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A rapid sonication based method for preparation of stromal vascular fraction and mesenchymal stem cells from fat tissue

机译:基于快速超声处理的脂肪组织制备间质血管部分和间充质干细胞的方法

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Introduction Much attention has been paid to the idea of cell therapy using stem cells from different sources of the body. Fat-derived stem cells that are called adipose derived stem cells (ADSCs) from stromal vascular fraction (SVF) are the subject of many studies in several cell therapy clinical trials. Despite production of some GMP-grade enzymes to isolate SVF for clinical trials, there are critical conditions like inconsistency in lot-to-lot enzyme activity, endotoxin residues, other protease activities and cleavage of some cell surface markers which significantly narrow the options. So we decided to develop a new method via sonication cavitation to homogenize fat tissue and disrupt partially adipose cells to obtain SVF and finally ADSCs at a minimum of time and expenses. Methods The fat tissue was chopped in a sterile condition by a blender mixer and then sonicated for 2 s before centrifugation. The next steps were performed as the regular methods of SVF harvesting, and then it was characterized using flow cytometry. Results Analysis of the surface markers of the cells revealed similar sets of surface antigens. The cells showed slightly high expression of CD34, CD73 and CD105. The differentiation capacity of these cells indicates that multipotent properties of the cells are not compromised after sonication. But we had the less osteogenic potential of cells when compared with the enzymatic method. Conclusion The current protocol based on the sonication-mediated cavitation is a rapid, safe and cost-effective method, which is proposed for isolation of SVF and of course ADSCs cultures in a large scale for the clinical trials or therapeutic purposes.
机译:引言人们已经非常关注使用来自身体不同来源的干细胞进行细胞治疗的想法。来自脂肪的干细胞,称为基质血管部分(SVF)的脂肪来源的干细胞(ADSC),是许多细胞疗法临床试验中许多研究的主题。尽管产生了一些GMP级酶以分离SVF进行临床试验,但仍存在一些关键条件,例如批次间酶活性,内毒素残基,其他蛋白酶活性和某些细胞表面标志物的裂解不一致,这大大缩小了选择范围。因此,我们决定通过超声空化技术开发一种新方法,以均匀化脂肪组织并破坏部分脂肪细胞,从而以最少的时间和费用获得SVF和ADSC。方法用混合机将脂肪组织在无菌条件下切碎,然后超声处理2 s,然后离心。下一步是按常规方法收集SVF,然后使用流式细胞仪对其进行表征。结果对细胞表面标志物的分析揭示了相似的表面抗原组。细胞显示出CD34,CD73和CD105的高表达。这些细胞的分化能力表明,超声处理后细胞的多能性没有受到损害。但是,与酶法相比,我们的细胞具有较低的成骨潜能。结论基于超声介导的空化作用的当前方案是一种快速,安全且具有成本效益的方法,为临床试验或治疗目的大规模分离SVF和ADSC培养提供了建议。

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