Influence of the First Chromophore-Forming Residue on Photobleaching and Oxidative Photoconversion of EGFP and EYFP

Tirthendu Sen; Anastasia Mamontova; Anastasia Titelmayer; Aleksander Shakhov; Artyom Astafiev; Atanu Acharya; Konstantin Lukyanov; Anna Krylov; Alexey Bogdanov

doi:10.3390/ijms20205229

Influence of the First Chromophore-Forming Residue on Photobleaching and Oxidative Photoconversion of EGFP and EYFP

International Journal of Molecular Sciences ◽

10.3390/ijms20205229 ◽

2019 ◽

Vol 20 (20) ◽

pp. 5229 ◽

Cited By ~ 2

Author(s):

Tirthendu Sen ◽

Anastasia Mamontova ◽

Anastasia Titelmayer ◽

Aleksander Shakhov ◽

Artyom Astafiev ◽

...

Keyword(s):

Excited State ◽

Amino Acid ◽

Fluorescent Protein ◽

Fluorescent Proteins ◽

Yellow Fluorescent Protein ◽

Radiative Lifetime ◽

Enhanced Yellow Fluorescent Protein ◽

Atomistic Calculations ◽

Oxidation Efficiency ◽

Green Fluorescent

Enhanced green fluorescent protein (EGFP)—one of the most widely applied genetically encoded fluorescent probes—carries the threonine-tyrosine-glycine (TYG) chromophore. EGFP efficiently undergoes green-to-red oxidative photoconversion (“redding”) with electron acceptors. Enhanced yellow fluorescent protein (EYFP), a close EGFP homologue (five amino acid substitutions), has a glycine-tyrosine-glycine (GYG) chromophore and is much less susceptible to redding, requiring halide ions in addition to the oxidants. In this contribution we aim to clarify the role of the first chromophore-forming amino acid in photoinduced behavior of these fluorescent proteins. To that end, we compared photobleaching and redding kinetics of EGFP, EYFP, and their mutants with reciprocally substituted chromophore residues, EGFP-T65G and EYFP-G65T. Measurements showed that T65G mutation significantly increases EGFP photostability and inhibits its excited-state oxidation efficiency. Remarkably, while EYFP-G65T demonstrated highly increased spectral sensitivity to chloride, it is also able to undergo redding chloride-independently. Atomistic calculations reveal that the GYG chromophore has an increased flexibility, which facilitates radiationless relaxation leading to the reduced fluorescence quantum yield in the T65G mutant. The GYG chromophore also has larger oscillator strength as compared to TYG, which leads to a shorter radiative lifetime (i.e., a faster rate of fluorescence). The faster fluorescence rate partially compensates for the loss of quantum efficiency due to radiationless relaxation. The shorter excited-state lifetime of the GYG chromophore is responsible for its increased photostability and resistance to redding. In EYFP and EYFP-G65T, the chromophore is stabilized by π-stacking with Tyr203, which suppresses its twisting motions relative to EGFP.

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High agonist-independent clearance of rabbit kinin B1 receptors in cultured cells

AJP Heart and Circulatory Physiology ◽

10.1152/ajpheart.00884.2002 ◽

2003 ◽

Vol 284 (5) ◽

pp. H1647-H1654 ◽

Cited By ~ 11

Author(s):

Jean-Philippe Fortin ◽

Johanne Bouthillier ◽

François Marceau

Keyword(s):

