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Multipotent Mesenchymal Stem Cells Derived from Sheep Bone Marrow: Isolation and Cryopreservation

机译:源自绵羊骨髓的多因间充质干细胞:分离和冷冻保存

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Sheep are often used as preclinical large animal models for testing the therapeutic potential of multipotent mesenchymal stem cells (MMSCs). A cell culture with characteristics typical for MMSCs was obtained due to optimization of the method of cell isolation from sheep bone marrow (BM) in a Ficoll density gradient. The advantage of using SepMate-15 tube compared to the isolation by the classical method has been demonstrated. The obtained cells demonstrated a strong adhesion to the culture plastic, fibroblast-like morphology, and, being induced in vitro, the ability to differentiate into cells of adipose, bone, and cartilage tissues. Adipogenic differentiation was confirmed on day 14, when adipocytes with lipid vesicles positive for Oil Red O specific staining had been formed. On day 14, specific alkaline phosphatase activity appeared in cells in osteogenic medium. Von Kossa staining revealed the presence of insoluble calcium salts in the intercellular space. Chondrogenic differentiation appeared on day 14 and was accompanied with the formation of multilayer structures with an abandon matrix, in which the isogenic groups that resemble hyaline cartilage lacunae were visualized. On day 21, the cells formed tight microgranules with glycosaminoglycan matrixes. Cells were cryopreserved in three different media at the zero passage. A comparative analysis of cell viability was then performed, which revealed a relatively good cell state (more than 70% of live cells). The MMSCs culture obtained from sheep BM was deposited at two to three passages in the specialized Collection of Somatic Cell Cultures of Agricultural and Industrial Animals at the All-Russian Research Institute of Experimental Veterinary Medicine of Russian Academy of Science and could be used in preclinical studies.
机译:绵羊经常用作测试多能间充质干细胞(MMSCs)的治疗潜力的临床前大型动物模型。由于Ficoll密度梯度中的羊骨髓(BM)的细胞分离方法优化,获得了具有典型MMSCs的细胞培养物。已经证明了使用级别方法的隔离相比使用浆酸-15管的优点。所获得的细胞对培养塑料,成纤维细胞样形态的强烈粘附,并且在体外诱导,分化成脂肪,骨和软骨组织的细胞的能力。在第14天确认脂肪发生分化,当已经形成了对油红色O的脂质囊泡阳性的脂肪细胞进行特异性染色时的脂肪细胞。在第14天,在骨质发生介质中的细胞中出现特异性碱性磷酸酶活性。 von kossa染色揭示了细胞间空间中不溶性钙盐的存在。在第14天出现有软骨生分化,并伴随着具有放弃基质的多层结构的形成,其中可视化类似透明软骨裂变裂变物的中生基团。在第21天,细胞与糖胺聚糖基质形成紧密的微粒。在零段通过3种不同介质中冷冻均保存细胞。然后进行细胞活力的对比分析,揭示了相对良好的细胞状态(超过70%的活细胞)。从绵羊BM获得的MMSCS培养物在俄罗斯科学院实验兽医的全俄和工业动物的专业集体细胞培养中沉积了两到三次通道,可以在临床前研究中使用。

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