Fish Scale-Derived Scaffolds for Culturing Human Corneal Endothelial Cells

PURPOSE: To investigate the biocompatibility of fish scale-derived scaffolds (FSS) with primary human corneal endothelial cells (HCEnCs). METHODS: HCEnCs were isolated from 30 donor corneas in a donor-matched study and plated in precoated Lab-Tek slides (n = 15) and FSS (n = 15). Cell morphology, pr...

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Autores principales: Parekh, Mohit, Van den Bogerd, Bert, Zakaria, Nadia, Ponzin, Diego, Ferrari, Stefano
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Hindawi 2018
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5949177/
https://www.ncbi.nlm.nih.gov/pubmed/29853917
http://dx.doi.org/10.1155/2018/8146834
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author Parekh, Mohit
Van den Bogerd, Bert
Zakaria, Nadia
Ponzin, Diego
Ferrari, Stefano
author_facet Parekh, Mohit
Van den Bogerd, Bert
Zakaria, Nadia
Ponzin, Diego
Ferrari, Stefano
author_sort Parekh, Mohit
collection PubMed
description PURPOSE: To investigate the biocompatibility of fish scale-derived scaffolds (FSS) with primary human corneal endothelial cells (HCEnCs). METHODS: HCEnCs were isolated from 30 donor corneas in a donor-matched study and plated in precoated Lab-Tek slides (n = 15) and FSS (n = 15). Cell morphology, proliferation/migration, and glucose uptake were studied (n = 30). Hoechst, ethidium homodimer, and calcein AM (HEC) staining was performed to determine viability and toxicity (n = 6). The cell surface area was calculated based on calcein AM staining. HCEnCs were stained for ZO-1 (n = 6) to detect tight junctions and to measure cell morphology; Ki-67 (n = 6) to measure proliferating cells; and vinculin to quantify focal adhesions (n = 6). The formation of de novo extracellular matrix was analyzed using histology (n = 6). RESULTS: HCEnCs attach and grow faster on Lab-Tek slides compared to the undulating topography of the FSS. At day 11, HCEnCs on Lab-Tek slide grew 100% confluent, while FSS was only 65% confluent (p = 0.0883), with no significant difference in glucose uptake between the two (p = 0.5181) (2.2 μg/mL in Lab-Tek versus 2.05 μg/mL in FSS). HEC staining showed no toxicity. The surface area of the cells in Lab-Tek was 409.1 μm(2) compared to 452.2 μm(2) on FSS, which was not significant (p = 0.5325). ZO-1 showed the presence of tight junctions in both conditions; however, hexagonality was higher (74% in Lab-Tek versus 45% in FSS; p = 0.0006) with significantly less polymorphic cells on Lab-Tek slides (8% in Lab-Tek versus 16% in FSS; p = 0.0041). Proliferative cells were detected in both conditions (4.6% in Lab-Tek versus 4.2% in FSS; p = 0.5922). Vinculin expression was marginally higher in HCEnCs cultured on Lab-Tek (234 versus 199 focal adhesions; p = 0.0507). Histological analysis did not show the formation of a basement membrane. CONCLUSIONS: HCEnCs cultured on precoated FSS form a monolayer, displaying correct morphology, cytocompatibility, and absence of toxicity. FSS needs further modification in terms of structure and surface chemistry before considering it as a potential carrier for cultured HCEnCs.
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spelling pubmed-59491772018-05-31 Fish Scale-Derived Scaffolds for Culturing Human Corneal Endothelial Cells Parekh, Mohit Van den Bogerd, Bert Zakaria, Nadia Ponzin, Diego Ferrari, Stefano Stem Cells Int Research Article PURPOSE: To investigate the biocompatibility of fish scale-derived scaffolds (FSS) with primary human corneal endothelial cells (HCEnCs). METHODS: HCEnCs were isolated from 30 donor corneas in a donor-matched study and plated in precoated Lab-Tek slides (n = 15) and FSS (n = 15). Cell morphology, proliferation/migration, and glucose uptake were studied (n = 30). Hoechst, ethidium homodimer, and calcein AM (HEC) staining was performed to determine viability and toxicity (n = 6). The cell surface area was calculated based on calcein AM staining. HCEnCs were stained for ZO-1 (n = 6) to detect tight junctions and to measure cell morphology; Ki-67 (n = 6) to measure proliferating cells; and vinculin to quantify focal adhesions (n = 6). The formation of de novo extracellular matrix was analyzed using histology (n = 6). RESULTS: HCEnCs attach and grow faster on Lab-Tek slides compared to the undulating topography of the FSS. At day 11, HCEnCs on Lab-Tek slide grew 100% confluent, while FSS was only 65% confluent (p = 0.0883), with no significant difference in glucose uptake between the two (p = 0.5181) (2.2 μg/mL in Lab-Tek versus 2.05 μg/mL in FSS). HEC staining showed no toxicity. The surface area of the cells in Lab-Tek was 409.1 μm(2) compared to 452.2 μm(2) on FSS, which was not significant (p = 0.5325). ZO-1 showed the presence of tight junctions in both conditions; however, hexagonality was higher (74% in Lab-Tek versus 45% in FSS; p = 0.0006) with significantly less polymorphic cells on Lab-Tek slides (8% in Lab-Tek versus 16% in FSS; p = 0.0041). Proliferative cells were detected in both conditions (4.6% in Lab-Tek versus 4.2% in FSS; p = 0.5922). Vinculin expression was marginally higher in HCEnCs cultured on Lab-Tek (234 versus 199 focal adhesions; p = 0.0507). Histological analysis did not show the formation of a basement membrane. CONCLUSIONS: HCEnCs cultured on precoated FSS form a monolayer, displaying correct morphology, cytocompatibility, and absence of toxicity. FSS needs further modification in terms of structure and surface chemistry before considering it as a potential carrier for cultured HCEnCs. Hindawi 2018-04-29 /pmc/articles/PMC5949177/ /pubmed/29853917 http://dx.doi.org/10.1155/2018/8146834 Text en Copyright © 2018 Mohit Parekh et al. http://creativecommons.org/licenses/by/4.0/ This is an open access article distributed under 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
Parekh, Mohit
Van den Bogerd, Bert
Zakaria, Nadia
Ponzin, Diego
Ferrari, Stefano
Fish Scale-Derived Scaffolds for Culturing Human Corneal Endothelial Cells
title Fish Scale-Derived Scaffolds for Culturing Human Corneal Endothelial Cells
title_full Fish Scale-Derived Scaffolds for Culturing Human Corneal Endothelial Cells
title_fullStr Fish Scale-Derived Scaffolds for Culturing Human Corneal Endothelial Cells
title_full_unstemmed Fish Scale-Derived Scaffolds for Culturing Human Corneal Endothelial Cells
title_short Fish Scale-Derived Scaffolds for Culturing Human Corneal Endothelial Cells
title_sort fish scale-derived scaffolds for culturing human corneal endothelial cells
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5949177/
https://www.ncbi.nlm.nih.gov/pubmed/29853917
http://dx.doi.org/10.1155/2018/8146834
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