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Optimization of Human Corneal Endothelial Cells for Culture: The Removal of Corneal Stromal Fibroblast Contamination Using Magnetic Cell Separation

机译:人角膜内皮细胞培养的优化:磁性细胞分离去除角膜基质成纤维细胞污染

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摘要

The culture of human corneal endothelial cells (CECs) is critical for the development of suitable graft alternative on biodegradable material, specifically for endothelial keratoplasty, which can potentially alleviate the global shortage of transplant-grade donor corneas available. However, the propagation of slow proliferative CECs in vitro can be hindered by rapid growing stromal corneal fibroblasts (CSFs) that may be coisolated in some cases. The purpose of this study was to evaluate a strategy using magnetic cell separation (MACS) technique to deplete the contaminating CSFs from CEC cultures using antifibroblast magnetic microbeads. Separated “labeled” and “flow-through” cell fractions were collected separately, cultured, and morphologically assessed. Cells from the “flow-through” fraction displayed compact polygonal morphology and expressed Na+/K+ATPase indicative of corneal endothelial cells, whilst cells from the “labeled” fraction were mostly elongated and fibroblastic. A separation efficacy of 96.88% was observed. Hence, MACS technique can be useful in the depletion of contaminating CSFs from within a culture of CECs.
机译:人角膜内皮细胞(CEC)的培养对于在可生物降解材料上开发合适的移植物替代物至关重要,特别是对于内皮角膜移植术而言,这可能缓解全球可用的移植级供体角膜短缺。但是,缓慢增生的CEC在体外的繁殖可能会受到快速生长的基质角膜成纤维细胞(CSF)的阻碍,在某些情况下,它们可能会被共隔离。本研究的目的是评估使用磁性细胞分离(MACS)技术使用抗成纤维细胞磁性微珠消除CEC培养物中污染的CSF的策略。分别收集分离的“标记”和“流通”细胞级分,进行培养并进行形态学评估。来自“流通”级分的细胞显示出紧凑的多边形形态,并表达指示角膜内皮细胞的Na + / K + ATPase,而来自“标记”级分的细胞则大部分呈细长状,并具有成纤维细胞性。观察到分离效率为96.88%。因此,MACS技术可用于消除CEC文化中的CSF污染。

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