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首页> 外文期刊>International journal of molecular medicine >Characterization of auricular chondrocytes and auricular/articular chondrocyte co-cultures in terms of an application in articular cartilage repair.
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Characterization of auricular chondrocytes and auricular/articular chondrocyte co-cultures in terms of an application in articular cartilage repair.

机译:根据在关节软骨修复中的应用,对耳软骨细胞和耳/关节软骨细胞共培养物进行表征。

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摘要

Cartilage injury remains a challenge in orthopedic surgery as articular cartilage only has a limited capacity for intrinsic healing. Autologous chondrocyte transplantation (ACT) is a suitable technique for cartilage repair, but requires articular cartilage biopsies for autologous chondrocyte expansion. The use of heterotopic chondrocytes derived from non-articular cartilage sources such as auricular chondrocytes may be a novel approach for ACT. The aim of the study is to evaluate whether co-cultured articular/auricular chondrocytes exhibit characteristics comparable to articular chondrocytes. Analysis of the proliferation rate, extracellular cartilage matrix (ECM) gene and protein expression (type II and I collagen, elastin, lubricin), beta1-integrins and the chondrogenic transcription factor sox9 in articular/auricular chondrocytes was performed using RTD-PCR, flow cytometry, immunofluorescence microscopy and Western blot analysis. Additionally, three-dimensional (3D) chondrocyte mono- and co-cultures were established. The proliferative activity and elastin gene expression were lower and that of type II collagen and lubricin was higher in articular compared with auricular chondrocytes. The species generally did not influence the chondrocyte characteristics, with the exception of type I collagen and sox9 expression, which was higher in porcine but not in human articular chondrocytes compared with both types of auricular chondrocytes. beta1-integrin gene expression did not differ significantly between the chondrocyte types. The type II collagen gene and protein expression was higher in articular chondrocyte monocultures and was slightly higher in co-cultures compared with monocultured auricular chondrocytes. Both chondrocyte types survived in co-culture. Despite their differing expression profiles, co-cultures revealed some adjustment in the ECM expression of both chondrocyte types.
机译:软骨损伤在整形外科中仍然是一个挑战,因为关节软骨仅具有有限的内在愈合能力。自体软骨细胞移植(ACT)是一种适用于软骨修复的技术,但需要进行关节软骨活检才能自体软骨细胞扩增。来源于非关节软骨来源的异位软骨细胞(如耳软骨细胞)的使用可能是ACT的一种新方法。该研究的目的是评估共培养的关节/耳软骨细胞是否表现出与关节软骨细胞相当的特性。使用RTD-PCR对流动/软骨细胞中的增殖率,细胞外软骨基质(ECM)基因和蛋白质表达(II型和I型胶原,弹性蛋白,lubricin),β1-整联蛋白和软骨形成转录因子sox9进行分析细胞计数,免疫荧光显微镜和蛋白质印迹分析。此外,建立了三维(3D)软骨细胞单培养和共培养。与耳软骨细胞相比,关节中的增殖活性和弹性蛋白基因表达较低,II型胶原和卢布林的增殖活性较高。该物种通常不影响软骨细胞的特性,但I型胶原和sox9表达除外,与两种类型的耳软骨细胞相比,猪中的I型胶原和sox9的表达更高,但人关节软骨细胞中的却没有。 β1-整合素基因表达在软骨细胞类型之间没有显着差异。与单一培养的耳软骨细胞相比,II型胶原基因和蛋白质表达在关节软骨细胞单培养中较高,而在共培养中则略高。两种软骨细胞类型均在共培养中存活。尽管它们的表达谱不同,但共培养显示两种软骨细胞类型的ECM表达都有一定的调节。

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