Banking of osteochondral allografts. Part I. Viability assays adapted for osteochondrol and cartilage studies

被引:13
|
作者
Csönge L. [1 ,6 ]
Bravo D. [2 ]
Newman-Gage H. [3 ]
Rigley T. [2 ]
Conrad E.U. [3 ]
Bakay A. [4 ]
Strong D.M. [5 ]
Pellet S. [1 ]
机构
[1] West Hungarian Regional Tissue Bank, Gyõr
[2] Northwest Tissue Center, Puget Sound Blood Center, Seattle, WA
[3] Northwest Tissue Center, Department of Orthopaedics, University of Washington, Seattle, WA
[4] Department of Traumatology, MÁV Hospital, Budapest
[5] Northwest Tissue Center, Department of Surgery, University of Washington, Seattle, WA
[6] Fulbright Scholar at NW Tissue Ctr., Seattle, WA
基金
匈牙利科学研究基金会;
关键词
Cartilage; Fluorescent dye; MTT assay; Osteochondral allograft; Viability;
D O I
10.1023/A:1023665418244
中图分类号
学科分类号
摘要
The aim of this study was to adapt a reliable, reproducible and simple viability assay for cartilage and osteochondral studies. The previous assays (radioisotope uptake, assessment of matrix components, histological methods, oxygen consumption etc.) were complex, laborious, time consuming or suffer from difficulty of interpretation. MTT assay was chosen because it has been widely and successfully used in different cell and tissue studies, but has not been published on human solid articular cartilage. Fresh intact cartilage samples of human tali were tested to investigate the assay. The reliability of the MTT assay was also tested by an fluorescent dye combination. The MTT assay is based on the production of purple formazan pigment from methyltetrazolium salt by the mitochondrial enzymes of viable chondrocytes. The enzyme kinetics of the reaction was also investigated because it was unknown in the case of cartilage. The amount of pigment formed can be measured by spectrophotometry after extraction by methyl cellosolve. The color density is proportional to mitochondrial enzyme activity, reflecting the number of viable chondrocytes. The optimal reagent concentration, biopsy size, and incubation period were established. There is a linear relationship between the cartilage weight and the pigment production activity, A 9.8% nonspecific raction was observed in the negative controls. The enzyme kinetics of the reaction was also investigated. The MTT clevage up to 0.1% (w/v) follows the Michaelis kinetics. We calculated the Michaelis constant (2835 ± 130 μM), the maximal velocity (36 ± 3.2 × 105 μMsec-1) and the velocity constant (1.27 ± 0.2 × 10-7 sec-1) of the reaction. The latter is a significant marker for each tissue type. The viability of cartilage was also assessed and calculated by a fluorescent dye combination comprising 1 μg/ml propidium iodide (PI) and 4 μM/ml SYTO-16 stains. The PI stains dead cells (red fluorescence), the SYTO-16 stains live cells (green fluorescence). The staining can be visualised simultaneously, and the live/dead ratio can be calculated by image analysis software from saved image files. The MTT assay is a simple, non-expensive, efficient, reliable, reproducible, sensitive viability test for cartilage studies. The MTT reduction assay and the staining method were corrobative.
引用
收藏
页码:151 / 159
页数:8
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