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2Institute of Cytology, Russian Academy of Sciences, Tikhoretskaya nab. 4, St. Petersburg, 194064 Russia; fax: (812) 247-0341
3Department of Molecular Biology, Odense University, DK-5230, Odense M, Denmark
* To whom correspondence should be addressed.
Received March 17, 2000; Revision received August 22, 2000
A comparative study of substrate specificity of bovine duodenal proteinases--chymotrypsin-like duodenase (ChlD) and dual-specificity duodenase (dsD)--was carried out using oligopeptide substrates (human proinsulin, glucagon, melittin, angiotensinogen fragment 1-14). ChlD displayed mainly chymotrypsin-like properties towards these substrates, hydrolyzing peptide bonds carboxy-terminally to bulky aliphatic or aromatic residues. In melittin, ChlD additionally cleaved peptide bonds after Thr and Ser residues. Dual-specificity duodenase (dsD) significantly restricted its specificity to only trypsin-like or only chymotrypsin-like or displayed full activity, combining both specificities, depending on substrate. Both ChlD and dsD efficiently hydrolyzed a single peptide bond (Phe8-His9) in angiotensinogen fragment 1-14. The kinetic parameters of angiotensinogen fragment 1-14 cleavage by ChlD and dsD were determined (kcat/Km = 80,500 M-1·sec-1 for ChlD and 103,000 M-1·sec-1 for dsD).
KEY WORDS: duodenases, serine proteases, substrate specificity
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