Substrate specificities of pepstatin-insensitive carboxyl proteinases from gram-negative bacteria

Pseudomonas carboxyl proteinase (PCP), isolated from Pseudomonas sp. 101, and Xanthomonas carboxyl proteinase (XCP), isolated from Xanthomonas sp. T-22, are the first and second examples of unique carboxyl proteinases [EC 3.4.23.33] which are insensitive to aspartic proteinase inhibitors, such as pepstatin, diazoacetyl- DL-norleucine methylester, and 1,2-epoxy-3(p-nitrophenoxy)propane. The substrate specificities of PCP and XCP were studied using a series of synthetic chromogenic peptide substrates with the general structure, P5-P4-P3-P2-Phe-Nph-P2'-P3' (P5, P4, P3, P2, P2', P3': a variety of amino acids, Nph is p-nitro-L-phenylalanine, and the Phe-Nph bond is cleaved). PCP and XCP were shown to hydrolyze a synthetic substrate, Lys-Pro-Ala-Leu-Phe-Nph-Arg-Leu, most effectively among 28 substrates. The kinetic parameters of this peptide for PCP were K-m=6.3 mu M, k(cat)=51.4(s-1), and k(cat)/K-m=8.16 mu M(-1). s(-1). The kinetic parameters for XCP were K-m=3.6 mu M, k(cat)=52.2(s-1), and k(cat)/K-m=14.5 mu M(-1). s(-1). PCP showed a stricter substrate specificity than XCP. That is, the specificity constant (k(cat)/K-m) of each substrate for PCP was in general < 0.5 mu M(-1). s(-1), but was drastically improved by the replacement of Lys by Leu at the P2 position. On the other hand, XCP showed a less stringent substrate specificity, with most of the peptides exhibiting reasonable k(cat)/K-m values (>1.0 mu M(-1). s(-1)). Thus it was found that the substrate specificities of PCP and XCP differ considerably, in spite of the high similarity in their primary structures. In addition, tyrostatin was found to be a competitive inhibitor for XCP, with a K-i value of 2.1 nM, as well as for PCP (K-i=2.6 nM).