Identification of peptide-binding sites within BSA using rapid, laser-induced covalent cross-linking combined with high-performance mass spectrometry

Melinda Hauser, Chen Qian, Steven T. King, Sarah Kauffman, Fred Naider, Robert L. Hettich, Jeffrey M. Becker

Research output: Contribution to journalArticlepeer-review

8 Scopus citations

Abstract

We are developing a rapid, time-resolved method using laser-activated cross-linking to capture protein-peptide interactions as a means to interrogate the interaction of serum proteins as delivery systems for peptides and other molecules. A model system was established to investigate the interactions between bovine serum albumin (BSA) and 2 peptides, the tridecapeptide budding-yeast mating pheromone (α-factor) and the decapeptide human gonadotropin-releasing hormone (GnRH). Cross-linking of α-factor, using a biotinylated, photoactivatable p-benzoyl-L-phenylalanine (Bpa)–modified analog, was energy-dependent and achieved within seconds of laser irradiation. Protein blotting with an avidin probe was used to detect biotinylated species in the BSA-peptide complex. The cross-linked complex was trypsinized and then interrogated with nano-LC–MS/MS to identify the peptide cross-links. Cross-linking was greatly facilitated by Bpa in the peptide, but some cross-linking occurred at higher laser powers and high concentrations of a non-Bpa–modified α-factor. This was supported by experiments using GnRH, a peptide with sequence homology to α-factor, which was likewise found to be cross-linked to BSA by laser irradiation. Analysis of peptides in the mass spectra showed that the binding site for both α-factor and GnRH was in the BSA pocket defined previously as the site for fatty acid binding. This model system validates the use of laser-activation to facilitate cross-linking of Bpa-containing molecules to proteins. The rapid cross-linking procedure and high performance of MS/MS to identify cross-links provides a method to interrogate protein-peptide interactions in a living cell in a time-resolved manner.

Original languageEnglish
Article numbere2680
JournalJournal of Molecular Recognition
Volume31
Issue number2
DOIs
StatePublished - Feb 2018

Funding

This work was supported by Grant GM112496 from the National Institute of General Medical Sciences, NIH. We thank Ed Wright, Bioanalytical Resources Facility of the BCMB Department, University of Tennessee, for assistance with conducting the SPR experiments.

FundersFunder number
National Institutes of Health
National Institute of General Medical SciencesR01GM112496

    Keywords

    • BSA-peptide cross-linking
    • laser irradiation
    • mass spectrometry (MS)
    • peptide hormone
    • peptide pheromone

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