Open AccessIdentification of highly selective covalent inhibitors by phage display
Author(s) -
Shiyu Chen,
S. Lovell,
Sumin Lee,
M. Fellner,
Peter D. Mace,
Matthew Bogyo
Publication year - 2020
Publication title -
nature biotechnology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 15.358
H-Index - 445
eISSN - 1546-1696
pISSN - 1087-0156
DOI - 10.1038/s41587-020-0733-7
Subject(s) - covalent bond , cysteine , chemistry , linker , small molecule , electrophile , combinatorial chemistry , phage display , proteases , chemical biology , biochemistry , stereochemistry , enzyme , peptide , organic chemistry , computer science , catalysis , operating system
Molecules that covalently bind macromolecular targets have found widespread applications as activity-based probes and as irreversibly binding drugs. However, the general reactivity of the electrophiles needed for covalent bond formation makes control of selectivity difficult. There is currently no rapid, unbiased screening method to identify new classes of covalent inhibitors from highly diverse pools of candidate molecules. Here we describe a phage display method to directly screen for ligands that bind to protein targets through covalent bond formation. This approach makes use of a reactive linker to form cyclic peptides on the phage surface while simultaneously introducing an electrophilic 'warhead' to covalently react with a nucleophile on the target. Using this approach, we identified cyclic peptides that irreversibly inhibited a cysteine protease and a serine hydrolase with nanomolar potency and exceptional specificity. This approach should enable rapid, unbiased screening to identify new classes of highly selective covalent inhibitors for diverse molecular targets.