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Corneal Limbal Microenvironment Can Induce Transdifferentiation of Hair Follicle Stem Cells into Corneal Epithelial-like Cells

机译:角膜缘微环境可以诱导毛囊干细胞转分化为角膜上皮样细胞

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摘要

The aim of this study was to investigate the transdifferentiation potential of murine vibrissa hair follicle (HF) stem cells into corneal epithelial-like cells through modulation by corneal- or limbus-specific microenvironmental factors. Adult epithelial stem cells were isolated from the HF bulge region by mechanical dissection or fluorescence-activated cell sorting using antibodies to α6 integrin, enriched by clonal expansion, and subcultivated on various extracellular matrices (type IV collagen, laminin-1, laminin-5, fibronectin) and in different conditioned media derived from central and peripheral corneal fibroblasts, limbal stromal fibroblasts, and 3T3 fibroblasts. Cellular phenotype and differentiation were evaluated by light and electron microscopy, real-time reverse transcription-polymerase chain reaction, immunocytochemistry, and Western blotting, using antibodies against putative stem cell markers (K15, α6 integrin) and differentiation markers characteristic for corneal epithelium (K12, Pax6) or epidermis (K10). Using laminin-5, a major component of the corneo-limbal basement membrane zone, and conditioned medium from limbal stromal fibroblasts, clonally enriched HF stem and progenitor cells adhered rapidly and formed regularly arranged stratified cell sheets. Conditioned medium derived from limbal fibroblasts markedly upregulated expression of cornea-specific K12 and Pax6 on the mRNA and protein level, whereas expression of the epidermal keratinocyte marker K10 was strongly downregulated. These findings suggest that adult HF epithelial stem cells are capable of differentiating into corneal epithelial-like cells in vitro when exposed to a limbus-specific microenvironment. Therefore, the HF may be an easily accessible alternative therapeutic source of autologous adult stem cells for replacement of the corneal epithelium and restoration of visual function in patients with ocular surface disorders.
机译:这项研究的目的是研究小鼠角膜毛囊(HF)干细胞通过角膜或角膜缘特异性微环境因子的调控而向角膜上皮样细胞的转分化潜能。使用抗α6整联蛋白的抗体,通过机械解剖或荧光激活细胞分选法,从HF隆起区分离成年上皮干细胞,通过克隆扩增富集,然后在各种细胞外基质(IV型胶原,层粘连蛋白1,层粘连蛋白5,纤连蛋白)和来自中央和周边角膜成纤维细胞,角膜缘基质成纤维细胞和3T3成纤维细胞的不同条件培养基中。使用抗推定干细胞标记物(K15,α6整联蛋白)和角膜上皮细胞特征性分化标记物(K12)的抗体通过光镜和电子显微镜,实时逆转录聚合酶链反应,免疫细胞化学和蛋白质印迹法评估细胞表型和分化,Pax6)或表皮(K10)。使用层粘连蛋白5(角膜-基底膜区的主要成分)和来自角膜基质成纤维细胞的条件培养基,克隆富集的HF干细胞和祖细胞迅速粘附并形成规则排列的分层细胞片。衍生自角膜缘成纤维细胞的条件培养基在mRNA和蛋白质水平上显着上调了角膜特异性K12和Pax6的表达,而表皮角质形成细胞标记K10的表达则强烈下调。这些发现表明,当暴露于角膜缘特异性微环境时,成年HF上皮干细胞能够在体外分化为角膜上皮样细胞。因此,HF可能是自体成体干细胞的一种易于获得的替代治疗来源,用于替换眼表疾病患者的角膜上皮和恢复视觉功能。

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