Issue 12, 2024

Induced degradation of SNAP-fusion proteins

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.

Graphical abstract: Induced degradation of SNAP-fusion proteins

Supplementary files

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Article information

Article type
Paper
Submitted
05 Aug 2024
Accepted
14 Oct 2024
First published
21 Oct 2024
This article is Open Access
Creative Commons BY license

RSC Chem. Biol., 2024,5, 1232-1247

Induced degradation of SNAP-fusion proteins

S. A. Pol, S. Liljenberg, J. Barr, G. Simon, L. Wong-Dilworth, D. L. Paterson, V. P. Berishvili, F. Bottanelli, F. Kaschani, M. Kaiser, M. Pettersson and D. Hellerschmied, RSC Chem. Biol., 2024, 5, 1232 DOI: 10.1039/D4CB00184B

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