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Selective Immobilization of Fluorescent Proteins for the Fabrication of Photoactive Materials

The immobilization of fluorescent proteins is a key technology enabling to fabricate a new generation of photoactive materials with potential technological applications. Herein we have exploited superfolder green (sGFP) and red (RFP) fluorescent proteins expressed with different polypeptide tags. We...

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Autores principales: Benítez-Mateos, Ana I., Mehravar, Ehsan, Velasco-Lozano, Susana, Tomovska, Radmila, Salassa, Luca, López-Gallego, Fernando
Formato: Online Artículo Texto
Lenguaje:English
Publicado: MDPI 2019
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6696454/
https://www.ncbi.nlm.nih.gov/pubmed/31366154
http://dx.doi.org/10.3390/molecules24152775
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author Benítez-Mateos, Ana I.
Mehravar, Ehsan
Velasco-Lozano, Susana
Tomovska, Radmila
Salassa, Luca
López-Gallego, Fernando
author_facet Benítez-Mateos, Ana I.
Mehravar, Ehsan
Velasco-Lozano, Susana
Tomovska, Radmila
Salassa, Luca
López-Gallego, Fernando
author_sort Benítez-Mateos, Ana I.
collection PubMed
description The immobilization of fluorescent proteins is a key technology enabling to fabricate a new generation of photoactive materials with potential technological applications. Herein we have exploited superfolder green (sGFP) and red (RFP) fluorescent proteins expressed with different polypeptide tags. We fused these fluorescent proteins to His-tags to immobilize them on graphene 3D hydrogels, and Cys-tags to immobilize them on porous microparticles activated with either epoxy or disulfide groups and with Lys-tags to immobilize them on upconverting nanoparticles functionalized with carboxylic groups. Genetically programming sGFP and RFP with Cys-tag and His-tag, respectively, allowed tuning the protein spatial organization either across the porous structure of two microbeads with different functional groups (agarose-based materials activated with metal chelates and epoxy-methacrylate materials) or across the surface of a single microbead functionalized with both metal-chelates and disulfide groups. By using different polypeptide tags, we can control the attachment chemistry but also the localization of the fluorescent proteins across the material surfaces. The resulting photoactive material formed by His-RFP immobilized on graphene hydrogels has been tested as pH indicator to measure pH changes in the alkaline region, although the immobilized fluorescent protein exhibited a narrower dynamic range to measure pH than the soluble fluorescent protein. Likewise, the immobilization of Lys-sGFP on alginate-coated upconverting nanoparticles enabled the infrared excitation of the fluorescent protein to be used as a green light emitter. These novel photoactive biomaterials open new avenues for innovative technological developments towards the fabrication of biosensors and photonic devices.
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spelling pubmed-66964542019-09-05 Selective Immobilization of Fluorescent Proteins for the Fabrication of Photoactive Materials Benítez-Mateos, Ana I. Mehravar, Ehsan Velasco-Lozano, Susana Tomovska, Radmila Salassa, Luca López-Gallego, Fernando Molecules Article The immobilization of fluorescent proteins is a key technology enabling to fabricate a new generation of photoactive materials with potential technological applications. Herein we have exploited superfolder green (sGFP) and red (RFP) fluorescent proteins expressed with different polypeptide tags. We fused these fluorescent proteins to His-tags to immobilize them on graphene 3D hydrogels, and Cys-tags to immobilize them on porous microparticles activated with either epoxy or disulfide groups and with Lys-tags to immobilize them on upconverting nanoparticles functionalized with carboxylic groups. Genetically programming sGFP and RFP with Cys-tag and His-tag, respectively, allowed tuning the protein spatial organization either across the porous structure of two microbeads with different functional groups (agarose-based materials activated with metal chelates and epoxy-methacrylate materials) or across the surface of a single microbead functionalized with both metal-chelates and disulfide groups. By using different polypeptide tags, we can control the attachment chemistry but also the localization of the fluorescent proteins across the material surfaces. The resulting photoactive material formed by His-RFP immobilized on graphene hydrogels has been tested as pH indicator to measure pH changes in the alkaline region, although the immobilized fluorescent protein exhibited a narrower dynamic range to measure pH than the soluble fluorescent protein. Likewise, the immobilization of Lys-sGFP on alginate-coated upconverting nanoparticles enabled the infrared excitation of the fluorescent protein to be used as a green light emitter. These novel photoactive biomaterials open new avenues for innovative technological developments towards the fabrication of biosensors and photonic devices. MDPI 2019-07-30 /pmc/articles/PMC6696454/ /pubmed/31366154 http://dx.doi.org/10.3390/molecules24152775 Text en © 2019 by the authors. Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license (http://creativecommons.org/licenses/by/4.0/).
spellingShingle Article
Benítez-Mateos, Ana I.
Mehravar, Ehsan
Velasco-Lozano, Susana
Tomovska, Radmila
Salassa, Luca
López-Gallego, Fernando
Selective Immobilization of Fluorescent Proteins for the Fabrication of Photoactive Materials
title Selective Immobilization of Fluorescent Proteins for the Fabrication of Photoactive Materials
title_full Selective Immobilization of Fluorescent Proteins for the Fabrication of Photoactive Materials
title_fullStr Selective Immobilization of Fluorescent Proteins for the Fabrication of Photoactive Materials
title_full_unstemmed Selective Immobilization of Fluorescent Proteins for the Fabrication of Photoactive Materials
title_short Selective Immobilization of Fluorescent Proteins for the Fabrication of Photoactive Materials
title_sort selective immobilization of fluorescent proteins for the fabrication of photoactive materials
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6696454/
https://www.ncbi.nlm.nih.gov/pubmed/31366154
http://dx.doi.org/10.3390/molecules24152775
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