Small fluorescence-activating and absorption-shifting tag for tunable protein imaging in vivo

Plamont, Marie‐Aude; Billon-Denis, Emmanuelle; Maurin, Sylvie; Gauron, Carole; Pimenta, Frederico M.; Specht, Christian G.; Shi, Jian; Querard, Jérôme; Pan, Buyan; Rossignol, Julien; Moncoq, Karine; Morellet, Nelly; Volovitch, Michel; Lescop, Ewen; Chen, Yong; Triller, Antoine; Vriz, Sophie; Saux, Thomas Le; Jullien, Ludovic; Gautier, Arnaud

doi:10.1073/pnas.1513094113

Cited by 193 publications

(343 citation statements)

References 50 publications

(30 reference statements)

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“…For instance, a recent publication has demonstrated that the subset of F-actin that is recognized by diverse ABDs can be altered by the fluorescent protein or the linker sequence between the ABD and the fluorescent protein (Lemieux et al, 2014). New applications for fluorescent labeling of proteins have become available recently, such as the use of Y-FAST, a small monomeric protein tag enabling reversible binding and activation of a cell-permeant and nontoxic fluorogenic molecule (Plamont et al, 2016), or the flavoprotein improved LOV (iLOV), a fluorescent protein based on the light, oxygen or voltage domain (LOV) from a variety of sources (Buckley et al, 2015). Both molecules offer advantages over GFP and other related fluorescent reporters owing to their relatively small size.…”

Section: Discussionmentioning

confidence: 99%

Actin visualization at a glance

Melak

Plessner

Grosse

2017

Journal of Cell Science

170

182

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There was an error published in J. Cell Sci. 130,[525][526][527][528][529][530] Unfortunately, the diagram of the actin filament in the poster was accidentally reflected during the creation of the figure. As a result, the filament was illustrated as a left-handed rather than a right-handed F-actin helix in the original version of this article. The online version of the article has been corrected accordingly. This change has no impact on the concepts presented in this article.The authors apologise to the readers for any confusion that this error might have caused. 1688 Journal of Cell Science CELL SCIENCE AT A GLANCE Actin visualization at a glanceMichael Melak, Matthias Plessner and Robert Grosse* ABSTRACT Actin functions in a multitude of cellular processes owing to its ability to polymerize into filaments, which can be further organized into higher-order structures by an array of actin-binding and regulatory proteins. Therefore, research on actin and actin-related functions relies on the visualization of actin structures without interfering with the cycles of actin polymerization and depolymerization that underlie cellular actin dynamics. In this Cell Science at a Glance and the accompanying poster, we briefly evaluate the different techniques and approaches currently applied to analyze and visualize cellular actin structures, including in the nuclear compartment. Referring to the gold standard F-actin marker phalloidin to stain actin in fixed samples and tissues, we highlight methods for visualization of actin in living cells, which mostly apply the principle of genetically fusing fluorescent proteins to different actin-binding domains, such as LifeAct, utrophin and F-tractin, as well as antiactin-nanobody technology. In addition, the compound SiR-actin and the expression of GFP-actin are also applicable for various types of live-cell analyses. Overall, the visualization of actin within a physiological context requires a careful choice of method, as well as a tight control of the amount or the expression level of a given detection probe in order to minimize its influence on endogenous actin dynamics.

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Section: Discussionmentioning

confidence: 99%

Actin visualization at a glance

Melak

Plessner

Grosse

2017

Journal of Cell Science

170

182

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“…Customized fluorescent proteins can be generated by engineering naturally occurring scaffolds to bind synthetic chromophores (Paige et al, 2011; Plamont et al, 2016; Tamura and Hamachi, 2014; Yapici et al, 2015). Chromophore-dependent microbial opsins provide an excellent platform for this approach since modified retinals are well accepted and their incorporation can dramatically alter and enhance opsin properties (Albeck et al, 1989; Asato et al, 1990; AzimiHashemi et al, 2014; Gaertner et al, 1981; Ganapathy et al, 2015; Hoischen et al, 1997; Nielsen, 2009; Sineshchekov et al, 2012).…”

