| Literature DB >> 32726587 |
Timurs Maculins1, Javier Garcia-Pardo2, Anamarija Skenderovic3, Jakob Gebel4, Mateusz Putyrski5, Andrew Vorobyov6, Philipp Busse7, Gabor Varga5, Maria Kuzikov8, Andrea Zaliani8, Simin Rahighi9, Veronique Schaeffer10, Michael J Parnham6, Sachdev S Sidhu11, Andreas Ernst5, Volker Dötsch4, Masato Akutsu3, Ivan Dikic12.
Abstract
Protein-protein interactions (PPIs) govern intracellular life, and identification of PPI inhibitors is challenging. Roadblocks in assay development stemming from weak binding affinities of natural PPIs impede progress in this field. We postulated that enhancing binding affinity of natural PPIs via protein engineering will aid assay development and hit discovery. This proof-of-principle study targets PPI between linear ubiquitin chains and NEMO UBAN domain, which activates NF-κB signaling. Using phage display, we generated ubiquitin variants that bind to the functional UBAN epitope with high affinity, act as competitive inhibitors, and structurally maintain the existing PPI interface. When utilized in assay development, variants enable generation of robust cell-based assays for chemical screening. Top compounds identified using this approach directly bind to UBAN and dampen NF-κB signaling. This study illustrates advantages of integrating protein engineering and chemical screening in hit identification, a development that we anticipate will have wide application in drug discovery.Entities:
Keywords: LUBAC; NF-κB; cellular screening; high throughput; hit identification; inhibitor; protein engineering; protein-protein interaction; small molecule; ubiquitin
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Year: 2020 PMID: 32726587 DOI: 10.1016/j.chembiol.2020.07.010
Source DB: PubMed Journal: Cell Chem Biol ISSN: 2451-9448 Impact factor: 8.116