Fluorescent Protein ◽

Cultured Cells ◽

Fluorescent Proteins ◽

Yellow Fluorescent Protein ◽

Brefeldin A ◽

Metabolic Inhibitors ◽

Maximal Effect ◽

Hek 293 ◽

B1 Receptors ◽

Green Fluorescent

We hypothesized that the inducible kinin B1 receptor (B1R) is rapidly cleared from cells when its synthesis subsides. The agonist-independent degradation of the rabbit B1Rs and related B2 receptors (B2Rs) was investigated. Endocytosis of the B1R-yellow fluorescent protein (YFP) conjugate was more intense than that of B2R-green fluorescent protein (GFP) based on fluorescence accumulation in HEK 293 cells treated with a lysosomal inhibitor. The cells expressing B1R-YFP contained more GFP/YFP-sized degradation product(s) than those expressing B2R-GFP (immunoblot, antibodies equally reacting with both fluorescent proteins). The binding site density of B1R-YFP decreased in the presence of protein synthesis or maturation inhibitors (anisomycin, brefeldin A), whereas that of B2R-GFP remained constant. Wild-type B1Rs were also cleared faster than B2Rs in rabbit smooth muscle cells treated with metabolic inhibitors. Contractility experiments based on brefeldin A-treated isolated rabbit blood vessels also functionally support that B1Rs are more rapidly eliminated than B2Rs (decreased maximal effect of agonist over 2 h). The highly regulated B1R is rapidly degraded, relative to the constitutive B2R.

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C-terminal eYFP fusion impairs Escherichia coli MinE function

Open Biology ◽

10.1098/rsob.200010 ◽

2020 ◽

Vol 10 (5) ◽

pp. 200010

Author(s):

Navaneethan Palanisamy ◽

Mehmet Ali Öztürk ◽

Emir Bora Akmeriç ◽

Barbara Di Ventura

Keyword(s):

Escherichia Coli ◽

In Silico ◽

Fluorescent Protein ◽

Fluorescent Proteins ◽

Yellow Fluorescent Protein ◽

Time Lapse ◽

Enhanced Yellow Fluorescent Protein ◽

Min Proteins

The Escherichia coli Min system plays an important role in the proper placement of the septum ring at mid-cell during cell division. MinE forms a pole-to-pole spatial oscillator with the membrane-bound ATPase MinD, resulting in MinD concentration being the lowest at mid-cell. MinC, the direct inhibitor of the septum initiator protein FtsZ, forms a complex with MinD at the membrane, mirroring its polar gradients. Therefore, MinC-mediated FtsZ inhibition occurs away from mid-cell. Min oscillations are often studied in living cells by time-lapse microscopy using fluorescently labelled Min proteins. Here, we show that, despite permitting oscillations to occur in a range of protein concentrations, the enhanced yellow fluorescent protein (eYFP) C-terminally fused to MinE impairs its function. Combining in vivo , in vitro and in silico approaches, we demonstrate that eYFP compromises the ability of MinE to displace MinC from MinD, to stimulate MinD ATPase activity and to directly bind to the membrane. Moreover, we reveal that MinE-eYFP is prone to aggregation. In silico analyses predict that other fluorescent proteins are also likely to compromise several functionalities of MinE, suggesting that the results presented here are not specific to eYFP.

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Enhancement of correct protein folding in vivo by a non-lytic baculovirus

Biochemical Journal ◽

10.1042/bj20040007 ◽

2004 ◽

Vol 382 (2) ◽

pp. 695-702 ◽

Cited By ~ 20

Author(s):

Yu HO ◽

Huei-Ru LO ◽

Tzu-Ching LEE ◽

Carol P. Y. WU ◽

Yu-Chan CHAO

Keyword(s):

