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Repair of rabbit ulna segmental bone defect using freshly isolated adipose-derived stromal vascular fraction

机译:新鲜分离的脂肪间质血管部分修复兔尺骨节段性骨缺损

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Background aims. Stromal vascular fractions (SVF) from adipose tissue have heterogeneous cell populations, and include multipotent adipose-derived stem cells. The advantages of using of SVF include the avoidance of an additional culture period, a reduced risk of extensive cell contamination, and cost-effectiveness. Methods. Unilateral 20-mm mid-diaphyseal segmental defects in rabbit ulna were treated with one of the following: polylactic glycolic acid (PLGA) scaffold alone (group 1, control), a PLGA scaffold with undifferentiated SVF cells (group 2), or a PLGA scaffold with osteogenically differentiated SVF cells (group 3). At 8 weeks after implantation, five rabbits in each treatment group were killed to assess bone defect healing by plain radiography, quantitative microcomputed tomography and histology. Results. The SVF cells were well grown on PLGA scaffolds and expressed type I collagen and alkaline phosphatase (ALP). The intensity of ALP and OPN gene expressions in osteogenic medium culture were increased from 14 days to 28 days. In vivo evaluations at 8 weeks showed that treatment of SVF cells with or without osteogenic differentiation resulted in more bone formation in the critically sized segmental defects than PLGA scaffold alone. Osteogenically differentiated SVF cells significantly enhanced bone healing compared with undifferentiated SVF cells. Conclusions. Adipose-derived stromal SVF showed osteogenic potential in vitro. Accordingly, SVF could provide a cell source for bone tissue engineering. However, treatment with uncultured SVF cells on bone healing was not satisfactory in the in vivo animal model.
机译:背景目标。来自脂肪组织的基质血管级分(SVF)具有异质细胞群,并包括多能脂肪来源的干细胞。使用SVF的优点包括避免了额外的培养时间,降低了广泛的细胞污染的风险以及成本效益。方法。用以下方法之一治疗兔尺骨的单侧20毫米干dia端节段性缺损:单独使用聚乳酸乙醇酸(PLGA)支架(第1组,对照组),具有未分化SVF细胞的PLGA支架(第2组)或PLGA具有成骨分化的SVF细胞的支架(第3组)。植入后第8周,处死每个治疗组的5只兔子,以通过平片,X线断层摄影术和组织学方法评估骨缺损的愈合情况。结果。 SVF细胞在PLGA支架上生长良好,并表达I型胶原蛋白和碱性磷酸酶(ALP)。成骨培养基中ALP和OPN基因表达的强度从14天增加到28天。在第8周的体内评估显示,与单独的PLGA支架相比,在有或没有成骨分化的情况下处理SVF细胞可在临界大小的节段缺损中导致更多的骨形成。与未分化的SVF细胞相比,成骨分化的SVF细胞显着增强了骨愈合。结论脂肪来源的基质SVF在体外显示成骨潜力。因此,SVF可以为骨组织工程提供细胞来源。然而,在体内动物模型中,未培养的SVF细胞对骨愈合的治疗并不令人满意。

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