Non-destructive monitoring of viability in an ex vivo organ culture model of osteochondral tissue

Non-destructive monitoring of viability in an ex vivo organ culture model of osteochondral tissue

Organ culture is an increasingly important tool in research, with advantages over monolayer cell culture due to the inherent natural environment of tissues. Successful organ cultures must retain cell viability. The aim of this study was to produce viable and non-viable osteochondral organ cultures,...

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Main Authors: KM Elson, N Fox, JL Tipper, J Kirkham, RM Hall, J Fisher, E Ingham
Format: Article
Language:English
Published: AO Research Institute Davos 2015-06-01
Series:European Cells & Materials
Subjects:
Organ culture
apoptosis
necrosis
viability monitoring
glucose
lactate dehydrogenase
matrix metalloproteinase
Online Access:http://www.ecmjournal.org/journal/papers/vol029/pdf/v029a27.pdf
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spelling doaj-9a98fefe80d14bc8a5f76402997f9f192020-11-25T01:00:14Zeng AO Research Institute DavosEuropean Cells & Materials1473-22622015-06-0129356369Non-destructive monitoring of viability in an ex vivo organ culture model of osteochondral tissue KM ElsonN FoxJL TipperJ KirkhamRM HallJ FisherE Ingham0School of Biomedical Science, 7.59 Garstang Building, University of Leeds, Leeds, LS2 9JT, UKOrgan culture is an increasingly important tool in research, with advantages over monolayer cell culture due to the inherent natural environment of tissues. Successful organ cultures must retain cell viability. The aim of this study was to produce viable and non-viable osteochondral organ cultures, to assess the accumulation of soluble markers in the conditioned medium for predicting tissue viability. Porcine femoral osteochondral plugs were cultured for 20 days, with the addition of Triton X-100 on day 6 (to induce necrosis), camptothecin (to induce apoptosis) or no toxic additives. Tissue viability was assessed by the tissue destructive XTT (2,3-bis[2-methoxy-4-nitro-5-sulfophenyl]-2H-tetrazolium-5-carboxyanilide tetrazolium salt) assay method and LIVE/DEAD® staining of the cartilage at days 0, 6 and 20. Tissue structure was assessed by histological evaluation using haematoxylin & eosin and safranin O. Conditioned medium was assessed every 3-4 days for glucose depletion, and levels of lactate dehydrogenase (LDH), alkaline phosphatase (AP), glycosaminoglycans (GAGs), and matrix metalloproteinase (MMP)-2 and MMP-9. Necrotic cultures immediately showed a reduction in glucose consumption, and an immediate increase in LDH, GAG, MMP-2 and MMP-9 levels. Apoptotic cultures showed a delayed reduction in glucose consumption and delayed increase in LDH, a small rise in MMP-2 and MMP-9, but no significant effect on GAGs released into the conditioned medium. The data showed that tissue viability could be monitored by assessing the conditioned medium for the aforementioned markers, negating the need for tissue destructive assays. Physiologically relevant whole- or part-joint organ culture models, necessary for research and pre-clinical assessment of therapies, could be monitored this way, reducing the need to sacrifice tissues to determine viability, and hence reducing the sample numbers necessary.http://www.ecmjournal.org/journal/papers/vol029/pdf/v029a27.pdfOrgan cultureapoptosisnecrosisviability monitoringglucoselactate dehydrogenasematrix metalloproteinase
collection DOAJ
language English
format Article
sources DOAJ
author KM Elson
N Fox
JL Tipper
J Kirkham
RM Hall
J Fisher
E Ingham
spellingShingle KM Elson
N Fox
JL Tipper
J Kirkham
RM Hall
J Fisher
E Ingham
Non-destructive monitoring of viability in an ex vivo organ culture model of osteochondral tissue
European Cells & Materials
Organ culture
apoptosis
necrosis
viability monitoring
glucose
lactate dehydrogenase
matrix metalloproteinase
author_facet KM Elson
N Fox
JL Tipper
J Kirkham
RM Hall
J Fisher
E Ingham
author_sort KM Elson
title Non-destructive monitoring of viability in an ex vivo organ culture model of osteochondral tissue
title_short Non-destructive monitoring of viability in an ex vivo organ culture model of osteochondral tissue
title_full Non-destructive monitoring of viability in an ex vivo organ culture model of osteochondral tissue
title_fullStr Non-destructive monitoring of viability in an ex vivo organ culture model of osteochondral tissue
title_full_unstemmed Non-destructive monitoring of viability in an ex vivo organ culture model of osteochondral tissue
title_sort non-destructive monitoring of viability in an ex vivo organ culture model of osteochondral tissue
publisher AO Research Institute Davos
series European Cells & Materials
issn 1473-2262
publishDate 2015-06-01
description Organ culture is an increasingly important tool in research, with advantages over monolayer cell culture due to the inherent natural environment of tissues. Successful organ cultures must retain cell viability. The aim of this study was to produce viable and non-viable osteochondral organ cultures, to assess the accumulation of soluble markers in the conditioned medium for predicting tissue viability. Porcine femoral osteochondral plugs were cultured for 20 days, with the addition of Triton X-100 on day 6 (to induce necrosis), camptothecin (to induce apoptosis) or no toxic additives. Tissue viability was assessed by the tissue destructive XTT (2,3-bis[2-methoxy-4-nitro-5-sulfophenyl]-2H-tetrazolium-5-carboxyanilide tetrazolium salt) assay method and LIVE/DEAD® staining of the cartilage at days 0, 6 and 20. Tissue structure was assessed by histological evaluation using haematoxylin & eosin and safranin O. Conditioned medium was assessed every 3-4 days for glucose depletion, and levels of lactate dehydrogenase (LDH), alkaline phosphatase (AP), glycosaminoglycans (GAGs), and matrix metalloproteinase (MMP)-2 and MMP-9. Necrotic cultures immediately showed a reduction in glucose consumption, and an immediate increase in LDH, GAG, MMP-2 and MMP-9 levels. Apoptotic cultures showed a delayed reduction in glucose consumption and delayed increase in LDH, a small rise in MMP-2 and MMP-9, but no significant effect on GAGs released into the conditioned medium. The data showed that tissue viability could be monitored by assessing the conditioned medium for the aforementioned markers, negating the need for tissue destructive assays. Physiologically relevant whole- or part-joint organ culture models, necessary for research and pre-clinical assessment of therapies, could be monitored this way, reducing the need to sacrifice tissues to determine viability, and hence reducing the sample numbers necessary.
topic Organ culture
apoptosis
necrosis
viability monitoring
glucose
lactate dehydrogenase
matrix metalloproteinase
url http://www.ecmjournal.org/journal/papers/vol029/pdf/v029a27.pdf
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AT nfox nondestructivemonitoringofviabilityinanexvivoorganculturemodelofosteochondraltissue
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AT jkirkham nondestructivemonitoringofviabilityinanexvivoorganculturemodelofosteochondraltissue
AT rmhall nondestructivemonitoringofviabilityinanexvivoorganculturemodelofosteochondraltissue
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