Energy Transfer ◽

Fusion Protein ◽

Fluorescent Protein ◽

Fluorescent Proteins ◽

Yellow Fluorescent Protein ◽

Random Mutagenesis ◽

Resonance Energy ◽

Vector System ◽

Enhanced Yellow Fluorescent Protein

The BEVS (baculovirus expression vector system) is widely used for the production of proteins. However, engineered proteins frequently experience the problem of degradation, possibly due to the lytic nature of the conventional BEVS (herein referred to as L-BEVS). In the present study, a non-lytic BEVS (N-BEVS) was established by random mutagenesis of viral genomes. At 5 days post-infection, N-BEVS showed only 7% cell lysis, whereas L-BEVS showed 60% lysis of cells. The quality of protein expressed in both N- and L-BEVSs was examined further using a novel FRET (fluorescence resonance energy transfer)-based assay. To achieve this, we constructed a concatenated fusion protein comprising LUC (luciferase) sandwiched between EYFP (enhanced yellow fluorescent protein) and ECFP (enhanced cyan fluorescent protein). The distance separating the two fluorescent proteins in the fusion protein EYFP–LUC–ECFP (designated hereafter as the YLC construct) governs energy transfer between EYFP and ECFP. FRET efficiency thus reflects the compactness of LUC, indicating its folding status. We found more efficient FRET in N-BEVS compared with that obtained in L-BEVS, suggesting that more tightly folded LUC was produced in N-BEVS. YLC expression was also analysed by Western blotting, revealing significantly less protein degradation in N-BEVS than in L-BEVS, in which extensive degradation was observed. This FRET-based in vivo folding technology showed that YLC produced in N-BEVS is more compact, correlating with improved resistance to degradation. N-BEVS is thus a convenient alternative for L-BEVS for the production of proteins vulnerable to degradation using baculoviruses.

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Against the NEER principle: The third type of photochromism for GFP chromophore derivatives

Physical Chemistry Chemical Physics ◽

10.1039/d1cp03581a ◽

2021 ◽

Author(s):

Jun-Wei Liao ◽

Robert Sung ◽

Kuangsen Sung

Keyword(s):

Excited State ◽

Green Fluorescent Protein ◽

Proton Transfer ◽

Fluorescent Protein ◽

Fluorescent Proteins ◽

The Third ◽

Excited State Proton Transfer ◽

Gfp Chromophore ◽

Green Fluorescent

Photochromism is the heart of photochromic fluorescent proteins. Excited-state proton transfer (ESPT) is the major photochromism for green fluorescent protein (GFP) and Z-E photoisomerization through τ-torsion is the major photochromism...

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Three-dimensional distribution of enhanced yellow fluorescent protein (eYFP)-expressing neurons (yellow) and enhanced green fluorescent protein (eGFP)-positive microglia (green) in the neocortex of a Thy1-eYFP×Cx3cr1-eGFP mouse implanted with an open skull window: Movie 87_1.

Cold Spring Harbor Protocols ◽

10.1101/pdb.mov107 ◽

2011 ◽

Vol 2011 (3) ◽

pp. mov107

Keyword(s):

Green Fluorescent Protein ◽

Enhanced Green Fluorescent Protein ◽

Fluorescent Protein ◽

Yellow Fluorescent Protein ◽

Three Dimensional ◽

Enhanced Yellow Fluorescent Protein ◽

Dimensional Distribution ◽

Green Fluorescent

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Structural analysis of the bright monomeric yellow-green fluorescent protein mNeonGreen obtained by directed evolution

Acta Crystallographica Section D Structural Biology ◽

10.1107/s2059798316018623 ◽

2016 ◽

Vol 72 (12) ◽

pp. 1298-1307 ◽

Cited By ~ 16

Author(s):

Damien Clavel ◽

Guillaume Gotthard ◽

David von Stetten ◽

Daniele De Sanctis ◽

Hélène Pasquier ◽

...

Keyword(s):

Green Fluorescent Protein ◽

Directed Evolution ◽

Fluorescent Protein ◽

Fluorescent Proteins ◽

Yellow Fluorescent Protein ◽

X Rays ◽

Visible Absorption ◽

X Ray ◽

X Ray Crystallography ◽

Green Fluorescent

Until recently, genes coding for homologues of the autofluorescent protein GFP had only been identified in marine organisms from the phyla Cnidaria and Arthropoda. New fluorescent-protein genes have now been found in the phylum Chordata, coding for particularly bright oligomeric fluorescent proteins such as the tetrameric yellow fluorescent proteinlanYFP fromBranchiostoma lanceolatum. A successful monomerization attempt led to the development of the bright yellow-green fluorescent protein mNeonGreen. The structures oflanYFP and mNeonGreen have been determined and compared in order to rationalize the directed evolution process leading from a bright, tetrameric to a still bright, monomeric fluorescent protein. An unusual discolouration of crystals of mNeonGreen was observed after X-ray data collection, which was investigated using a combination of X-ray crystallography and UV–visible absorption and Raman spectroscopies, revealing the effects of specific radiation damage in the chromophore cavity. It is shown that X-rays rapidly lead to the protonation of the phenolate O atom of the chromophore and to the loss of its planarity at the methylene bridge.

