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Discovery of a monomeric green fluorescent protein sensor for chloride by structure-guided bioinformatics

Chloride is an essential anion for all forms of life. Beyond electrolyte balance, an increasing body of evidence points to new roles for chloride in normal physiology and disease. Over the last two decades, this understanding has been advanced by chloride-sensitive fluorescent proteins for imaging a...

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Autores principales: Peng, Weicheng, Maydew, Caden C., Kam, Hiu, Lynd, Jacob K., Tutol, Jasmine N., Phelps, Shelby M., Abeyrathna, Sameera, Meloni, Gabriele, Dodani, Sheel C.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: The Royal Society of Chemistry 2022
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9645410/
https://www.ncbi.nlm.nih.gov/pubmed/36519056
http://dx.doi.org/10.1039/d2sc03903f
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author Peng, Weicheng
Maydew, Caden C.
Kam, Hiu
Lynd, Jacob K.
Tutol, Jasmine N.
Phelps, Shelby M.
Abeyrathna, Sameera
Meloni, Gabriele
Dodani, Sheel C.
author_facet Peng, Weicheng
Maydew, Caden C.
Kam, Hiu
Lynd, Jacob K.
Tutol, Jasmine N.
Phelps, Shelby M.
Abeyrathna, Sameera
Meloni, Gabriele
Dodani, Sheel C.
author_sort Peng, Weicheng
collection PubMed
description Chloride is an essential anion for all forms of life. Beyond electrolyte balance, an increasing body of evidence points to new roles for chloride in normal physiology and disease. Over the last two decades, this understanding has been advanced by chloride-sensitive fluorescent proteins for imaging applications in living cells. To our surprise, these sensors have primarily been engineered from the green fluorescent protein (GFP) found in the jellyfish Aequorea victoria. However, the GFP family has a rich sequence space that could already encode for new sensors with desired properties, thereby minimizing protein engineering efforts and accelerating biological applications. To efficiently sample this space, we present and validate a stepwise bioinformatics strategy focused first on the chloride binding pocket and second on a monomeric oligomerization state. Using this, we identified GFPxm163 from GFPxm found in the jellyfish Aequorea macrodactyla. In vitro characterization shows that the binding of chloride as well as bromide, iodide, and nitrate rapidly tunes the ground state chromophore equilibrium from the phenolate to the phenol state generating a pH-dependent, turn-off fluorescence response. Furthermore, live-cell fluorescence microscopy reveals that GFPxm163 provides a reversible, yet indirect readout of chloride transport via iodide exchange. With this demonstration, we anticipate that the pairing of bioinformatics with protein engineering methods will provide an efficient methodology to discover and design new chloride-sensitive fluorescent proteins for cellular applications.
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spelling pubmed-96454102022-12-13 Discovery of a monomeric green fluorescent protein sensor for chloride by structure-guided bioinformatics Peng, Weicheng Maydew, Caden C. Kam, Hiu Lynd, Jacob K. Tutol, Jasmine N. Phelps, Shelby M. Abeyrathna, Sameera Meloni, Gabriele Dodani, Sheel C. Chem Sci Chemistry Chloride is an essential anion for all forms of life. Beyond electrolyte balance, an increasing body of evidence points to new roles for chloride in normal physiology and disease. Over the last two decades, this understanding has been advanced by chloride-sensitive fluorescent proteins for imaging applications in living cells. To our surprise, these sensors have primarily been engineered from the green fluorescent protein (GFP) found in the jellyfish Aequorea victoria. However, the GFP family has a rich sequence space that could already encode for new sensors with desired properties, thereby minimizing protein engineering efforts and accelerating biological applications. To efficiently sample this space, we present and validate a stepwise bioinformatics strategy focused first on the chloride binding pocket and second on a monomeric oligomerization state. Using this, we identified GFPxm163 from GFPxm found in the jellyfish Aequorea macrodactyla. In vitro characterization shows that the binding of chloride as well as bromide, iodide, and nitrate rapidly tunes the ground state chromophore equilibrium from the phenolate to the phenol state generating a pH-dependent, turn-off fluorescence response. Furthermore, live-cell fluorescence microscopy reveals that GFPxm163 provides a reversible, yet indirect readout of chloride transport via iodide exchange. With this demonstration, we anticipate that the pairing of bioinformatics with protein engineering methods will provide an efficient methodology to discover and design new chloride-sensitive fluorescent proteins for cellular applications. The Royal Society of Chemistry 2022-10-06 /pmc/articles/PMC9645410/ /pubmed/36519056 http://dx.doi.org/10.1039/d2sc03903f Text en This journal is © The Royal Society of Chemistry https://creativecommons.org/licenses/by-nc/3.0/
spellingShingle Chemistry
Peng, Weicheng
Maydew, Caden C.
Kam, Hiu
Lynd, Jacob K.
Tutol, Jasmine N.
Phelps, Shelby M.
Abeyrathna, Sameera
Meloni, Gabriele
Dodani, Sheel C.
Discovery of a monomeric green fluorescent protein sensor for chloride by structure-guided bioinformatics
title Discovery of a monomeric green fluorescent protein sensor for chloride by structure-guided bioinformatics
title_full Discovery of a monomeric green fluorescent protein sensor for chloride by structure-guided bioinformatics
title_fullStr Discovery of a monomeric green fluorescent protein sensor for chloride by structure-guided bioinformatics
title_full_unstemmed Discovery of a monomeric green fluorescent protein sensor for chloride by structure-guided bioinformatics
title_short Discovery of a monomeric green fluorescent protein sensor for chloride by structure-guided bioinformatics
title_sort discovery of a monomeric green fluorescent protein sensor for chloride by structure-guided bioinformatics
topic Chemistry
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9645410/
https://www.ncbi.nlm.nih.gov/pubmed/36519056
http://dx.doi.org/10.1039/d2sc03903f
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