Predicting proteinase specificities from free energy calculations
Autor: | Seble Merid Mekonnen, Arne O. Smalås, Bjørn Olav Brandsdal, Magne Olufsen |
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Rok vydání: | 2006 |
Předmět: |
Models
Molecular Serine Proteinase Inhibitors Stereochemistry Protonation Subtilase Structure-Activity Relationship X-Ray Diffraction Endopeptidases Materials Chemistry Computer Simulation Subtilisins Homology modeling Physical and Theoretical Chemistry Spectroscopy chemistry.chemical_classification Binding Sites biology Serine Endopeptidases Subtilisin Proteins Interaction energy Proteinase K Computer Graphics and Computer-Aided Design Amino acid Crystallography chemistry biology.protein Thermodynamics Endopeptidase K Thermitase Algorithms Protein Binding |
Zdroj: | Journal of Molecular Graphics and Modelling. 25:176-185 |
ISSN: | 1093-3263 |
Popis: | The role of the primary binding residue (P1) in complexes between three different subtilases (subtilisin Carlsberg, thermitase and proteinase K) and their canonical protein inhibitor eglin c have been studied by free energy calculations. Based on the crystal structures of eglin c in complex with subtilisin Carlsberg and thermitase, and a homology model of the eglin c–proteinase K complex, a total of 57 mutants have been constructed and docked into their host proteins. The binding free energy was then calculated using molecular dynamics (MD) simulations combined with the linear interaction energy (LIE) method for all complexes differing only in the nature of the amino acid at the P1 position. LIE calculations for 19 different complexes for each subtilase were thus carried out excluding proline. The effects of substitutions at the P1 position on the binding free energies are found to be very large, and positively charged residues (Arg, Lys and His) are particularly deleterious for all three enzymes. The charged variants of the acidic side chains are found to bind more favorably as compared to their protonated states in all three subtilases. Furthermore, hydrophobic amino acids are accommodated most favorably at the S1-site in all three enzymes. Comparison of the three series of binding free energies shows only minor differences in the 19 computed relative binding free energies among these subtilases. This is further reflected in the correlation coefficient between the 23 relative binding free energies obtained, including the possible protonation states of ionizable side chains, but excluding the P1 Pro, for subtilisin Carlsberg versus thermitase (0.95), subtilisin versus proteinase K (0.94) and thermitase versus proteinase K (0.96). |
Databáze: | OpenAIRE |
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