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pFPL Vectors for High-Throughput Protein Localization in Fungi: Detecting Cytoplasmic Accumulation of Putative Effector Proteins

Molecular Plant-Microbe Interactions ◽

10.1094/mpmi-05-14-0144-ta ◽

2015 ◽

Vol 28 (2) ◽

pp. 107-121 ◽

Cited By ~ 13

Author(s):

Xiaoyan Gong ◽

Oscar Hurtado ◽

Baohua Wang ◽

Congqing Wu ◽

Mihwa Yi ◽

...

Keyword(s):

High Throughput ◽

Large Scale ◽

Fluorescent Protein ◽

Fluorescent Proteins ◽

Protein Localization ◽

Yellow Fluorescent Protein ◽

Effector Proteins ◽

Fungal Transformation ◽

In Planta ◽

Green Fluorescent

As part of a large-scale project whose goal was to identify candidate effector proteins in Magnaporthe oryzae, we developed a suite of vectors that facilitate high-throughput protein localization experiments in fungi. These vectors utilize Gateway recombinational cloning to place a gene's promoter and coding sequences upstream and in frame with enhanced cyan fluorescent protein, green fluorescent protein (GFP), monomeric red fluorescence protein (mRFP), and yellow fluorescent protein or a nucleus-targeted mCHERRY variant. The respective Gateway cassettes were incorporated into Agrobacterium-based plasmids to allow efficient fungal transformation using hygromycin or geneticin resistance selection. mRFP proved to be more sensitive than the GFP spectral variants for monitoring proteins secreted in planta; and extensive testing showed that Gateway-derived fusion proteins produced localization patterns identical to their “directly fused” counterparts. Use of plasmid for fungal protein localization (pFPL) vectors with two different selectable markers provided a convenient way to label fungal cells with different fluorescent proteins. We demonstrate the utility of the pFPL vectors for identifying candidate effector proteins and we highlight a number of important factors that must be taken into consideration when screening for proteins that are translocated across the host plasma membrane.

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Optimized expression of dual reporter genes in transient transfection of purifiedToxoplasma gondiiusing different promoters

Canadian Journal of Microbiology ◽

10.1139/w2012-017 ◽

2012 ◽

Vol 58 (4) ◽

pp. 483-489

Author(s):

Yongxin Hao ◽

Jianmin Yang ◽

Xuelian Li ◽

Jun Ding ◽

Wei Zhang ◽

...

Keyword(s):

Fluorescent Protein ◽

Yellow Fluorescent Protein ◽

Reporter Genes ◽

Transient Transfection ◽

Luciferase Reporter ◽

Reporter System ◽

Enhanced Yellow Fluorescent Protein ◽

Dual Reporter ◽

Green Fluorescent ◽

Living Tissues

Fluorescent protein and luciferase genes are valuable reporter genes and have been widely used for noninvasive monitoring of gene expression in living tissues and cells. We tested expression of the dual reporter genes in transient transfection of purified Toxoplasma gondii tachyzoites. Two copies of the enhanced yellow fluorescent protein (EYFP) gene were put under the control of 3 representative T. gondii promoters (GRA1, SAG1, and DHFR). Fluorescence from each EYFP reporter was significantly higher than that from a green fluorescent protein (GFP) reporter. The GRA1-EYFP reporter gave the highest fluorescence. Although both fluorescence and luciferase were expressed in the dual reporter system, the luciferase reporter was more efficient than either the EYFP or GFP reporters, and it required fewer parasites to be successfully used.

