Literature DB >> 25140415

Evaluation of fluorophores to label SNAP-tag fused proteins for multicolor single-molecule tracking microscopy in live cells.

Peter J Bosch1, Ivan R Corrêa2, Michael H Sonntag3, Jenny Ibach4, Luc Brunsveld3, Johannes S Kanger1, Vinod Subramaniam5.   

Abstract

Single-molecule tracking has become a widely used technique for studying protein dynamics and their organization in the complex environment of the cell. In particular, the spatiotemporal distribution of membrane receptors is an active field of study due to its putative role in the regulation of signal transduction. The SNAP-tag is an intrinsically monovalent and highly specific genetic tag for attaching a fluorescent label to a protein of interest. Little information is currently available on the choice of optimal fluorescent dyes for single-molecule microscopy utilizing the SNAP-tag labeling system. We surveyed 6 green and 16 red excitable dyes for their suitability in single-molecule microscopy of SNAP-tag fusion proteins in live cells. We determined the nonspecific binding levels and photostability of these dye conjugates when bound to a SNAP-tag fused membrane protein in live cells. We found that only a limited subset of the dyes tested is suitable for single-molecule tracking microscopy. The results show that a careful choice of the dye to conjugate to the SNAP-substrate to label SNAP-tag fusion proteins is very important, as many dyes suffer from either rapid photobleaching or high nonspecific staining. These characteristics appear to be unpredictable, which motivated the need to perform the systematic survey presented here. We have developed a protocol for evaluating the best dyes, and for the conditions that we evaluated, we find that Dy 549 and CF 640 are the best choices tested for single-molecule tracking. Using an optimal dye pair, we also demonstrate the possibility of dual-color single-molecule imaging of SNAP-tag fusion proteins. This survey provides an overview of the photophysical and imaging properties of a range of SNAP-tag fluorescent substrates, enabling the selection of optimal dyes and conditions for single-molecule imaging of SNAP-tagged fusion proteins in eukaryotic cell lines.
Copyright © 2014 Biophysical Society. Published by Elsevier Inc. All rights reserved.

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Year:  2014        PMID: 25140415      PMCID: PMC4142238          DOI: 10.1016/j.bpj.2014.06.040

Source DB:  PubMed          Journal:  Biophys J        ISSN: 0006-3495            Impact factor:   4.033


  72 in total

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3.  An engineered protein tag for multiprotein labeling in living cells.

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Authors:  Xiaoli Sun; Aihua Zhang; Brenda Baker; Luo Sun; Angela Howard; John Buswell; Damien Maurel; Anastasiya Masharina; Kai Johnsson; Christopher J Noren; Ming-Qun Xu; Ivan R Corrêa
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  28 in total

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Review 3.  Visualizing the in vitro assembly of tropomyosin/actin filaments using TIRF microscopy.

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4.  Workflows of the Single-Molecule Imaging Analysis in Living Cells: Tutorial Guidance to the Measurement of the Drug Effects on a GPCR.

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6.  Single-Color Fluorescence Lifetime Cross-Correlation Spectroscopy In Vivo.

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7.  Simultaneous Multicolor Single-Molecule Tracking with Single-Laser Excitation via Spectral Imaging.

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9.  Single-Molecule Fluorescence Detection of the Epidermal Growth Factor Receptor in Membrane Discs.

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10.  Influence of fluorescent tag on the motility properties of kinesin-1 in single-molecule assays.

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