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Modulation of the photobehavior of gefitinib and its phenolic metabolites by human transport proteins

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Modulation of the photobehavior of gefitinib and its phenolic metabolites by human transport proteins

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dc.contributor.author Tamarit-Mayo, Lorena es_ES
dc.contributor.author El Ouardi, Meryem es_ES
dc.contributor.author Lence, Emilio es_ES
dc.contributor.author Andreu, Inmaculada es_ES
dc.contributor.author González-Bello, Concepción es_ES
dc.contributor.author Miranda Alonso, Miguel Ángel es_ES
dc.contributor.author Vayá Pérez, Ignacio es_ES
dc.date.accessioned 2024-11-14T19:13:19Z
dc.date.available 2024-11-14T19:13:19Z
dc.date.issued 2024-05-16 es_ES
dc.identifier.uri http://hdl.handle.net/10251/211802
dc.description.abstract [EN] The photobiological damage that certain drugs or their metabolites can photosensitize in proteins is generally associated with the nature of the excited species that are generated upon interaction with UVA light. In this regard, the photoinduced damage of the anticancer drug gefitinib (GFT) and its two main photoactive metabolites GFT-M1 and GFT-M2 in cellular milieu was recently investigated. With this background, the photophysical properties of both the drug and its metabolites have now been studied in the presence of the two main transport proteins of human plasma, i.e., serum albumin (HSA) and ¿1-acid glycoprotein (HAG) upon UVA light excitation. In general, the observed photobehavior was strongly affected by the confined environment provided by the protein. Thus, GFT-M1 (which exhibits the highest phototoxicity) showed the highest fluorescence yield arising from long-lived HSA-bound phenolate-like excited species. Conversely, locally excited (LE) states were formed within HAG, resulting in lower fluorescence yields. The reserve was true for GFT-M2, which despite being also a phenol, led mainly to formation of LE states within HSA, and phenolate-like species (with a minor contribution of LE) inside HAG. Finally, the parent drug GFT, which is known to form LE states within HSA, exhibited a parallel behavior in the two proteins. In addition, determination of the association constants by both absorption and emission spectroscopy revealed that the two metabolites bind stronger to HSA than the parent drug, whereas smaller differences were observed for HAG. This was further confirmed by studying the competing interactions between GFT or its metabolites with the two proteins using fluorescence measurements. These above experimental findings were satisfactorily correlated with the results obtained by means of molecular dynamics (MD) simulations, which revealed the high affinity binding sites, the strength of interactions and the involved amino acid residues. In general, the differences observed in the photobehavior of the drug and its two photoactive metabolites in protein media are consistent with their relative photosensitizing potentials. es_ES
dc.description.sponsorship The Ministry of Science, Innovation and Universities of Spain, the Conselleria d'Innovacio, Universitats, Ciencia i Societat Digital, the University of Valencia, the Health Research Institute Hospital La Fe (IIS La Fe) and La Xunta de Galicia are gratefully acknowledged for financial support. All authors are grateful to the Centro de Supercomputacion de Galicia (CESGA) for use of the Finis Terrae computer.The author(s) declare that financial support was received for the research, authorship, and/or publication of this article. Grants PID2020-115010RB-I00 and PID2022-136963OB-I00 funded by MCIN/AEI/10.13039/501100011033, grant CIAICO/2021/061 funded by Conselleria d'Innovacio, Universitats, Ciencia i Societat Digital and grant AP2022-5 funded by Programa d'Accions Preparatories UV-La Fe. Grants from the Xunta de Galicia [ED431C 2021/29 and the Centro singular de investigacion de Galicia accreditation 2019-2022 (ED431G 2019/03), CG-B], and the European Regional Development Fund (ERDF). es_ES
dc.language Inglés es_ES
dc.publisher Frontiers Media SA es_ES
dc.relation.ispartof Frontiers in Pharmacology es_ES
dc.rights Reconocimiento (by) es_ES
dc.subject Anticancer drugs es_ES
dc.subject Fluorescence es_ES
dc.subject Metabolites es_ES
dc.subject Molecular dynamics es_ES
dc.subject Protein binding constants es_ES
dc.subject.classification QUIMICA ORGANICA es_ES
dc.title Modulation of the photobehavior of gefitinib and its phenolic metabolites by human transport proteins es_ES
dc.type Artículo es_ES
dc.identifier.doi 10.3389/fphar.2024.1387057 es_ES
dc.relation.projectID info:eu-repo/grantAgreement/AEI/Plan Estatal de Investigación Científica y Técnica y de Innovación 2021-2023/PID2022-136963OB-I00/ES/NUEVOS AGENTES ANTIBACTERIANOS DE PRECISION Y TERAPIAS COMBINADAS PARA COMBATIR INFECCIONES MULTIRRESISTENTES/ es_ES
dc.relation.projectID info:eu-repo/grantAgreement/AGENCIA ESTATAL DE INVESTIGACION//PID2020-115010RB-I00//FOTOCOMPORTAMIENTO DE LOS INHIBIDORES DE LA TIROSINA QUINASA: DE DISOLUCION A CELULAS/ es_ES
dc.relation.projectID info:eu-repo/grantAgreement/Conselleria de Innovación, Universidades, Ciencia y Sociedad Digital, Generalitat Valenciana//CIAICO%2F2021%2F061//Sunscreen-based photocages/ es_ES
dc.relation.projectID info:eu-repo/grantAgreement/Xunta de Galicia//ED431C 2021%2F29 / es_ES
dc.relation.projectID info:eu-repo/grantAgreement/Xunta de Galicia//ED431G 2019%2F03/ es_ES
dc.relation.projectID info:eu-repo/grantAgreement/GVA//AP2022-5/ es_ES
dc.rights.accessRights Abierto es_ES
dc.contributor.affiliation Universitat Politècnica de València. Escuela Técnica Superior de Ingenieros Industriales - Escola Tècnica Superior d'Enginyers Industrials es_ES
dc.contributor.affiliation Universitat Politècnica de València. Instituto Universitario Mixto de Tecnología Química - Institut Universitari Mixt de Tecnologia Química es_ES
dc.description.bibliographicCitation Tamarit-Mayo, L.; El Ouardi, M.; Lence, E.; Andreu, I.; González-Bello, C.; Miranda Alonso, MÁ.; Vayá Pérez, I. (2024). Modulation of the photobehavior of gefitinib and its phenolic metabolites by human transport proteins. Frontiers in Pharmacology. 15. https://doi.org/10.3389/fphar.2024.1387057 es_ES
dc.description.accrualMethod S es_ES
dc.relation.publisherversion https://doi.org/10.3389/fphar.2024.1387057 es_ES
dc.type.version info:eu-repo/semantics/publishedVersion es_ES
dc.description.volume 15 es_ES
dc.identifier.eissn 1663-9812 es_ES
dc.identifier.pmid 38818381 es_ES
dc.identifier.pmcid PMC11137198 es_ES
dc.relation.pasarela S\519967 es_ES
dc.contributor.funder Xunta de Galicia es_ES
dc.contributor.funder Generalitat Valenciana es_ES
dc.contributor.funder AGENCIA ESTATAL DE INVESTIGACION es_ES
dc.contributor.funder Agencia Estatal de Investigación es_ES
dc.contributor.funder European Regional Development Fund es_ES
dc.contributor.funder Conselleria de Innovación, Universidades, Ciencia y Sociedad Digital, Generalitat Valenciana es_ES
upv.costeAPC 4000 es_ES


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