Protein & Peptide Letters

Author(s): Anna G. Mikhailova, Viktoria V. Likhareva, Niels Teich and Lev D. Rumsh

DOI: 10.2174/092986607780090793

The Ways of Realization of High Specificity and Efficiency of Enteropeptidase

Page: [227 - 232] Pages: 6

  • * (Excluding Mailing and Handling)

Abstract

Comparative substrate analysis of full-length bovine enteropeptidase and trypsin, bovine and human enteropeptidase light chains was performed using model N-terminal dodecapeptides corresponding to wild-type human trypsinogen and pancreatitis-associated mutant trypsinogens K23R and D22G. The substitution of Lys residue by Arg at P1 leads to 2- fold increase in the efficiency of enteropeptidase hydrolysis; the absence of the negatively charged residue at P2 reduces the efficiency of such hydrolysis by two orders of magnitude. The difference in efficiency of peptide chain hydrolysis after Lys/Arg residues by enteropeptidase compared to trypsin is equal to the difference in hydrolysis by serine proteases of different primary specificity of their specific substrates.

Keywords: Enteropeptidase, trypsin, trypsinogen, selectivity, substrate analysis