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Altered properties of feline adipose-derived mesenchymal stem cells duringcontinuous in vitro cultivation

机译:猫脂肪来源的间充质干细胞在移植过程中的特性改变连续体外培养

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摘要

Cytotherapy with mesenchymal stem cells (MSCs) has been studied in many species, and often requires in vitro cell expansion to obtain therapeutic doses of stem cells. Because the characteristics of MSCs, such as self-renewal and multi-lineage differentiation, can be altered by long-term culture, it is important to maintain stemness during cultivation. This study assessed the changes in the characteristics of feline adipose tissue-derived (fAT)-MSCs during in vitro passaging. Stem cells isolated from the adipose tissue of donor cats were cultured for seven sub-passages. Proliferation capacity was analyzed by calculating the cell doubling time and by colorimetric assay. Expression of stem cell-specific markers was evaluated by quantitative reverse transcription (qRT)-PCR and immunophenotyping. Expression of adipogenic and osteogenic differentiation markers was also measured by qRT-PCR. Histochemical staining and measurement of β-galactosidase activity were conducted to detect cellular senescence. The cell proliferation rate decreased significantly at passage 5 (P5). Gene expression levels of pluripotency markers (Sox2, Nanog and Klf4) and stem cell surface markers (CD9, CD44, CD90 and CD105) decreased during continuous culture; in most assays, statistically significant changes were observedat P5. The ability of cells to undergo adipogenic or osteogenic differentiation wasinversely proportional to the number of passages. The proportion of senescent cellsincreased with the number of passages. These results suggest that repeated passages alterthe proliferation and multipotency of fAT-MSCs. In clinical trials, early-passage cellsshould be used to achieve the maximum therapeutic effect.
机译:间充质干细胞(MSCs)的细胞疗法已在许多物种中得到研究,并且通常需要体外细胞扩增以获得治疗剂量的干细胞。由于长期培养可以改变MSC的特征,如自我更新和多系分化,因此在培养过程中保持茎干很重要。这项研究评估了在体外传代过程中猫脂肪组织(fAT)-MSCs的特征变化。从供体猫的脂肪组织中分离出的干细胞培养了七个亚代。通过计算细胞倍增时间和比色法分析增殖能力。通过定量逆转录(qRT)-PCR和免疫表型评估干细胞特异性标志物的表达。还通过qRT-PCR测量成脂分化和成骨分化标志物的表达。进行组织化学染色和β-半乳糖苷酶活性的测定以检测细胞衰老。在第5代(P5),细胞增殖率显着下降。在连续培养过程中,多能性标志物(Sox2,Nanog和Klf4)和干细胞表面标志物(CD9,CD44,CD90和CD105)的基因表达水平下降;在大多数测定中,观察到统计学上的显着变化在P5。细胞经历成脂或成骨分化的能力为与段落数成反比。衰老细胞的比例随着段落数的增加。这些结果表明重复的段落会改变fAT-MSC的增殖和多能性。在临床试验中,早期传代细胞应该用来达到最大的治疗效果。

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