Interrogating surface versus intracellular transmembrane receptor populations 
using cell-impermeable SNAP-tag substrates

Poc, Pascal; Gutzeit, Vanessa A.; Ast, Julia; Lee, Joon; Jones, Ben J.; D´Este, Elisa; Mathes, Bettina; Hodson, David J.; Levitz, Joshua; Broichhagen, Johannes

doi:10.1101/2020.01.29.924829

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Interrogating surface versus intracellular transmembrane receptor populations using cell-impermeable SNAP-tag substrates

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Poc, Pascal
Max Planck Institute for Medical Research, Max Planck Society;

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D´Este, Elisa
Department of NanoBiophotonics, MPI for Biophysical Chemistry, Max Planck Society;

/persons/resource/persons244947

Mathes, Bettina
Max Planck Institute for Medical Research, Max Planck Society;

/persons/resource/persons208663

Broichhagen, Johannes
Chemical Biology, Max Planck Institute for Medical Research, Max Planck Society;

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https://www.biorxiv.org/content/10.1101/2020.01.29.924829v1.full.pdf
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https://pubs.rsc.org/en/content/articlepdf/2020/sc/d0sc02794d
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Citation

Poc, P., Gutzeit, V. A., Ast, J., Lee, J., Jones, B. J., D´Este, E., et al. (2020). Interrogating surface versus intracellular transmembrane receptor populations using cell-impermeable SNAP-tag substrates. Chemical Science, 2020(30), 7871-7883. doi:10.1101/2020.01.29.924829.

Cite as: https://hdl.handle.net/21.11116/0000-0005-9AB9-D

Abstract

Employing self-labelling protein tags for the attachment of fluorescent dyes has become a routine and powerful technique in optical microscopy to visualize and track fused proteins. However, membrane permeability of the dyes and the associated background signals can interfere with the analysis of extracellular labeling sites. Here we describe a novel approach to improve extracellular labeling by functionalizing the SNAP-tag substrate benzyl guanine (“BG”) with a charged sulfonate (“SBG”). This chemical manipulation improves solubility, reduces non-specific staining and renders the bioconjugation handle impermeable while leaving its cargo untouched. We report SBG-conjugated fluorophores across the visible spectrum, which cleanly label SNAP-fused proteins in the plasma membrane of living cells. We demonstrate the utility of SBG-conjugated fluorophores to interrogate class A, B and C G protein-coupled receptors (GPCRs) using a range of imaging approaches including nanoscopic super-resolution imaging, analysis of GPCR trafficking from intra- and extracellular pools, in vivo labelling in mouse brain and analysis of receptor stoichiometry using single molecule pull down.