用连续监测方法从透明软骨中分离软骨细胞

V. Cobzac, L. Verestiuc, M. Jian, V. Nacu
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引用次数: 1

摘要

背景:关节软骨具有较差的再生能力。许多软骨修复技术是已知的,包括自体软骨细胞植入。材料和方法:取兔股骨髁软骨18块。切碎的软骨用0.25%胰蛋白酶- edta处理。第一组(n=9)在37°C, 5%CO2培养箱中摇晃,用0.6%胶原酶消化15 ml管中的软骨。第二组(n=9)在放置于侧面的25cm2细胞培养瓶中进行消化,120分钟后在显微镜下观察消化过程。将分离的细胞培养到80-90%的汇合度。过融合培养16天后,用组织化学染色鉴定软骨细胞。结果:第一组软骨细胞分离时间固定为360分钟,第二组为- 140±10分钟。第1组分离到9.2 × 104±3.1 × 104软骨细胞,存活率为85.36±16.41%;第2组分离到1.6 × 105±3.4 × 104软骨细胞,存活率为98.09±3.85%。第一组平均细胞培养时间为15±2天,第二组平均细胞培养时间为11±3天。第一组第一代获得- 1.2x106±4.3x105个软骨细胞,第二组获得- 2.92x106±3.6x105个软骨细胞。软骨细胞分泌的细胞外基质染色专门用于软骨组织。结论:软骨细胞分离的方法直接影响到分离细胞的数量、生存能力,也影响到培养时间和第一次传代获得的细胞数量。
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Chondrocytes isolation from hyaline cartilage by continuous monitoring method
Background: Articular cartilage has poor regenerative capacities. Numerous cartilage repair techniques are known, including implantation of autologous chondrocytes. Material and methods: From 18 rabbits pieces of cartilage were harvested from femoral condyle. Minced cartilage was treated with 0.25% trypsin-EDTA. In the 1st group (n=9) the cartilage was digested with 0.6% collagenase in 15 ml tubes by shaking in incubator at 37°C, 5%CO2 . In the 2nd group (n=9) digestion was performed in 25cm2 cell culture flasks placed on the lateral side, monitoring the process under a microscope after 120 minutes. The isolated cells were cultured to a 80-90% confluence. The chondrocytes were identified using histochemical staining after culturing for 16 days in overconfluence. Results: Chondrocytes isolation in the 1st group lasted a fixed 360 minutes, in the 2nd group – 140±10 minutes. In the 1stgroup were isolated 9.2x104 ±3.1x104 chondrocytes with a viability of 85.36±16.41%, but in the 2nd group – 1.6x105 ±3.4x104 chondrocytes with a viability of 98.09±3.85%. The mean period of cell culture in the 1st group was 15±2 days, in the 2nd group – 11±3 days. In first passage of the 1st group were obtained – 1.2x106 ±4.3x105 chondrocytes and in the 2nd group – 2.92x106 ±3.6x105 chondrocytes. The secreted extracellular matrix by chondrocytes was stained specifically for cartilaginous tissue. Conclusions: The method used for chondrocytes isolation has a direct impact on the number of isolated cells, their viability, but also upon the culture period and the number of cells obtained during the first passage.
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