DNA-programmable Protein Degradation: Dynamic Control of PROTAC Activity via DNA Hybridization and Strand Displacement

11 March 2025, Version 1
This content is a preprint and has not undergone peer review at the time of posting.

Abstract

Targeted protein degradation is a powerful therapeutic approach: expanding the druggable proteome, providing enhanced selectivity, and having the ability to overcome conventional resistance mechanisms. A major class of such molecules are proteolysis-targeting chimeras (PROTACs). PROTACs are catalytic heterobifunctional small molecules that simultaneously bind a protein of interest (POI) and an E3 ligase. These PROTACs induce a proximity-dependant ubiquitination of the POI, which causes its subsequent degradation by the ubiquitin–proteasome system. While PROTACs have successfully transitioned from academia to industry, increasing awareness of off-target effects and related toxicities highlight the urgent need for precise control mechanisms over their activity. Achieving this level of control, however, remains challenging with traditional chemistries. DNA nanotechnology, with its unparalleled programmability and structural versatility, presents a powerful tool for achieving such control. Here, we report the design and characterization of oligonucleotide-linked PROTACs (OligoPROTACs). These constructs comprise PROTAC warheads covalently linked to separate, complementary DNA strands, brought together in space via DNA hybridisation. OligoPROTACs are able to degrade the POI in a distance-dependant manner. Furthermore, we demonstrate the first-instance of a dynamic off-switch mechanism for PROTAC activity, enabled by toehold-mediated strand displacement using a third DNA strand. This work highlights the potential of DNA nanotechnology to enhance the safety and functionality of PROTAC systems, paving the way for more refined and translatable therapeutic strategies.

Keywords

DNA nanotechnology
PROTAC
Targeted protein degradation

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