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J Biol Chem, Vol. 273, Issue 29, 18130-18138, July 17, 1998
From the Immunology Research Institute, Ghen Corporation, 839-1 Sano, Gifu City 501-11, Japan
A simple, reproducible and high yield method of
Helicobacter pylori urease enzyme purification was
developed using a heparinoid (Cellufine sulfate) affinity gel. The
purification method involved two sequential steps using the same gel
that takes advantage of the differential affinity of urease to the
heparinoid at two levels of hydrogen ion concentration.
SDS-polyacrylamide gel electrophoresis analysis of affinity-purified
urease revealed two major protein bands with about 62- and 30-kDa
molecular mass. When whole cell lysates of clinical and laboratory
strains of H. pylori were probed by Western blot,
anti-urease hyperimmune serum produced by affinity-purified urease in
rabbit recognized only the two bands corresponding to the urease A and
B subunits. To probe the molecular relevance of affinity gel adherence
to mucin adherence, the purified urease was derivatized with
N-hydroxysuccinimidobiotin and used in adherence assays.
Competitive inhibition tests revealed commonality of urease receptors
among gastric mucin, heparin, and heparinoid. Composite data on
adherence kinetics modulated by pH, salt, incubation time, and
concentration of urease or mucin were indicative of
conformation-dependent ligand-receptor interaction.
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