Induced degradation of SNAP-fusion proteins

Savina Abraham Pol; Sara Liljenberg; Jack Barr; Gina Simon; Luis Wong-Dilworth; Danielle L Paterson; Vladimir P Berishvili; Francesca Bottanelli; Farnusch Kaschani; Markus Kaiser; Mariell Pettersson; Doris Hellerschmied

doi:10.1039/d4cb00184b

Induced degradation of SNAP-fusion proteins

RSC Chem Biol. 2024 Oct 21. doi: 10.1039/d4cb00184b. Online ahead of print.

Affiliations

¹ Department of Mechanistic Cell Biology, University of Duisburg-Essen, Center of Medical Biotechnology, Faculty of Biology Essen Germany doris.hellerschmied@uni-due.de.
² Medicinal Chemistry, Research and Early Development, Cardiovascular, Renal and Metabolism (CVRM), BioPharmaceuticals R&D, AstraZeneca Gothenburg 431 83 Sweden mariell.pettersson@astrazeneca.com.
³ Institut für Biochemie, Freie Universität Berlin Thielallee 63 Berlin 14195 Germany.
⁴ Department of Chemical Biology, University of Duisburg-Essen, Center for Medical Biotechnology, Faculty of Biology Essen Germany.

Abstract

Self-labeling protein tags are an efficient means to visualize, manipulate, and isolate engineered fusion proteins with suitable chemical probes. The SNAP-tag, which covalently conjugates to benzyl-guanine and -chloropyrimidine derivatives is used extensively in fluorescence microscopy, given the availability of suitable SNAP-ligand-based probes. Here, we extend the applicability of the SNAP-tag to targeted protein degradation. We developed a set of SNAP PROteolysis TArgeting Chimeras (SNAP-PROTACs), which recruit the VHL or CRBN-ubiquitin E3 ligases to induce the degradation of SNAP-fusion proteins. Endogenous tagging enabled the visualization and the selective depletion of a SNAP-clathrin light chain fusion protein using SNAP-PROTACs. The addition of PROTACs to the SNAP-tag reagent toolbox facilitates the comprehensive analysis of protein function with a single gene tagging event.