Sortase-mediated enrichment of ubiquitinated proteins from complex samples
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Despite its importance in cellular signaling and protein fate, the detection of protein ubiquitination in proteomics experiments presents many challenges for researchers. Importantly, current techniques that often rely on antibodies specific for lysine sidechain modifications may miss non-canonical ubiquitination sites in experiments. We envisioned a strategy that uses sortase, a bacterial transpeptidase enzyme, to selectively modify ubiquitination sites with a Biotin tag for enrichment and downstream proteomics experiments. In this work, we demonstrate our ability to selectively modify N-terminal diglycine remnants in digested proteins with a Biotin-modified peptide, enabling downstream enrichment of previously ubiquitinated proteins. We show this proof of concept on several recombinant proteins, revealing a site of autoubiquitination in the E2 conjugating enzyme Ubc13. We show that elution of the enriched peptides can be achieved by using common guanidinium elutions or by leveraging the reversibility of sortase. Finally, we include a bifunctional peptide that is labile to trypsinization to better streamline this strategy for downstream proteomics approaches. We envision that this approach will provide an accessible strategy for the detection of ubiquitinated proteins in proteomics experiments, with the goal of enabling researchers to better detect noncanonical protein ubiquitination.