Binding to DPF-motif by the POB1 EH domain is responsible for POB1-Eps15 interaction

doi:10.1186/1471-2091-8-29

BMC Biochemistry

Volume 8

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Castagnoli L
Cesareni G

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Research article

Binding to DPF-motif by the POB1 EH domain is responsible for POB1-Eps15 interaction

Elena Santonico¹ , Simona Panni¹ , Mattia Falconi² , Luisa Castagnoli¹ and Gianni Cesareni¹

¹Department of Biology, University of Rome Tor Vergata, Rome, Italy

²Structural Bioinformatics and Computational Biochemistry, Department of Biology, University of Rome Tor Vergata, Rome, Italy

author email corresponding author email

BMC Biochemistry 2007, 8:29doi:10.1186/1471-2091-8-29


Published:	21 December 2007

Abstract

Background

Eps15 homology (EH) domains are protein interaction modules binding to peptides containing Asn-Pro-Phe (NPF) motifs and mediating critical events during endocytosis and signal transduction. The EH domain of POB1 associates with Eps15, a protein characterized by a striking string of DPF triplets, 15 in human and 13 in mouse Eps15, at the C-terminus and lacking the typical EH-binding NPF motif.

Results

By screening a multivalent nonapeptide phage display library we have demonstrated that the EH domain of POB1 has a different recognition specificity since it binds to both NPF and DPF motifs. The region of mouse Eps15 responsible for the interaction with the EH domain of POB1 maps within a 18 amino acid peptide (residues 623–640) that includes three DPF repeats. Finally, mutational analysis in the EH domain of POB1, revealed that several solvent exposed residues, while distal to the binding pocket, mediate specific recognition of binding partners through both hydrophobic and electrostatic contacts.

Conclusion

In the present study we have analysed the binding specificity of the POB1 EH domain. We show that it differs from other EH domains since it interacts with both NPF- and DPF-containing sequences. These unusual binding properties could be attributed to a different conformation of the binding pocket that allows to accommodate negative charges; moreover, we identified a cluster of solvent exposed Lys residues, which are only found in the EH domain of POB1, and influence binding to both NPF and DPF motifs. The characterization of structures of the DPF ligands described in this study and the POB1 EH domain will clearly determine the involvement of the positive patch and the rationalization of our findings.