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Comprehensive characterization of chondrocyte cultures in plasma and whole blood biomatrices for cartilage tissue engineering

机译:软骨组织工程血浆和全血生物基质中软骨细胞培养物的综合表征

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Many synthetic polymers and biomaterials have been used as matrices for 3D chondrocyte seeding and transplantation in the field of cartilage tissue engineering. To develop a fully autologous carrier for chondrocyte cultivation, we examined the feasibility of allogeneic plasma and whole blood-based matrices and compared them to agarose constructs. Primary articular chondrocytes isolated from 12-month-old pigs were embedded into agarose, plasma and whole blood matrices and cultivated under static-free swelling conditions for up to four weeks. To evaluate the quality of the synthesized extracellular matrix (ECM), constructs were subjected to weekly examinations using histological staining, spectrophotometry, immunohistochemistry and biochemical analysis. In addition, gene expression of cartilage-specific markers such as aggrecan, Sox9 and collagen types I, II and X was determined by RT-PCR. Chondrocyte morphology was assessed via scanning electron microscopy and viability staining, including proliferation and apoptosis assays. Finally, 13C NMR spectroscopy provided further evidence of synthesis of ECM components. It was shown that chondrocyte cultivation in allogeneic plasma and whole-blood matrices promoted sufficient chondrocyte viability and differentiation behaviour, resulting in neo-formation of a hyaline-like cartilage matrix.
机译:在软骨组织工程领域,许多合成聚合物和生物材料已被用作3D软骨细胞播种和移植的基质。为了开发用于软骨细胞培养的完全自体载体,我们检查了同种异体血浆和全血基基质的可行性,并将它们与琼脂糖构建体进行了比较。从12个月大的猪中分离出的原发性软骨细胞被嵌入琼脂糖,血浆和全血基质中,并在无静电的溶胀条件下培养长达4周。为了评估合成的细胞外基质(ECM)的质量,使用组织学染色,分光光度法,免疫组织化学和生化分析对构建体进行每周检查。另外,通过RT-PCR确定软骨特异性标记物如软骨聚集蛋白聚糖,Sog9和I,II和X型胶原的基因表达。通过扫描电子显微镜和生存力染色,包括增殖和凋亡分析,评估软骨细胞的形态。最后,13 C NMR光谱学提供了ECM成分合成的进一步证据。结果表明,在同种异体血浆和全血基质中培养软骨细胞可促进足够的软骨细胞活力和分化行为,从而形成透明质样软骨基质的新形式。

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