Investigating the Binding of Peptidyl-prolyl Isomerase Pin1 to a Multi-site Phosphorylated Substrate Modeled After Phosphatase CDC25C.
Author | : Michelle K. Dubinsky |
Publisher | : |
Total Pages | : |
Release | : 2015 |
ISBN-10 | : OCLC:1067252523 |
ISBN-13 | : |
Rating | : 4/5 (23 Downloads) |
Download or read book Investigating the Binding of Peptidyl-prolyl Isomerase Pin1 to a Multi-site Phosphorylated Substrate Modeled After Phosphatase CDC25C. written by Michelle K. Dubinsky and published by . This book was released on 2015 with total page pages. Available in PDF, EPUB and Kindle. Book excerpt: Pin1 is a human protein classified as a peptidyl-prolyl cis/trans isomerase. The protein regulates the conformation of phosphorylated protein substrates by rotating the peptide bond between phosphorylated serine/threonine residues that precede proline residues. Structurally, Pin1 consists of an N-terminal WW domain and a C-terminal PPIase domain. The PPIase domain catalyzes cis/trans isomerization of peptide bonds in substrate proteins that contain the aforementioned consensus motif. We hypothesize that Pin1 binding is positively impacted when two phospho-acceptor sites on peptides derived from mitotic phosphatase CDC25C, a known Pin1-interacting protein, are phosphorylated. Using nuclear magnetic resonance and fluorescence polarization, binding affinities of CDC25C peptides to Pin1 were calculated. The results indicate that doubly-phosphorylated peptides bound to Pin1 have lower dissociation constants and consequently greater binding affinities, than complexes containing non- or singly-phosphorylated peptides, at the equivalent residues. This suggests that Pin1 has two independent phospho-binding sites that when bound, increase substrate binding affinity.