Figure - PMC

Skip to main content

An official website of the United States government

Here's how you know

Here's how you know

Official websites use .gov
A .gov website belongs to an official government organization in the United States.

Secure .gov websites use HTTPS
A lock ( ) or https:// means you've safely connected to the .gov website. Share sensitive information only on official, secure websites.

View full-text article in PMC

. 2018 Jan 16;17(4):737–763. doi: 10.1074/mcp.RA118.000573

Search in PMC
Search in PubMed
View in NLM Catalog
Add to search

© 2018 by The American Society for Biochemistry and Molecular Biology, Inc.

Author's Choice—Final version free via Creative Commons CC-BY license.

PMC Copyright notice

Fig. 13. — Summary of the biochemical properties of the peptide-docking site mutations in AGR2 produced based on hydrogen-deuterium exchange mapping. Based on the hydrogen-deuterium exchange mapping data (Fig. 4 and 5), we focused on creating three alanine substitutions mutations in the VDPSL loop motif, from amino acids 131–135, residing between two β-sheets (Fig. 6). The mutant proteins exhibit inverse trends in their specific activity. Consensus peptide binding reactions demonstrate that wt-AGR2 = S134A>D132A>P133A with two mutants showing a loss-of-function. Although in EpCAM binding, S134A>D132A>P133A = wt-AGR2 with two mutants showing a gain-of-function. These data suggest that although mutating some amino acids in the VDPSL motif can impact on specific peptide binding, the global conformation changed induced by loop mutation (for example in the gain-of-function S134A mutation (Fig. 11) might result in binding to a distinct site on the EpCAM molecule. Thus, one interpretation of such data is that one purpose of the VDPSL motif is to not only drive specific peptide binding by AGR2 but to constrain the conformational dynamics (or monomer-dimer equilibrium) of AGR2 so as to minimize its “binding to other sites” on its client proteins.