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Nature-inspired Circular-economy Recycling (NaCRe) for Proteins: Proof of Concept

10.1101/2020.09.23.309799 ◽

2020 ◽

Author(s):

Simone Giaveri ◽

Adeline M. Schmitt ◽

Laura Roset Julià ◽

Anna Murello ◽

Laure Menin ◽

...

Keyword(s):

Amino Acids ◽

Amino Acid ◽

Circular Economy ◽

Fluorescent Protein ◽

Fluorescent Proteins ◽

Raw Materials ◽

Free Cell ◽

Translation System ◽

Natural Polymers ◽

Green Fluorescent

AbstractIn 2070, 1012 Kg of polymer-based materials (i.e. plastics) might be produced yearly, posing one of the greatest challenges that humanity has to face. Even though natural polymers, such as proteins and nucleic acids, are more abundant than synthetic ones, they are sustainable. The key property of such natural polymers is that they are sequence-defined. This allows for recycling to start with depolymerization into monomers, and end in the re-assembly of new polymers of arbitrarily different sequence. This process breaks a common recycling paradigm that a material is recycled only into itself. An organism digests proteins into amino acids. These are re-assembled into new proteins whose identity depends on the cell’s needs at the time of protein synthesis. Here we show that the process described above is achievable extra-cellularly. Specifically, we depolymerized a mixture of different peptides and/or proteins into their amino acid constituents and used these amino acids to synthesize fluorescent proteins using an amino acid-free cell-free transcription-translation system. We were successful in recycling proteins with high relevance in materials engineering (β-lactoglobulin films, used for water filtration, or silk fibroin solutions) into a biotechnologically relevant protein (green fluorescent protein). The potential long-term impact of this approach to recycling lies in its compatibility with circular-economy models where raw materials remain in use as long as possible, thus reducing the burden on the planet.

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Simultaneous Visualization of the Yellow and Green Forms of the Green Fluorescent Protein in Living Cells

Journal of Histochemistry & Cytochemistry ◽

10.1177/002215549804600911 ◽

1998 ◽

Vol 46 (9) ◽

pp. 1073-1076 ◽

Cited By ~ 18

Author(s):

Chris T. Baumann ◽

Carol S. Lim ◽

Gordon L. Hager

Keyword(s):

Green Fluorescent Protein ◽

Laser Scanning ◽

Fluorescent Protein ◽

Yellow Fluorescent Protein ◽

Simultaneous Detection ◽

Argon Laser ◽

Living Cells ◽

Left Shoulder ◽

Enhanced Yellow Fluorescent Protein ◽

Green Fluorescent

In this study we sought to develop a method for the co-localization of proteins in living cells utilizing the enhanced green fluorescent protein (EGFP) and a redshifted EGFP variant, EYFP (enhanced yellow fluorescent protein). EYFP was expressed as an unsubstituted molecule while EGFP was fused to NF1 (EGFP-NF1), a transcription factor found exclusively in the nucleus. The Leica TCS SP laser scanning confocal microscope was used. This microscope allows the user to monitor the emitted light at defined wavelengths owing to the presence of a monochrometer in the emission light path. pEGFP-NF1 and pEYFP were co-expressed in the same cell and excited with the 476–nm and 488–nm argon laser lines. To separate the EYFP and EGFP fluorescence, EGFP-NF1 emission was recorded between 496 and 505 nm. These wavelengths are on the left shoulder of the EGFP emission peak and exclude most of the EYFP fluorescence. The EYFP emission was followed between 670 and 754 nm, utilizing the tail of EYFP emission that extends well beyond that for EGFP. Under these conditions we obtained excellent discrimination between EYFP fluorescence and EGFP-NF1 emission. These observations demonstrate that EYFP- and EGFP-substituted chimeras can be used for simultaneous detection in living cells.

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