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Human Adult Stem Cells Maintain a Constant Phenotype Profile Irrespective of Their Origin Basal Media and Long Term Cultures

机译:人类成体干细胞无论其来源基础培养基和长期培养如何都保持恒定的表型特征

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摘要

The study aims to identify the phenotypic marker expressions of different human adult stem cells derived from, namely, bone marrow, subcutaneous fat, and omentum fat, cultured in different media, namely, DMEM-Low Glucose, Alpha-MEM, DMEM-F12 and DMEM-KO and under long term culture conditions (>P20). We characterized immunophenotype by using various hematopoietic, mesenchymal, endothelial markers, and cell adhesion molecules in the long term cultures (Passages-P1, P3, P5, P9, P12, P15, and P20.) Interestingly, data revealed similar marker expression profiles irrespective of source, basal media, and extensive culturing. This demonstrates that all adult stem cell sources mentioned in this study share similar phenotypic marker and all media seem appropriate for culturing these sources. However, a disparity was observed in the markers such as CD49d, CD54, CD117, CD29, and CD106, thereby warranting further research on these markers. Besides the aforesaid objective, it is understood from the study that immunophenotyping acts as a valuable tool to identify inherent property of each cell, thereby leading to a valuable cell based therapy.
机译:这项研究旨在鉴定在不同培养基(即DMEM低血糖,Alpha-MEM,DMEM-F12和DMEM)中培养的不同人类成体干细胞的表型标记物表达,它们分别来自骨髓,皮下脂肪和大网膜脂肪。 DMEM-KO并在长期培养条件下(> P20)。我们通过在长期培养物中使用各种造血,间充质,内皮标记物和细胞粘附分子(Passages-P1,P3,P5,P9,P12,P15和P20)来表征免疫表型。有趣的是,数据揭示了相似的标记物表达谱来源,基础媒体和广泛的培养。这表明该研究中提到的所有成年干细胞来源都具有相似的表型标记,并且所有培养基似乎都适合于培养这些来源。但是,在诸如CD49d,CD54,CD117,CD29和CD106的标记中观察到差异,因此有必要进一步研究这些标记。除了上述目的之外,从该研究中可以理解,免疫表型作为鉴定每个细胞固有特性的有价值的工具,从而导致有价值的基于细胞的治疗。

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