lambda ZapII genomic library.Nucleotide sequencing of this insert (pYB 2) revealed a 785-bpsequence that overlapped the downstream region of pMC3. Translationof the complete nucleotide sequence of cagA revealed an openreading frame of 1,181 amino acids yielding a protein of 131,517daltons. There was no significant homology with any previouslyreported protein sequence. These findings indicate the cloningand characterization of a high-molecular-mass H. pylori antigenpotentially associated with virulence and with cytotoxin production.

Infect Immun. 1993 May; 61(5): 1799-1809

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