Literature DB >> 26308583

Expression-Enhanced Fluorescent Proteins Based on Enhanced Green Fluorescent Protein for Super-resolution Microscopy.

Sam Duwé, Elke De Zitter, Vincent Gielen, Benjamien Moeyaert, Wim Vandenberg, Tim Grotjohann1, Koen Clays, Stefan Jakobs2,1, Luc Van Meervelt, Peter Dedecker.   

Abstract

"Smart fluorophores", such as reversibly switchable fluorescent proteins, are crucial for advanced fluorescence imaging. However, only a limited number of such labels is available, and many display reduced biological performance compared to more classical variants. We present the development of robustly photoswitchable variants of enhanced green fluorescent protein (EGFP), named rsGreens, that display up to 30-fold higher fluorescence in E. coli colonies grown at 37 °C and more than 4-fold higher fluorescence when expressed in HEK293T cells compared to their ancestor protein rsEGFP. This enhancement is not due to an intrinsic increase in the fluorescence brightness of the probes, but rather due to enhanced expression levels that allow many more probe molecules to be functional at any given time. We developed rsGreens displaying a range of photoswitching kinetics and show how these can be used for multimodal diffraction-unlimited fluorescence imaging such as pcSOFI and RESOLFT, achieving a spatial resolution of ∼70 nm. By determining the first ever crystal structures of a negative reversibly switchable FP derived from Aequorea victoria in both the "on"- and "off"-conformation we were able to confirm the presence of a cis-trans isomerization and provide further insights into the mechanisms underlying the photochromism. Our work demonstrates that genetically encoded "smart fluorophores" can be readily optimized for biological performance and provides a practical strategy for developing maturation- and stability-enhanced photochromic fluorescent proteins.

Entities:  

Keywords:  RESOLFT; SOFI; crystal structure determination; fluorescent proteins; reversible photoswitching; rsEGFP; super-resolution fluorescence microscopy; superfolder

Mesh:

Substances:

Year:  2015        PMID: 26308583     DOI: 10.1021/acsnano.5b04129

Source DB:  PubMed          Journal:  ACS Nano        ISSN: 1936-0851            Impact factor:   15.881


  22 in total

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4.  NMR Reveals Light-Induced Changes in the Dynamics of a Photoswitchable Fluorescent Protein.

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6.  RefSOFI for Mapping Nanoscale Organization of Protein-Protein Interactions in Living Cells.

Authors:  Fabian Hertel; Gary C H Mo; Sam Duwé; Peter Dedecker; Jin Zhang
Journal:  Cell Rep       Date:  2015-12-31       Impact factor: 9.423

7.  In vivo super-resolution RESOLFT microscopy of Drosophila melanogaster.

Authors:  Sebastian Schnorrenberg; Tim Grotjohann; Gerd Vorbrüggen; Alf Herzig; Stefan W Hell; Stefan Jakobs
Journal:  Elife       Date:  2016-06-29       Impact factor: 8.140

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Authors:  Bas M C Cloin; Elke De Zitter; Desiree Salas; Vincent Gielen; Gert E Folkers; Marina Mikhaylova; Maike Bergeler; Bartosz Krajnik; Jeremy Harvey; Casper C Hoogenraad; Luc Van Meervelt; Peter Dedecker; Lukas C Kapitein
Journal:  Proc Natl Acad Sci U S A       Date:  2017-06-19       Impact factor: 11.205

9.  Two-photon excited photoconversion of cyanine-based dyes.

Authors:  Sheldon J J Kwok; Myunghwan Choi; Brijesh Bhayana; Xueli Zhang; Chongzhao Ran; Seok-Hyun Yun
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10.  Rational design of ultrastable and reversibly photoswitchable fluorescent proteins for super-resolution imaging of the bacterial periplasm.

Authors:  Mariam El Khatib; Alexandre Martins; Dominique Bourgeois; Jacques-Philippe Colletier; Virgile Adam
Journal:  Sci Rep       Date:  2016-01-06       Impact factor: 4.379

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