Premium
On the calculation of binding free energies using continuum methods: Application to MHC class I protein‐peptide interactions
Author(s) -
Froloff Nicolas,
Windemuth Andreas,
Honig Barry
Publication year - 1997
Publication title -
protein science
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 3.353
H-Index - 175
eISSN - 1469-896X
pISSN - 0961-8368
DOI - 10.1002/pro.5560060617
Subject(s) - chemistry , peptide , binding energy , solvation , electrostatics , gibbs free energy , ligand (biochemistry) , affinities , poisson–boltzmann equation , thermodynamics , crystallography , computational chemistry , stereochemistry , solvent , physics , biochemistry , receptor , ion , atomic physics , organic chemistry
This paper describes a methodology to calculate the binding free energy (Δ G ) of a protein‐ligand complex using a continuum model of the solvent. A formal thermodynamic cycle is used to decompose the binding free energy into electrostatic and non‐electrostatic contributions. In this cycle, the reactants are discharged in water, associated as purely nonpolar entities, and the final complex is then recharged. The total electrostatic free energies of the protein, the ligand, and the complex in water are calculated with the finite difference Poisson‐Boltzmann (FDPB) method. The nonpolar (hydrophobic) binding free energy is calculated using a free energy‐surface area relationship, with a single alkane/water surface tension coefficient (γ aw ). The loss in backbone and side‐chain configurational entropy upon binding is estimated and added to the electrostatic and the nonpolar components of Δ G. The methodology is applied to the binding of the murine MHC class I protein H‐2K b with three distinct peptides, and to the human MHC class I protein HLA‐A2 in complex with five different peptides. Despite significant differences in the amino acid sequences of the different peptides, the experimental binding free energy differences (ΔΔ G exp ) are quite small (<0.3 and <2.7 kcal/mol for the H‐2K b and HLA‐A2 complexes, respectively). For each protein, the calculations are successful in reproducing a fairly small range of values for ΔΔ G calc (<4.4 and <5.2 kcal/mol, respectively) although the relative peptide binding affinities of H‐2K b and HLA‐A2 are not reproduced. For all protein‐peptide complexes that were treated, it was found that electrostatic interactions oppose binding whereas nonpolar interactions drive complex formation. The two types of interactions appear to be correlated in that larger nonpolar contributions to binding are generally opposed by increased electrostatic contributions favoring dissociation. The factors that drive the binding of peptides to MHC proteins are discussed in light of our results.