首页> 外文期刊>Journal of plastic, reconstructive & aesthetic surgery: JPRAS >Adipogenic differentiation potential of rat adipose tissue-derived subpopulations of stromal cells.
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Adipogenic differentiation potential of rat adipose tissue-derived subpopulations of stromal cells.

机译:大鼠脂肪组织来源的基质细胞亚群的成脂分化潜能。

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摘要

Adipose-derived stromal cells (ASCs) are mostly isolated by enzymatic digestion, centrifugation and adherent growth resulting in a very heterogeneous cell population. Therefore, other cell types in the cell culture can comprise the differentiation and proliferation potential of the ASC population. Recent studies indicated that an antibody-aided isolation of distinct ASC subpopulations provides advantages over the conventional method of ASC isolation. The aim of this study was to investigate the adipogenic differentiation potential of CD29-, CD71-, CD73- and CD90-selected ASCs in?vitro. The stromal vascular fraction (SVF) was obtained from rat adipose tissue by enzymatic digestion and centrifugation. Subsequently, CD29(+)-, CD71(+)-, CD73(+)- and CD90(+) cells were isolated by magnetic activated cell sorting (MACS), seeded into culture plates and differentiated into the adipogenic lineage. ASCs isolated by adherent growth only served as controls. Adipogenic differentiation was assessed by Oil Red O staining and quantification of the adiponectin and leptin concentrations in the cell culture supernatants. Statistical analysis was carried out using one-way analysis of variance (ANOVA) followed by the Scheffe's post hoc procedure. The results showed that different subpopulations with different adipogenic differentiation potentials can be isolated by the MACS procedure. The highest adipogenic differentiation potential was determined in the CD29-selected ASC population followed by the unsorted ASC population. The CD71-, CD73- and CD90-selected cells exhibited significantly the lowest adipogenic differentiation potential. In conclusion, the CD29-selected ASCs and the unsorted ASCs exhibited a similar adipogenic differentiation potential. Therefore, we do not see a clear advantage in the application of an anti-CD29-based isolation of ASCs over the conventional technique using adherent growth. However, the research on isolation/purification methods of adipogenic ASCs should continue in order to make this stem cell source even more attractive for future adipose tissue engineering applications.
机译:脂肪来源的基质细胞(ASC)大多是通过酶消化,离心和贴壁生长分离的,从而导致细胞种类非常异质。因此,细胞培养物中的其他细胞类型可包含ASC群体的分化和增殖潜能。最新研究表明,与传统的ASC分离方法相比,不同ASC亚群的抗体辅助分离具有优势。这项研究的目的是调查CD29,CD71,CD73和CD90选择的ASCs在体外的成脂分化潜能。通过酶消化和离心从大鼠脂肪组织获得间质血管部分(SVF)。随后,通过磁激活细胞分选术(MACS)分离CD29(+)-,CD71(+)-,CD73(+)-和CD90(+)细胞,接种到培养板中并分化为成脂谱系。通过粘附生长分离的ASC仅用作对照。通过油红O染色和定量细胞培养上清液中的脂联素和瘦素浓度来评估成脂分化。使用单向方差分析(ANOVA),然后进行Scheffe的事后程序进行统计分析。结果表明,可以通过MACS程序分离具有不同成脂分化潜能的不同亚群。在选择CD29的ASC人群中确定了最高的成脂分化潜能,其次是未分类的ASC人群。 CD71,CD73和CD90选择的细胞表现出最低的成脂分化潜能。总之,CD29选择的ASC和未分选的ASC表现出相似的成脂分化潜能。因此,与使用粘附生长的常规技术相比,我们在应用基于抗CD29的ASC分离中没有看到明显的优势。但是,应继续进行成脂ASC分离/纯化方法的研究,以使这种干细胞来源对未来的脂肪组织工程应用更具吸引力。

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