A Novel Organ Culture Model to Quantify Collagen Remodeling in Tree Shrew Sclera

Increasing evidence suggests that unknown collagen remodeling mechanisms in the sclera underlie myopia development. We are proposing a novel organ culture system in combination with two-photon fluorescence imaging to quantify collagen remodeling at the tissue- and lamella-level. Tree shrew scleral s...

Descripción completa

Detalles Bibliográficos
Autores principales: Baldivia, Sarah, Levy, Alexander, Hegde, Shylaja, Aper, Stijn J. A., Merkx, Maarten, Grytz, Rafael
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2016
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5117658/
https://www.ncbi.nlm.nih.gov/pubmed/27870875
http://dx.doi.org/10.1371/journal.pone.0166644
_version_ 1782468843673747456
author Baldivia, Sarah
Levy, Alexander
Hegde, Shylaja
Aper, Stijn J. A.
Merkx, Maarten
Grytz, Rafael
author_facet Baldivia, Sarah
Levy, Alexander
Hegde, Shylaja
Aper, Stijn J. A.
Merkx, Maarten
Grytz, Rafael
author_sort Baldivia, Sarah
collection PubMed
description Increasing evidence suggests that unknown collagen remodeling mechanisms in the sclera underlie myopia development. We are proposing a novel organ culture system in combination with two-photon fluorescence imaging to quantify collagen remodeling at the tissue- and lamella-level. Tree shrew scleral shells were cultured up to 7 days in serum-free media and cellular viability was investigated under: (i) minimal tissue manipulations; (ii) removal of intraocular tissues; gluing the eye to a washer using (iii) 50 μL and (iv) 200 μL of cyanoacrylate adhesive; (v) supplementing media with Ham's F-12 Nutrient Mixture; and (vi) culturing eyes subjected to 15 mmHg intraocular pressure in our new bioreactor. Two scleral shells of normal juvenile tree shrews were fluorescently labeled using a collagen specific protein and cultured in our bioreactor. Using two-photon microscopy, grid patterns were photobleached into and across multiple scleral lamellae. These patterns were imaged daily for 3 days, and tissue-/lamella-level strains were calculated from the deformed patterns. No significant reduction in cell viability was observed under conditions (i) and (v). Compared to condition (i), cell viability was significantly reduced starting at day 0 (condition (ii)) and day 3 (conditions (iii, iv, vi)). Tissue-level strain and intralamellar shear angel increased significantly during the culture period. Some scleral lamellae elongated while others shortened. Findings suggest that tree shrew sclera can be cultured in serum-free media for 7 days with no significant reduction in cell viability. Scleral fibroblasts are sensitive to tissue manipulations and tissue gluing. However, Ham's F-12 Nutrient Mixture has a protective effect on cell viability and can offset the cytotoxic effect of cyanoacrylate adhesive. This is the first study to quantify collagen micro-deformations over a prolonged period in organ culture providing a new methodology to study scleral remodeling in myopia.
format Online
Article
Text
id pubmed-5117658
institution National Center for Biotechnology Information
language English
publishDate 2016
publisher Public Library of Science
record_format MEDLINE/PubMed
spelling pubmed-51176582016-12-15 A Novel Organ Culture Model to Quantify Collagen Remodeling in Tree Shrew Sclera Baldivia, Sarah Levy, Alexander Hegde, Shylaja Aper, Stijn J. A. Merkx, Maarten Grytz, Rafael PLoS One Research Article Increasing evidence suggests that unknown collagen remodeling mechanisms in the sclera underlie myopia development. We are proposing a novel organ culture system in combination with two-photon fluorescence imaging to quantify collagen remodeling at the tissue- and lamella-level. Tree shrew scleral shells were cultured up to 7 days in serum-free media and cellular viability was investigated