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首页> 外文期刊>Cellular reprogramming >Chemically Defined Conditions Mediate an Efficient Induction of Mesodermal Lineage from Human Umbilical Cord- and Bone Marrow- Mesenchymal Stem Cells and Dental Pulp Pluripotent-Like Stem Cells
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Chemically Defined Conditions Mediate an Efficient Induction of Mesodermal Lineage from Human Umbilical Cord- and Bone Marrow- Mesenchymal Stem Cells and Dental Pulp Pluripotent-Like Stem Cells

机译:化学定义的病症介导高效诱导人脐带和骨髓间充质干细胞和牙髓多能物质干细胞的中胚层谱系

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The human umbilical cord Wharton's Jelly- and the bone marrow- mesenchymal stem cells (WJ-MSCs and BM-MSCs, respectively) and the newly identified dental pulp pluripotent-like stem cells (DPPSCs) are new sources for stem cells with prospective use in cell regeneration and therapy. These cells are self-renewable, can be differentiated into several lineages, and can potentiate the immune responses. We hypothesized that three-dimensional (3D) culture conditions and directed differentiation using specific signaling regulators will enhance an efficient generation of mesoderm (MD) lineage independent from the origin or source of the stem cells. For a period of 3-days, cell aggregates were generated in a serum-free media containing ascorbic acid, retinoic acid, and keratinocyte growth factor; sonic hedgehog and bone morphogenic protein-4 signaling were inhibited using small molecules. In all cell types used, the biochemical and molecular analysis revealed a time course-dependent induction of the mesodermal, but not endodermal or ectodermal makers. In this study, we utilized a novel and efficient serum-free protocol to differentiate WJ-MSCs, BM-MSCs, and DPPSCs into MD-cells. Successful development of an efficient differentiation protocol can further be utilized and expanded on to obtain MD- derivative cell lineages.
机译:人脐带瓦顿果冻 - 和骨髓间充质干细胞(分别为WJ-MSC和BM-MSCs)和新鉴定的牙科培养皿多能干细胞(DPPSC)是干细胞具有前瞻性使用的新来源细胞再生和治疗。这些细胞是自我可再生的,可以分化为几个谱系,并且可以提高免疫应答。我们假设使用特定信号调节剂的三维(3D)培养条件和定向分化将增强与干细胞的起源或源无关的中胚层(MD)谱系的有效产生。在3天的时间内,在含有抗坏血酸,视黄酸和角质形成细胞生长因子的无血清培养基中产生细胞骨料;使用小分子抑制声音刺猬和骨形态发生蛋白-4信号传导。在所使用的所有细胞类型中,生物化学和分子分析揭示了中胚层,但不是内透层的或异位制造商的时间依赖性诱导。在本研究中,我们利用一种新颖和有效的无血清方案来将WJ-MSCs,BM-MSC和DPPSC分化为MD细胞。可以进一步利用和扩展有效分化协议的成功发展,以获得MD-衍生细胞谱系。

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