Donor cornea transfer from Optisol GS to organ culture storage: a two-step procedure to increase donor tissue lifespan

PURPOSE: Storage time for donor corneas in Optisol GS is limited compared to Eye Bank Organ Culture (EBOC). We here examine the epithelium on donor corneoscleral rims after primary storage in Optisol GS and subsequent incubation in EBOC. METHODS: Morphology was monitored by light and electron micros...

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Autores principales: Haug, Kristiane, Azqueta, Amaya, Johnsen-Soriano, Siv, Shahdadfar, Aboulghassem, Drolsum, Liv K, Moe, Morten C, Røger, Magnus T, Romero, Francisco J, Collins, Andrew R, Nicolaissen, Bjørn
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Blackwell Publishing Ltd 2013
Materias:
Original Articles
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3652042/
https://www.ncbi.nlm.nih.gov/pubmed/22429721
http://dx.doi.org/10.1111/j.1755-3768.2012.02390.x
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author Haug, Kristiane
Azqueta, Amaya
Johnsen-Soriano, Siv
Shahdadfar, Aboulghassem
Drolsum, Liv K
Moe, Morten C
Røger, Magnus T
Romero, Francisco J
Collins, Andrew R
Nicolaissen, Bjørn
author_facet Haug, Kristiane
Azqueta, Amaya
Johnsen-Soriano, Siv
Shahdadfar, Aboulghassem
Drolsum, Liv K
Moe, Morten C
Røger, Magnus T
Romero, Francisco J
Collins, Andrew R
Nicolaissen, Bjørn
author_sort Haug, Kristiane
collection PubMed
description PURPOSE: Storage time for donor corneas in Optisol GS is limited compared to Eye Bank Organ Culture (EBOC). We here examine the epithelium on donor corneoscleral rims after primary storage in Optisol GS and subsequent incubation in EBOC. METHODS: Morphology was monitored by light and electron microscopy, expression of phenotypic and genotypic markers by immunohistochemistry and RT-PCR and changes in oxidative lipid and DNA damage by ELISA and COMET assay. RESULTS: A prominent loss of cells was observed after storage in Optisol GS. After maintenance in EBOC, spreading apical cells were Occludin(+), while the staining for E-cadherin and Connexin-43 was less intense. There were an upregulation of Occludin and a downregulation of E-cadherin and Connexin-43. Eye Bank Organ Culture was associated with an ongoing proliferative activity and a downregulation of putative progenitor/stem cell marker ABCG2 and p63. Staining for 8-OHdG and Caspase-3 did not increase, while levels of malondialdehyde and number of DNA strand breaks and oxidized bases increased. CONCLUSIONS: This dual procedure should be pursued as an option to increase the storage time and the pool of available donor corneas. The observed downregulation of markers associated with stemness during EBOC is relevant considering the potential use of donor epithelium in the treatment of ocular surface disorders.
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spelling pubmed-36520422013-05-13 Donor cornea transfer from Optisol GS to organ culture storage: a two-step procedure to increase donor tissue lifespan Haug, Kristiane Azqueta, Amaya Johnsen-Soriano, Siv Shahdadfar, Aboulghassem Drolsum, Liv K Moe, Morten C Røger, Magnus T Romero, Francisco J Collins, Andrew R Nicolaissen, Bjørn Acta Ophthalmol Original Articles PURPOSE: Storage time for donor corneas in Optisol GS is limited compared to Eye Bank Organ Culture (EBOC). We here examine the epithelium on donor corneoscleral rims after primary storage in Optisol GS and subsequent incubation in EBOC. METHODS: Morphology was monitored by light and electron microscopy, expression of phenotypic and genotypic markers by immunohistochemistry and RT-PCR and changes in oxidative lipid and DNA damage by ELISA and COMET assay. RESULTS: A prominent loss of cells was observed after storage in Optisol GS. After maintenance in EBOC, spreading apical cells were Occludin(+), while the staining for E-cadherin and Connexin-43 was less intense. There were an upregulation of Occludin and a downregulation of E-cadherin and Connexin-43. Eye Bank Organ Culture was associated with an ongoing proliferative activity and a downregulation of putative progenitor/stem cell marker ABCG2 and p63. Staining for 8-OHdG and Caspase-3 did not increase, while levels of malondialdehyde and number of DNA strand breaks and oxidized bases increased. CONCLUSIONS: This dual procedure should be pursued as an option to increase the storage time and the pool of available donor corneas. The observed downregulation of markers associated with stemness during EBOC is relevant considering the potential use of donor epithelium in the treatment of ocular surface disorders. Blackwell Publishing Ltd 2013-05 /pmc/articles/PMC3652042/ /pubmed/22429721 http://dx.doi.org/10.1111/j.1755-3768.2012.02390.x Text en © 2012 The Authors. Acta Ophthalmologica © 2012 Acta Ophthalmologica Scandinavica Foundation http://creativecommons.org/licenses/by/2.5/ Re-use of this article is permitted in accordance with the Creative Commons Deed, Attribution 2.5, which does not permit commercial exploitation.
spellingShingle Original Articles
Haug, Kristiane
Azqueta, Amaya
Johnsen-Soriano, Siv
Shahdadfar, Aboulghassem
Drolsum, Liv K
Moe, Morten C
Røger, Magnus T
Romero, Francisco J
Collins, Andrew R
Nicolaissen, Bjørn
Donor cornea transfer from Optisol GS to organ culture storage: a two-step procedure to increase donor tissue lifespan
title Donor cornea transfer from Optisol GS to organ culture storage: a two-step procedure to increase donor tissue lifespan
title_full Donor cornea transfer from Optisol GS to organ culture storage: a two-step procedure to increase donor tissue lifespan
title_fullStr Donor cornea transfer from Optisol GS to organ culture storage: a two-step procedure to increase donor tissue lifespan
title_full_unstemmed Donor cornea transfer from Optisol GS to organ culture storage: a two-step procedure to increase donor tissue lifespan
title_short Donor cornea transfer from Optisol GS to organ culture storage: a two-step procedure to increase donor tissue lifespan
title_sort donor cornea transfer from optisol gs to organ culture storage: a two-step procedure to increase donor tissue lifespan
topic Original Articles
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3652042/
https://www.ncbi.nlm.nih.gov/pubmed/22429721
http://dx.doi.org/10.1111/j.1755-3768.2012.02390.x
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