under: (i) minimal tissue manipulations; (ii) removal of intraocular tissues; gluing the eye to a washer using (iii) 50 μL and (iv) 200 μL of cyanoacrylate adhesive; (v) supplementing media with Ham's F-12 Nutrient Mixture; and (vi) culturing eyes subjected to 15 mmHg intraocular pressure in our new bioreactor. Two scleral shells of normal juvenile tree shrews were fluorescently labeled using a collagen specific protein and cultured in our bioreactor. Using two-photon microscopy, grid patterns were photobleached into and across multiple scleral lamellae. These patterns were imaged daily for 3 days, and tissue-/lamella-level strains were calculated from the deformed patterns. No significant reduction in cell viability was observed under conditions (i) and (v). Compared to condition (i), cell viability was significantly reduced starting at day 0 (condition (ii)) and day 3 (conditions (iii, iv, vi)). Tissue-level strain and intralamellar shear angel increased significantly during the culture period. Some scleral lamellae elongated while others shortened. Findings suggest that tree shrew sclera can be cultured in serum-free media for 7 days with no significant reduction in cell viability. Scleral fibroblasts are sensitive to tissue manipulations and tissue gluing. However, Ham's F-12 Nutrient Mixture has a protective effect on cell viability and can offset the cytotoxic effect of cyanoacrylate adhesive. This is the first study to quantify collagen micro-deformations over a prolonged period in organ culture providing a new methodology to study scleral remodeling in myopia. Public Library of Science 2016-11-21 /pmc/articles/PMC5117658/ /pubmed/27870875 http://dx.doi.org/10.1371/journal.pone.0166644 Text en © 2016 Baldivia 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 (http://creativecommons.org/licenses/by/4.0/) , which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
spellingShingle Research Article
Baldivia, Sarah
Levy, Alexander
Hegde, Shylaja
Aper, Stijn J. A.
Merkx, Maarten
Grytz, Rafael
A Novel Organ Culture Model to Quantify Collagen Remodeling in Tree Shrew Sclera
title A Novel Organ Culture Model to Quantify Collagen Remodeling in Tree Shrew Sclera
title_full A Novel Organ Culture Model to Quantify Collagen Remodeling in Tree Shrew Sclera
title_fullStr A Novel Organ Culture Model to Quantify Collagen Remodeling in Tree Shrew Sclera
title_full_unstemmed A Novel Organ Culture Model to Quantify Collagen Remodeling in Tree Shrew Sclera
title_short A Novel Organ Culture Model to Quantify Collagen Remodeling in Tree Shrew Sclera
title_sort novel organ culture model to quantify collagen remodeling in tree shrew sclera
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5117658/
https://www.ncbi.nlm.nih.gov/pubmed/27870875
http://dx.doi.org/10.1371/journal.pone.0166644
work_keys_str_mv AT baldiviasarah anovelorganculturemodeltoquantifycollagenremodelingintreeshrewsclera
AT levyalexander anovelorganculturemodeltoquantifycollagenremodelingintreeshrewsclera
AT hegdeshylaja anovelorganculturemodeltoquantifycollagenremodelingintreeshrewsclera
AT aperstijnja anovelorganculturemodeltoquantifycollagenremodelingintreeshrewsclera
AT merkxmaarten anovelorganculturemodeltoquantifycollagenremodelingintreeshrewsclera
AT grytzrafael anovelorganculturemodeltoquantifycollagenremodelingintreeshrewsclera
AT baldiviasarah novelorganculturemodeltoquantifycollagenremodelingintreeshrewsclera
AT levyalexander novelorganculturemodeltoquantifycollagenremodelingintreeshrewsclera
AT hegdeshylaja novelorganculturemodeltoquantifycollagenremodelingintreeshrewsclera
AT aperstijnja novelorganculturemodeltoquantifycollagenremodelingintreeshrewsclera
AT merkxmaarten novelorganculturemodeltoquantifycollagenremodelingintreeshrewsclera
AT grytzrafael novelorganculturemodeltoquantifycollagenremodelingintreeshrewsclera

Ejemplares similares