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Development of Singlet Oxygen Luminescence Kinetics during the Photodynamic Inactivation of Green Algae

Recent studies show the feasibility of photodynamic inactivation of green algae as a vital step towards an effective photodynamic suppression of biofilms by using functionalized surfaces. The investigation of the intrinsic mechanisms of photodynamic inactivation in green algae represents the next st...

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Autores principales: Bornhütter, Tobias, Pohl, Judith, Fischer, Christian, Saltsman, Irena, Mahammed, Atif, Gross, Zeev, Röder, Beate
Formato: Online Artículo Texto
Lenguaje:English
Publicado: MDPI 2016
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6272977/
https://www.ncbi.nlm.nih.gov/pubmed/27089311
http://dx.doi.org/10.3390/molecules21040485
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author Bornhütter, Tobias
Pohl, Judith
Fischer, Christian
Saltsman, Irena
Mahammed, Atif
Gross, Zeev
Röder, Beate
author_facet Bornhütter, Tobias
Pohl, Judith
Fischer, Christian
Saltsman, Irena
Mahammed, Atif
Gross, Zeev
Röder, Beate
author_sort Bornhütter, Tobias
collection PubMed
description Recent studies show the feasibility of photodynamic inactivation of green algae as a vital step towards an effective photodynamic suppression of biofilms by using functionalized surfaces. The investigation of the intrinsic mechanisms of photodynamic inactivation in green algae represents the next step in order to determine optimization parameters. The observation of singlet oxygen luminescence kinetics proved to be a very effective approach towards understanding mechanisms on a cellular level. In this study, the first two-dimensional measurement of singlet oxygen kinetics in phototrophic microorganisms on surfaces during photodynamic inactivation is presented. We established a system of reproducible algae samples on surfaces, incubated with two different cationic, antimicrobial potent photosensitizers. Fluorescence microscopy images indicate that one photosensitizer localizes inside the green algae while the other accumulates along the outer algae cell wall. A newly developed setup allows for the measurement of singlet oxygen luminescence on the green algae sample surfaces over several days. The kinetics of the singlet oxygen luminescence of both photosensitizers show different developments and a distinct change over time, corresponding with the differences in their localization as well as their photosensitization potential. While the complexity of the signal reveals a challenge for the future, this study incontrovertibly marks a crucial, inevitable step in the investigation of photodynamic inactivation of biofilms: it shows the feasibility of using the singlet oxygen luminescence kinetics to investigate photodynamic effects on surfaces and thus opens a field for numerous investigations.
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spelling pubmed-62729772018-12-28 Development of Singlet Oxygen Luminescence Kinetics during the Photodynamic Inactivation of Green Algae Bornhütter, Tobias Pohl, Judith Fischer, Christian Saltsman, Irena Mahammed, Atif Gross, Zeev Röder, Beate Molecules Article Recent studies show the feasibility of photodynamic inactivation of green algae as a vital step towards an effective photodynamic suppression of biofilms by using functionalized surfaces. The investigation of the intrinsic mechanisms of photodynamic inactivation in green algae represents the next step in order to determine optimization parameters. The observation of singlet oxygen luminescence kinetics proved to be a very effective approach towards understanding mechanisms on a cellular level. In this study, the first two-dimensional measurement of singlet oxygen kinetics in phototrophic microorganisms on surfaces during photodynamic inactivation is presented. We established a system of reproducible algae samples on surfaces, incubated with two different cationic, antimicrobial potent photosensitizers. Fluorescence microscopy images indicate that one photosensitizer localizes inside the green algae while the other accumulates along the outer algae cell wall. A newly developed setup allows for the measurement of singlet oxygen luminescence on the green algae sample surfaces over several days. The kinetics of the singlet oxygen luminescence of both photosensitizers show different developments and a distinct change over time, corresponding with the differences in their localization as well as their photosensitization potential. While the complexity of the signal reveals a challenge for the future, this study incontrovertibly marks a crucial, inevitable step in the investigation of photodynamic inactivation of biofilms: it shows the feasibility of using the singlet oxygen luminescence kinetics to investigate photodynamic effects on surfaces and thus opens a field for numerous investigations. MDPI 2016-04-13 /pmc/articles/PMC6272977/ /pubmed/27089311 http://dx.doi.org/10.3390/molecules21040485 Text en © 2016 by the authors. Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons by Attribution (CC-BY) license (http://creativecommons.org/licenses/by/4.0/).
spellingShingle Article
Bornhütter, Tobias
Pohl, Judith
Fischer, Christian
Saltsman, Irena
Mahammed, Atif
Gross, Zeev
Röder, Beate
Development of Singlet Oxygen Luminescence Kinetics during the Photodynamic Inactivation of Green Algae
title Development of Singlet Oxygen Luminescence Kinetics during the Photodynamic Inactivation of Green Algae
title_full Development of Singlet Oxygen Luminescence Kinetics during the Photodynamic Inactivation of Green Algae
title_fullStr Development of Singlet Oxygen Luminescence Kinetics during the Photodynamic Inactivation of Green Algae
title_full_unstemmed Development of Singlet Oxygen Luminescence Kinetics during the Photodynamic Inactivation of Green Algae
title_short Development of Singlet Oxygen Luminescence Kinetics during the Photodynamic Inactivation of Green Algae
title_sort development of singlet oxygen luminescence kinetics during the photodynamic inactivation of green algae
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC6272977/
https://www.ncbi.nlm.nih.gov/pubmed/27089311
http://dx.doi.org/10.3390/molecules21040485
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