Abstract
Understanding the mechanisms of protein–protein interaction is a fundamental problem with many practical applications. The fact that different proteins can bind similar partners suggests that convergently evolved binding interfaces are reused in different complexes. A set of protein complexes composed of non-homologous domains interacting with homologous partners at equivalent binding sites was collected in 2006, offering an opportunity to investigate this point. We considered 433 pairs of protein–protein complexes from the ABAC database (AB and AC binary protein complexes sharing a homologous partner A) and analyzed the extent of physico-chemical similarity at the atomic and residue level at the protein–protein interface. Homologous partners of the complexes were superimposed using Multiprot, and similar atoms at the interface were quantified using a five class grouping scheme and a distance cut-off. We found that the number of interfacial atoms with similar properties is systematically lower in the non-homologous proteins than in the homologous ones. We assessed the significance of the similarity by bootstrapping the atomic properties at the interfaces. We found that the similarity of binding sites is very significant between homologous proteins, as expected, but generally insignificant between the non-homologous proteins that bind to homologous partners. Furthermore, evolutionarily conserved residues are not colocalized within the binding sites of non-homologous proteins. We could only identify a limited number of cases of structural mimicry at the interface, suggesting that this property is less generic than previously thought. Our results support the hypothesis that different proteins can interact with similar partners using alternate strategies, but do not support convergent evolution.
Highlights
Protein-protein interaction is the basis of numerous biological functions, such as immune response, supra-molecular assembly, enzymatic reactions, and many more
Among the properties playing a role in this process, hydrophobicity was suggested as a major factor by Chothia and Janin in their pioneering work [3]
Our results suggest that different proteins that bind the same protein do not imitate binding sites, but probably target specific locations or residues at the binding site
Summary
Protein-protein interaction is the basis of numerous biological functions, such as immune response, supra-molecular assembly, enzymatic reactions, and many more. The collection of all protein-protein interactions, the interactome, is of great importance for drug discovery [1]. Given their variety and often transient nature, the number of protein-protein complexes for which crystallographic structures are available is very limited compared to the number of individual protein structures in the Protein Data Bank [2]. Even with this limited amount of data, the observation of available complexes has helped to decipher some rules for protein-protein interactions. Different types of complexes (e.g. homo- or hetero-dimers, transient or permanent) display different properties [8,12,13]
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