Dynamics and Flexibility of Human Aromatase Probed by FTIR and Time Resolved Fluorescence Spectroscopy

Human aromatase (CYP19A1) is a steroidogenic cytochrome P450 converting androgens into estrogens. No ligand-free crystal structure of the enzyme is available to date. The crystal structure in complex with the substrate androstenedione and the steroidal inhibitor exemestane shows a very compact confo...

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Autores principales: Di Nardo, Giovanna, Breitner, Maximilian, Sadeghi, Sheila J., Castrignanò, Silvia, Mei, Giampiero, Di Venere, Almerinda, Nicolai, Eleonora, Allegra, Paola, Gilardi, Gianfranco
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2013
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Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3859599/
https://www.ncbi.nlm.nih.gov/pubmed/24349198
http://dx.doi.org/10.1371/journal.pone.0082118
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author Di Nardo, Giovanna
Breitner, Maximilian
Sadeghi, Sheila J.
Castrignanò, Silvia
Mei, Giampiero
Di Venere, Almerinda
Nicolai, Eleonora
Allegra, Paola
Gilardi, Gianfranco
author_facet Di Nardo, Giovanna
Breitner, Maximilian
Sadeghi, Sheila J.
Castrignanò, Silvia
Mei, Giampiero
Di Venere, Almerinda
Nicolai, Eleonora
Allegra, Paola
Gilardi, Gianfranco
author_sort Di Nardo, Giovanna
collection PubMed
description Human aromatase (CYP19A1) is a steroidogenic cytochrome P450 converting androgens into estrogens. No ligand-free crystal structure of the enzyme is available to date. The crystal structure in complex with the substrate androstenedione and the steroidal inhibitor exemestane shows a very compact conformation of the enzyme, leaving unanswered questions on the conformational changes that must occur to allow access of the ligand to the active site. As H/D exchange kinetics followed by FTIR spectroscopy can provide information on the conformational changes in proteins where solvent accessibility is affected, here the amide I region was used to measure the exchange rates of the different elements of the secondary structure for aromatase in the ligand-free form and in the presence of the substrate androstenedione and the inhibitor anastrozole. Biphasic exponential functions were found to fit the H/D exchange data collected as a function of time. Two exchange rates were assigned to two populations of protons present in different flexible regions of the protein. The addition of the substrate androstenedione and the inhibitor anastrozole lowers the H/D exchange rates of the α-helices of the enzyme when compared to the ligand-free form. Furthermore, the presence of the inhibitor anastrozole lowers exchange rate constant (k(1)) for β-sheets from 0.22±0.06 min(−1) for the inhibitor-bound enzyme to 0.12±0.02 min(−1) for the free protein. Dynamics effects localised in helix F were studied by time resolved fluorescence. The data demonstrate that the fluorescence lifetime component associated to Trp224 emission undergoes a shift toward longer lifetimes (from ≈5.0 to ≈5.5 ns) when the substrate or the inhibitor are present, suggesting slower dynamics in the presence of ligands. Together the results are consistent with different degrees of flexibility of the access channel and therefore different conformations adopted by the enzyme in the free, substrate- and inhibitor-bound forms.
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spelling pubmed-38595992013-12-13 Dynamics and Flexibility of Human Aromatase Probed by FTIR and Time Resolved Fluorescence Spectroscopy Di Nardo, Giovanna Breitner, Maximilian Sadeghi, Sheila J. Castrignanò, Silvia Mei, Giampiero Di Venere, Almerinda Nicolai, Eleonora Allegra, Paola Gilardi, Gianfranco PLoS One Research Article Human aromatase (CYP19A1) is a steroidogenic cytochrome P450 converting androgens into estrogens. No ligand-free crystal structure of the enzyme is available to date. The crystal structure in complex with the substrate androstenedione and the steroidal inhibitor exemestane shows a very compact conformation of the enzyme, leaving unanswered questions on the conformational changes that must occur to allow access of the ligand to the active site. As H/D exchange kinetics followed by FTIR spectroscopy can provide information on the conformational changes in proteins where solvent accessibility is affected, here the amide I region was used to measure the exchange rates of the different elements of the secondary structure for aromatase in the ligand-free form and in the presence of the substrate androstenedione and the inhibitor anastrozole. Biphasic exponential functions were found to fit the H/D exchange data collected as a function of time. Two exchange rates were assigned to two populations of protons present in different flexible regions of the protein. The addition of the substrate androstenedione and the inhibitor anastrozole lowers the H/D exchange rates of the α-helices of the enzyme when compared to the ligand-free form. Furthermore, the presence of the inhibitor anastrozole lowers exchange rate constant (k(1)) for β-sheets from 0.22±0.06 min(−1) for the inhibitor-bound enzyme to 0.12±0.02 min(−1) for the free protein. Dynamics effects localised in helix F were studied by time resolved fluorescence. The data demonstrate that the fluorescence lifetime component associated to Trp224 emission undergoes a shift toward longer lifetimes (from ≈5.0 to ≈5.5 ns) when the substrate or the inhibitor are present, suggesting slower dynamics in the presence of ligands. Together the results are consistent with different degrees of flexibility of the access channel and therefore different conformations adopted by the enzyme in the free, substrate- and inhibitor-bound forms. Public Library of Science 2013-12-11 /pmc/articles/PMC3859599/ /pubmed/24349198 http://dx.doi.org/10.1371/journal.pone.0082118 Text en © 2013 Di Nardo et al http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Di Nardo, Giovanna
Breitner, Maximilian
Sadeghi, Sheila J.
Castrignanò, Silvia
Mei, Giampiero
Di Venere, Almerinda
Nicolai, Eleonora
Allegra, Paola
Gilardi, Gianfranco
Dynamics and Flexibility of Human Aromatase Probed by FTIR and Time Resolved Fluorescence Spectroscopy
title Dynamics and Flexibility of Human Aromatase Probed by FTIR and Time Resolved Fluorescence Spectroscopy
title_full Dynamics and Flexibility of Human Aromatase Probed by FTIR and Time Resolved Fluorescence Spectroscopy
title_fullStr Dynamics and Flexibility of Human Aromatase Probed by FTIR and Time Resolved Fluorescence Spectroscopy
title_full_unstemmed Dynamics and Flexibility of Human Aromatase Probed by FTIR and Time Resolved Fluorescence Spectroscopy
title_short Dynamics and Flexibility of Human Aromatase Probed by FTIR and Time Resolved Fluorescence Spectroscopy
title_sort dynamics and flexibility of human aromatase probed by ftir and time resolved fluorescence spectroscopy
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3859599/
https://www.ncbi.nlm.nih.gov/pubmed/24349198
http://dx.doi.org/10.1371/journal.pone.0082118
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