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Combination of Low Calcium with Y-27632 Rock Inhibitor Increases the Proliferative Capacity Expansion Potential and Lifespan of Primary Human Keratinocytes while Retaining Their Capacity to Differentiate into Stratified Epidermis in a 3D Skin Model

机译:低钙与Y-27632岩石抑制剂的组合可增加原代人角质形成细胞的增殖能力扩增潜能和寿命同时在3D皮肤模型中保持其分化为分层表皮的能力。

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摘要

Human keratinocytes are difficult to isolate and have a limited lifespan. Traditionally, immortalised keratinocyte cell lines are used in vitro due to their ability to bypass senescence and survive indefinitely. However these cells do not fully retain their ability to differentiate in vitro and they are unable to form a normal stratum corneum in organotypic culture. Here we aimed to generate a pool of phenotypically similar keratinocytes from human donors that could be used in monolayer culture, without a fibroblast feeder layer, and in 3D human skin equivalent models. Primary human neonatal epidermal keratinocytes (HEKn) were cultured in low calcium, (0.07mM) media, +/-10μM Y-27632 ROCK inhibitor (HEKn-CaY). mRNA and protein was extracted and expression of differentiation markers Keratin 14 (K14), Keratin 10 (K10) and Involucrin (Inv) assessed by qRT-PCR and Western blotting. The differentiation potential of the HEKn-CaY cultures was assessed by increasing calcium levels and removing the Y-27632 for 72hrs prior to assessment of K14, K10 and Inv. The ability of the HEKn-CaY, to form a stratified epithelium was assessed using a human skin equivalent (HSE) model in the absence of Y-27632. Increased proliferative capacity, expansion potential and lifespan of HEKn was observed with the combination of low calcium and 10μM ROCK inhibitor Y-27632. The removal of Y-27632 and the addition of high calcium to induce differentiation allowed the cells to behave as primary keratinocytes even after extended serial passaging. Prolonged lifespan HEK-CaYs were capable of forming an organised stratified epidermis in 3D HSE cultures, demonstrating their ability to fully stratify and retain their original, primary characteristics. In conclusion, the use of 0.07mM Calcium and 10μM Y-27632 in HEKn monocultures provides the opportunity to culture primary human keratinocytes without a cell feeder layer for extended periods of culture whilst retaining their ability to differentiate and form a stratified epithelium.
机译:人角质形成细胞难以分离且寿命有限。传统上,永生化的角质形成细胞系因其绕过衰老并无限期存活的能力而在体外使用。然而,这些细胞不能完全保留其体外分化能力,并且不能在器官型培养物中形成正常的角质层。在这里,我们旨在从人类供体中产生表型相似的角质形成细胞库,这些细胞可用于单层培养,而无需成纤维细胞饲养层,也可用于3D人体皮肤等效模型。在低钙(0.07mM)培养基,+ /-10μMY-27632 ROCK抑制剂(HEKn-CaY)中培养原代人新生儿表皮角质形成细胞(HEKn)。提取mRNA和蛋白质,并通过qRT-PCR和Western印迹法评估分化标记物Keratin 14(K14),Keratin 10(K10)和Involucrin(Inv)的表达。 HEKn-CaY培养物的分化潜能通过在评估K14,K10和Inv之前增加钙水平并去除Y-27632 72小时来评估。在不存在Y-27632的情况下,使用人皮肤等效(HSE)模型评估了HEKn-CaY形成分层上皮的能力。低钙和10μMROCK抑制剂Y-27632的组合可增加HEKn的增殖能力,扩增潜能和寿命。去除Y-27632并添加高钙以诱导分化,即使经过长时间的连续传代后,细胞仍可以充当原代角质形成细胞。延长寿命的HEK-CaYs能够在3D HSE文化中形成有组织的分层表皮,这表明它们能够完全分层并保留其原始的主要特征。总之,在HEKn单培养中使用0.07mM的钙和10μM的Y-27632提供了机会,可以在没有细胞饲养层的情况下培养原代人类角质形成细胞,以延长培养时间,同时保留它们分化和形成分层上皮的能力。

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