Section: Discussionmentioning

confidence: 99%

“…In order to access Arch variants with bright NIR emission, we drew inspiration from previous demonstrations that desirable fluorescent protein properties could be obtained by expanding the limited repertoire of naturally known chromophores (Plamont et al, 2016; Tamura and Hamachi, 2014; Yapici et al, 2015). Spectral properties of the natural ATR chromophore (Figure 1 A , Compound 1) can be modulated by adding electron-withdrawing groups (Gaertner et al, 1981; Hendrickx et al, 1995) or changing the length of the conjugated π-bond system (Albeck et al, 1989; Nielsen, 2009).…”

Section: Introductionmentioning

confidence: 99%

Directed Evolution of a Bright Near-Infrared Fluorescent Rhodopsin Using a Synthetic Chromophore

Herwig

Rice

Bedbrook

et al. 2017

Cell Chemical Biology

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Summary By engineering a microbial rhodopsin, Archaerhodopsin-3 (Arch), to bind a synthetic chromophore, merocyanine retinal, in place of the natural chromophore all-trans-retinal (ATR), we generated a protein with exceptionally bright and unprecedentedly red-shifted near-infrared (NIR) fluorescence. We show that chromophore substitution generates a fluorescent Arch-complex with a 200 nm bathochromic excitation shift relative to ATR-bound wild-type Arch and an emission maximum at 772 nm. Directed evolution of this complex produced variants with pH-sensitive NIR fluorescence and molecular brightness 8.5-fold greater than the brightest ATR-bound Arch variant. The resulting proteins are well suited to bacterial imaging; expression and stability have not been optimized for mammalian cell imaging. By targeting both the protein and its chromophore we overcome inherent challenges associated with engineering bright NIR fluorescence into Archaerhodopsin. This work demonstrates an efficient strategy for engineering non-natural, tailored properties into microbial opsins, properties relevant for imaging and interrogating biological systems.

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“…FAP systems based on single‐chain antibodies are relatively large, resulting in fluorescent complexes on the order of GFP or larger. A smaller alternative non‐covalent system is the Fluoresence‐activating and Absorption‐Shifiting Tag (FAST), which was recently developed by directed evolution of the bacterial photoreceptor photoactive yellow protein (PYP) . FAST reversibly and quickly binds a family of hydroxybenzylidene rhodanine derivatives to generate complexes with emission wavelengths from green‐yellow to orange‐red .…”

Section: Introductionmentioning

confidence: 99%

“…A smaller alternative non‐covalent system is the Fluoresence‐activating and Absorption‐Shifiting Tag (FAST), which was recently developed by directed evolution of the bacterial photoreceptor photoactive yellow protein (PYP) . FAST reversibly and quickly binds a family of hydroxybenzylidene rhodanine derivatives to generate complexes with emission wavelengths from green‐yellow to orange‐red . Furthermore, it has been shown to be an effective fluorescence marker in bacteria, yeast, mammalian cell culture, and zebrafish.…”

Section: Introductionmentioning

confidence: 99%

Fluorogenic Protein‐Based Strategies for Detection, Actuation, and Sensing

Gautier

Tebo

2018

BioEssays

Self Cite

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Fluorescence imaging has become an indispensable tool in cell and molecular biology. GFP-like fluorescent proteins have revolutionized fluorescence microscopy, giving experimenters exquisite control over the localization and specificity of tagged constructs. However, these systems present certain drawbacks and as such, alternative systems based on a fluorogenic interaction between a chromophore and a protein have been developed. While these systems are initially designed as fluorescent labels, they also present new opportunities for the development of novel labeling and detection strategies. This review focuses on new labeling protocols, actuation methods, and biosensors based on fluorogenic protein systems.

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Small fluorescence-activating and absorption-shifting tag for tunable protein imaging in vivo

Cited by 193 publications

References 50 publications

Actin visualization at a glance

Actin visualization at a glance

Directed Evolution of a Bright Near-Infrared Fluorescent Rhodopsin Using a Synthetic Chromophore

Fluorogenic Protein‐Based Strategies for Detection, Actuation, and Sensing

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