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Rational Design of CDK12/13 and BRD4 Molecular Glue Degraders

24 October 2024, Version 1
Working Paper
This content is a preprint and has not undergone peer review at the time of posting.

Abstract

Targeted protein degradation (TPD) is an emerging therapeutic approach for the selective elimination of disease-related proteins. While molecular glue degraders exhibit drug-like properties, their discovery has traditionally been serendipitous and often requires post-hoc rationalization. In this study, we demonstrate the rational design of molecular glue degraders using gluing moieties. By appending a chemical gluing moiety to several small molecule inhibitors, we successfully transformed them into degraders, obviat-ing the need for a specific E3 ubiquitin ligase recruiter. Specifically, we found that incorporating a hydrophobic gluing moiety into a cyclin-dependent kinase 12 and 13 (CDK12/13) dual inhibitor enabled the recruitment of DNA damage-binding protein 1 (DDB1), thereby transforming a high-molecular-weight bivalent CDK12 degrader into a potent monovalent CDK12/13 molecular glue de-grader. We also showcase that attaching a cysteine-reactive warhead to a BRD4 inhibitor converts it into a degrader by recruiting the DDB1 and CUL4 associated factor 16 (DCAF16) E3 ligase.

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Version History

Oct 24, 2024 Version 1

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The content is available under CC BY NC ND 4.0 [opens in a new tab]

DOI

10.26434/chemrxiv-2024-jc65t
D O I: 10.26434/chemrxiv-2024-jc65t [opens in a new tab]

Funding

National Institutes of Health
R01CA262188
National Institutes of Health
R01CA2144608
National Institutes of Health
1S10OD028697-01
Basic Science Research Program through the National Research Foundation of Korea (NRF) funded by the Ministry of Education
RS-2024-00410290
Departmental funds from Stanford Chemical and Systems Biology and Stanford Cancer Institute

Author’s competing interest statement

N.S.G. is a founder, science advisory board member (SAB) and equity holder in Syros, C4, Allorion, Lighthorse, Voronoi, Incep-tion, Matchpoint, Shenandoah (board member), Larkspur (board member) and Soltego (board member). The Gray lab receives or has received research funding from Novartis, Takeda, Astellas, Taiho, Jansen, Kinogen, Arbella, Deerfield, Springworks, Inter-line and Sanofi. E.S.F. is a founder, scientific advisory board (SAB) member, and equity holder of Civetta Therapeutics, Prox-imity Therapeutics, and Neomorph, Inc. (also board of directors). He is an equity holder and SAB member for Avilar Therapeutics, Photys Therapeutics, and Ajax Therapeutics and an equity holder in Lighthorse Therapeutics. E.S.F. is a consultant to Novartis, EcoR1 capital, Odyssey and Deerfield. The Fischer lab receives or has received research funding from Deerfield, Novartis, Ajax, Interline, Bayer and Astellas. K.A.D. receives or has received consulting fees from Kronos Bio and Neomorph Inc. All other authors declare no competing interests.

Ethics

The author(s) have declared ethics committee/IRB approval is not relevant to this content

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