Switching from ultrafast electron transfer to proton transfer in excited drug–protein complexes upon biotransformation

Photosensitization by drugs is directly related with the excited species and the photoinduced processes arising from interaction with UVA light. In this context, the ability of gefitinib (GFT), a tyrosine kinase inhibitor (TKI) used for the treatment of a variety of cancers, to induce phototoxicity...

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Autores principales: Tamarit, Lorena, El Ouardi, Meryem, Lence, Emilio, Andreu, Inmaculada, González-Bello, Concepción, Vayá, Ignacio, Miranda, Miguel A.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: The Royal Society of Chemistry 2022
Materias:
Chemistry
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9400592/
https://www.ncbi.nlm.nih.gov/pubmed/36091919
http://dx.doi.org/10.1039/d2sc03257k
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author Tamarit, Lorena
El Ouardi, Meryem
Lence, Emilio
Andreu, Inmaculada
González-Bello, Concepción
Vayá, Ignacio
Miranda, Miguel A.
author_facet Tamarit, Lorena
El Ouardi, Meryem
Lence, Emilio
Andreu, Inmaculada
González-Bello, Concepción
Vayá, Ignacio
Miranda, Miguel A.
author_sort Tamarit, Lorena
collection PubMed
description Photosensitization by drugs is directly related with the excited species and the photoinduced processes arising from interaction with UVA light. In this context, the ability of gefitinib (GFT), a tyrosine kinase inhibitor (TKI) used for the treatment of a variety of cancers, to induce phototoxicity and photooxidation of proteins has recently been demonstrated. In principle, photodamage can be generated not only by a given drug but also by its photoactive metabolites that maintain the relevant chromophore. In the present work, a complete study of O-desmorpholinopropyl gefitinib (GFT-MB) has been performed by means of fluorescence and ultrafast transient absorption spectroscopies, in addition to molecular dynamics (MD) simulations. The photobehavior of the GFT-MB metabolite in solution is similar to that of GFT. However, when the drug or its metabolite are in a constrained environment, i.e. within a protein, their behavior and the photoinduced processes that arise from their interaction with UVA light are completely different. For GFT in complex with human serum albumin (HSA), locally excited (LE) singlet states are mainly formed; these species undergo photoinduced electron transfer with Tyr and Trp. By contrast, since GFT-MB is a phenol, excited state proton transfer (ESPT) to form phenolate-like excited species might become an alternative deactivation pathway. As a matter of fact, the protein-bound metabolite exhibits higher fluorescence yields and longer emission wavelengths and lifetimes than GFT@HSA. Ultrafast transient absorption measurements support direct ESPT deprotonation of LE states (rather than ICT), to form phenolate-like species. This is explained by MD simulations, which reveal a close interaction between the phenolic OH group of GFT-MB and Val116 within site 3 (subdomain IB) of HSA. The reported findings are relevant to understand the photosensitizing properties of TKIs and the role of biotransformation in this type of adverse side effects.
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spelling pubmed-94005922022-09-08 Switching from ultrafast electron transfer to proton transfer in excited drug–protein complexes upon biotransformation Tamarit, Lorena El Ouardi, Meryem Lence, Emilio Andreu, Inmaculada González-Bello, Concepción Vayá, Ignacio Miranda, Miguel A. Chem Sci Chemistry Photosensitization by drugs is directly related with the excited species and the photoinduced processes arising from interaction with UVA light. In this context, the ability of gefitinib (GFT), a tyrosine kinase inhibitor (TKI) used for the treatment of a variety of cancers, to induce phototoxicity and photooxidation of proteins has recently been demonstrated. In principle, photodamage can be generated not only by a given drug but also by its photoactive metabolites that maintain the relevant chromophore. In the present work, a complete study of O-desmorpholinopropyl gefitinib (GFT-MB) has been performed by means of fluorescence and ultrafast transient absorption spectroscopies, in addition to molecular dynamics (MD) simulations. The photobehavior of the GFT-MB metabolite in solution is similar to that of GFT. However, when the drug or its metabolite are in a constrained environment, i.e. within a protein, their behavior and the photoinduced processes that arise from their interaction with UVA light are completely different. For GFT in complex with human serum albumin (HSA), locally excited (LE) singlet states are mainly formed; these species undergo photoinduced electron transfer with Tyr and Trp. By contrast, since GFT-MB is a phenol, excited state proton transfer (ESPT) to form phenolate-like excited species might become an alternative deactivation pathway. As a matter of fact, the protein-bound metabolite exhibits higher fluorescence yields and longer emission wavelengths and lifetimes than GFT@HSA. Ultrafast transient absorption measurements support direct ESPT deprotonation of LE states (rather than ICT), to form phenolate-like species. This is explained by MD simulations, which reveal a close interaction between the phenolic OH group of GFT-MB and Val116 within site 3 (subdomain IB) of HSA. The reported findings are relevant to understand the photosensitizing properties of TKIs and the role of biotransformation in this type of adverse side effects. The Royal Society of Chemistry 2022-08-02 /pmc/articles/PMC9400592/ /pubmed/36091919 http://dx.doi.org/10.1039/d2sc03257k Text en This journal is © The Royal Society of Chemistry https://creativecommons.org/licenses/by-nc/3.0/
spellingShingle Chemistry
Tamarit, Lorena
El Ouardi, Meryem
Lence, Emilio
Andreu, Inmaculada
González-Bello, Concepción
Vayá, Ignacio
Miranda, Miguel A.
Switching from ultrafast electron transfer to proton transfer in excited drug–protein complexes upon biotransformation
title Switching from ultrafast electron transfer to proton transfer in excited drug–protein complexes upon biotransformation
title_full Switching from ultrafast electron transfer to proton transfer in excited drug–protein complexes upon biotransformation
title_fullStr Switching from ultrafast electron transfer to proton transfer in excited drug–protein complexes upon biotransformation
title_full_unstemmed Switching from ultrafast electron transfer to proton transfer in excited drug–protein complexes upon biotransformation
title_short Switching from ultrafast electron transfer to proton transfer in excited drug–protein complexes upon biotransformation
title_sort switching from ultrafast electron transfer to proton transfer in excited drug–protein complexes upon biotransformation
topic Chemistry
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9400592/
https://www.ncbi.nlm.nih.gov/pubmed/36091919
http://dx.doi.org/10.1039/d2sc03257k
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