Critical assessment of LC3/GABARAP ligands used for degrader development and ligandability of LC3/GABARAP binding pockets

ULK1 化学 生物化学 蛋白激酶A 安普克
作者
Martin P. Schwalm,Johannes Dopfer,Adarsh Kumar,Francesco Greco,Nicolas Bauer,Frank Löhr,Jan Heering,Sara Cano-Franco,Severin Lechner,Thomas Hanke,Ivana Jaser,Viktoria Morasch,Christopher Lenz,D. Fearon,Peter Marples,Charles W. Tomlinson,Lorène Brunello,Krishna Saxena,Nathan B. P. Adams,F. von Delft
出处
期刊:Nature Communications [Nature Portfolio]
卷期号:15 (1) 被引量:1
标识
DOI:10.1038/s41467-024-54409-5
摘要

Recent successes in developing small molecule degraders that act through the ubiquitin system have spurred efforts to extend this technology to other mechanisms, including the autophagosomal-lysosomal pathway. Therefore, reports of autophagosome tethering compounds (ATTECs) have received considerable attention from the drug development community. ATTECs are based on the recruitment of targets to LC3/GABARAP, a family of ubiquitin-like proteins that presumably bind to the autophagosome membrane and tether cargo-loaded autophagy receptors into the autophagosome. In this work, we rigorously tested the target engagement of the reported ATTECs to validate the existing LC3/GABARAP ligands. Surprisingly, we were unable to detect interaction with their designated target LC3 using a diversity of biophysical methods. Intrigued by the idea of developing ATTECs, we evaluated the ligandability of LC3/GABARAP by in silico docking and large-scale crystallographic fragment screening. Data based on approximately 1000 crystal structures revealed that most fragments bound to the HP2 but not to the HP1 pocket within the LIR docking site, suggesting a favorable ligandability of HP2. Through this study, we identified diverse validated LC3/GABARAP ligands and fragments as starting points for chemical probe and ATTEC development.

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