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一种从皮肤外植体培养人角质形成细胞的改进方法:细胞扩增与活化祖细胞标志物相关。

An improved method of human keratinocyte culture from skin explants: cell expansion is linked to markers of activated progenitor cells.

作者信息

Guo Aihua, Jahoda Colin A B

机构信息

Department of Biological Sciences, University of Durham, Durham, DH1 3LE, UK.

出版信息

Exp Dermatol. 2009 Aug;18(8):720-6. doi: 10.1111/j.1600-0625.2009.00900.x. Epub 2009 Jun 23.

DOI:10.1111/j.1600-0625.2009.00900.x
PMID:19558495
Abstract

Human keratinocyte primary cultures are commonly established by tissue dissociation and often rely on feeder cell supports and culture medium that is not defined. Further, contamination by unwanted fibroblasts can be problematic. Here, we developed a skin explant method for growing primary keratinocytes that was rapid, simple, and reliably generated keratinocyte cultures free of fibroblast contamination. The process capitalized on the observation that fibroblasts migrate out of adult skin explants later than epidermal cells, allowing the early harvesting of keratinocytes by trypsinization. When grown subsequently in defined medium in the absence of feeder cells, the explant-derived cells grew rapidly and could be cultured for multiple passages. Immunofluorescence microscopy revealed that a high percentage of cells harvested from the explant outgrowths expressed K15, while very few expressed the differentiation marker K10. Cells that were stained while migrating out from explants strongly expressed markers associated with progenitor cells, including p63, K15 and CD133, and displayed intense K6 expression, indicative of activated keratinocytes in wound-healing epidermis. By replenishing the explants with fresh medium after harvesting, further epidermal outgrowths could be obtained, offering the possibility of greatly increased keratinocyte yields for clinical applications.

摘要

人角质形成细胞原代培养通常通过组织解离建立,且常常依赖饲养细胞支持以及成分未明确的培养基。此外,不需要的成纤维细胞污染可能会带来问题。在此,我们开发了一种用于培养原代角质形成细胞的皮肤外植体方法,该方法快速、简单,并且能可靠地产生无成纤维细胞污染的角质形成细胞培养物。该过程利用了这样一个观察结果,即成纤维细胞从成人皮肤外植体中迁出的时间比表皮细胞晚,这使得通过胰蛋白酶消化能够早期收获角质形成细胞。随后在无饲养细胞的限定培养基中培养时,外植体来源的细胞生长迅速,并且可以传代培养多次。免疫荧光显微镜检查显示,从外植体生长物中收获的细胞中有很大比例表达K15,而很少有细胞表达分化标志物K10。从外植体迁出时染色的细胞强烈表达与祖细胞相关的标志物,包括p63、K15和CD133,并显示出强烈的K6表达,这表明在伤口愈合表皮中角质形成细胞被激活。通过在收获后用新鲜培养基补充外植体,可以获得更多的表皮生长物,这为临床应用中大幅提高角质形成细胞产量提供了可能性。

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