Direct fluorescent-dye labeling of α-tubulin in mammalian cells for live cell and superresolution imaging

Genetic code expansion and bioorthogonal labeling provide for the first time a way for direct, site-specific labeling of proteins with fluorescent-dyes in live cells. Although the small size and superb photophysical parameters of fluorescent-dyes offer unique advantages for high-resolution microscop...

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Autores principales: Schvartz, Tomer, Aloush, Noa, Goliand, Inna, Segal, Inbar, Nachmias, Dikla, Arbely, Eyal, Elia, Natalie
Formato: Online Artículo Texto
Lenguaje:English
Publicado: The American Society for Cell Biology 2017
Materias:
Brief Reports
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5638579/
https://www.ncbi.nlm.nih.gov/pubmed/28835375
http://dx.doi.org/10.1091/mbc.E17-03-0161
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author Schvartz, Tomer
Aloush, Noa
Goliand, Inna
Segal, Inbar
Nachmias, Dikla
Arbely, Eyal
Elia, Natalie
author_facet Schvartz, Tomer
Aloush, Noa
Goliand, Inna
Segal, Inbar
Nachmias, Dikla
Arbely, Eyal
Elia, Natalie
author_sort Schvartz, Tomer
collection PubMed
description Genetic code expansion and bioorthogonal labeling provide for the first time a way for direct, site-specific labeling of proteins with fluorescent-dyes in live cells. Although the small size and superb photophysical parameters of fluorescent-dyes offer unique advantages for high-resolution microscopy, this approach has yet to be embraced as a tool in live cell imaging. Here we evaluated the feasibility of this approach by applying it for α-tubulin labeling. After a series of calibrations, we site-specifically labeled α-tubulin with silicon rhodamine (SiR) in live mammalian cells in an efficient and robust manner. SiR-labeled tubulin successfully incorporated into endogenous microtubules at high density, enabling video recording of microtubule dynamics in interphase and mitotic cells. Applying this labeling approach to structured illumination microscopy resulted in an increase in resolution, highlighting the advantages in using a smaller, brighter tag. Therefore, using our optimized assay, genetic code expansion provides an attractive tool for labeling proteins with a minimal, bright tag in quantitative high-resolution imaging.
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spelling pubmed-56385792017-12-30 Direct fluorescent-dye labeling of α-tubulin in mammalian cells for live cell and superresolution imaging Schvartz, Tomer Aloush, Noa Goliand, Inna Segal, Inbar Nachmias, Dikla Arbely, Eyal Elia, Natalie Mol Biol Cell Brief Reports Genetic code expansion and bioorthogonal labeling provide for the first time a way for direct, site-specific labeling of proteins with fluorescent-dyes in live cells. Although the small size and superb photophysical parameters of fluorescent-dyes offer unique advantages for high-resolution microscopy, this approach has yet to be embraced as a tool in live cell imaging. Here we evaluated the feasibility of this approach by applying it for α-tubulin labeling. After a series of calibrations, we site-specifically labeled α-tubulin with silicon rhodamine (SiR) in live mammalian cells in an efficient and robust manner. SiR-labeled tubulin successfully incorporated into endogenous microtubules at high density, enabling video recording of microtubule dynamics in interphase and mitotic cells. Applying this labeling approach to structured illumination microscopy resulted in an increase in resolution, highlighting the advantages in using a smaller, brighter tag. Therefore, using our optimized assay, genetic code expansion provides an attractive tool for labeling proteins with a minimal, bright tag in quantitative high-resolution imaging. The American Society for Cell Biology 2017-10-15 /pmc/articles/PMC5638579/ /pubmed/28835375 http://dx.doi.org/10.1091/mbc.E17-03-0161 Text en © 2017 Schvartz et al. This article is distributed by The American Society for Cell Biology under license from the author(s). Two months after publication it is available to the public under an Attribution–Noncommercial–Share Alike 3.0 Unported Creative Commons License (http://creativecommons.org/licenses/by-nc-sa/3.0). “ASCB®,” “The American Society for Cell Biology®,” and “Molecular Biology of the Cell®” are registered trademarks of The American Society for Cell Biology.
spellingShingle Brief Reports
Schvartz, Tomer
Aloush, Noa
Goliand, Inna
Segal, Inbar
Nachmias, Dikla
Arbely, Eyal
Elia, Natalie
Direct fluorescent-dye labeling of α-tubulin in mammalian cells for live cell and superresolution imaging
title Direct fluorescent-dye labeling of α-tubulin in mammalian cells for live cell and superresolution imaging
title_full Direct fluorescent-dye labeling of α-tubulin in mammalian cells for live cell and superresolution imaging
title_fullStr Direct fluorescent-dye labeling of α-tubulin in mammalian cells for live cell and superresolution imaging
title_full_unstemmed Direct fluorescent-dye labeling of α-tubulin in mammalian cells for live cell and superresolution imaging
title_short Direct fluorescent-dye labeling of α-tubulin in mammalian cells for live cell and superresolution imaging
title_sort direct fluorescent-dye labeling of α-tubulin in mammalian cells for live cell and superresolution imaging
topic Brief Reports
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5638579/
https://www.ncbi.nlm.nih.gov/pubmed/28835375
http://dx.doi.org/10.1091/mbc.E17-03-0161
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