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Photoreceptor damage induced by low-intensity light: model of retinal degeneration in mammals

PURPOSE: Retinal degeneration caused by a defect in the phototransduction cascade leads to the apoptosis of photoreceptor cells, although the precise molecular mechanism is still unknown. In addition, constant low light exposure produces photoreceptor cell death through the activation of downstream...

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Autores principales: Contín, Maria Ana, Arietti, Milagros M., Benedetto, María M., Bussi, Claudio, Guido, Mario E.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Molecular Vision 2013
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3724958/
https://www.ncbi.nlm.nih.gov/pubmed/23901245
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author Contín, Maria Ana
Arietti, Milagros M.
Benedetto, María M.
Bussi, Claudio
Guido, Mario E.
author_facet Contín, Maria Ana
Arietti, Milagros M.
Benedetto, María M.
Bussi, Claudio
Guido, Mario E.
author_sort Contín, Maria Ana
collection PubMed
description PURPOSE: Retinal degeneration caused by a defect in the phototransduction cascade leads to the apoptosis of photoreceptor cells, although the precise molecular mechanism is still unknown. In addition, constant low light exposure produces photoreceptor cell death through the activation of downstream phototransduction. The authors investigated the time course and molecular mechanisms of death and the rhodopsin phosphorylation occurring during retinal degeneration after exposure to continuous low-intensity light. METHODS: Wistar rats were exposed to constant cool white 200 lx intensity LED light (LL) for one to ten days and compared with animals kept in the dark (DD) or controls exposed to a regular 12:12 h (LD) cycle. One eye from each rat was used for histological and quantitative outer nuclear layer (ONL) analysis and the other for biochemical assays. RESULTS: The histological analysis showed a significant reduction in the ONL of LL-exposed rats after seven days compared with LD- or DD-exposed rats. Retinal analysis by flow cytometer and the TUNEL assay revealed an increase in cell death in the ONL, the in vitro enzymatic activity assay and western blot analysis showing no caspase-3 activation. The rhodopsin analysis demonstrated more phosphorylation in serine 334 residues (Ser(334)) in LL-exposed than in LD- or DD-exposed rats. However, for all times studied, rhodopsin was completely dephosphorylated after four days of DD treatment. CONCLUSIONS: Constant light exposure for seven days produces ONL reduction by photoreceptor cell death through a capase-3-independent mechanism. Increases in rhodopsin-phospho-Ser(334) levels were observed, supporting the notion that changes in the regulation of the phototransduction cascade occur during retinal degeneration.
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spelling pubmed-37249582013-07-30 Photoreceptor damage induced by low-intensity light: model of retinal degeneration in mammals Contín, Maria Ana Arietti, Milagros M. Benedetto, María M. Bussi, Claudio Guido, Mario E. Mol Vis Research Article PURPOSE: Retinal degeneration caused by a defect in the phototransduction cascade leads to the apoptosis of photoreceptor cells, although the precise molecular mechanism is still unknown. In addition, constant low light exposure produces photoreceptor cell death through the activation of downstream phototransduction. The authors investigated the time course and molecular mechanisms of death and the rhodopsin phosphorylation occurring during retinal degeneration after exposure to continuous low-intensity light. METHODS: Wistar rats were exposed to constant cool white 200 lx intensity LED light (LL) for one to ten days and compared with animals kept in the dark (DD) or controls exposed to a regular 12:12 h (LD) cycle. One eye from each rat was used for histological and quantitative outer nuclear layer (ONL) analysis and the other for biochemical assays. RESULTS: The histological analysis showed a significant reduction in the ONL of LL-exposed rats after seven days compared with LD- or DD-exposed rats. Retinal analysis by flow cytometer and the TUNEL assay revealed an increase in cell death in the ONL, the in vitro enzymatic activity assay and western blot analysis showing no caspase-3 activation. The rhodopsin analysis demonstrated more phosphorylation in serine 334 residues (Ser(334)) in LL-exposed than in LD- or DD-exposed rats. However, for all times studied, rhodopsin was completely dephosphorylated after four days of DD treatment. CONCLUSIONS: Constant light exposure for seven days produces ONL reduction by photoreceptor cell death through a capase-3-independent mechanism. Increases in rhodopsin-phospho-Ser(334) levels were observed, supporting the notion that changes in the regulation of the phototransduction cascade occur during retinal degeneration. Molecular Vision 2013-07-25 /pmc/articles/PMC3724958/ /pubmed/23901245 Text en Copyright © 2013 Molecular Vision. http://creativecommons.org/licenses/by/3.0/ 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 work is properly cited.
spellingShingle Research Article
Contín, Maria Ana
Arietti, Milagros M.
Benedetto, María M.
Bussi, Claudio
Guido, Mario E.
Photoreceptor damage induced by low-intensity light: model of retinal degeneration in mammals
title Photoreceptor damage induced by low-intensity light: model of retinal degeneration in mammals
title_full Photoreceptor damage induced by low-intensity light: model of retinal degeneration in mammals
title_fullStr Photoreceptor damage induced by low-intensity light: model of retinal degeneration in mammals
title_full_unstemmed Photoreceptor damage induced by low-intensity light: model of retinal degeneration in mammals
title_short Photoreceptor damage induced by low-intensity light: model of retinal degeneration in mammals
title_sort photoreceptor damage induced by low-intensity light: model of retinal degeneration in mammals
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3724958/
https://www.ncbi.nlm.nih.gov/pubmed/23901245
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