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Investigating the effect of chitosan/ polycaprolactone blends in differentiation of corneal endothelial cells and extracellular matrix compositions

机译:研究壳聚糖/聚己内酯共混物在角膜内皮细胞分化中的作用和细胞外基质组合物

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摘要

This study aimed to investigate the underlying mechanisms of corneal endothelial cells (CECs) differentiation and identify the extracellular matrix (ECM) compositions using chitosan/polycaprolactone (PCL) blended membrane, hence exploring the potential use of chitosan/PCL blends in tissue engineering of CECs. We utilized the chitosan/PCL blends named as PCL25 consisting of PCL at 25% by weight. The surface characteristics of PCL25 were confirmed by using Fourier Transform Infrared Spectroscopy (FTIR) and Atomic Force Microscope (AFM). Bovine CECs were cultured on the blends, compared with TCPS and pure chitosan membrane. Cell behaviors in terms of cell attachment, proliferation, differentiation phenotype and expression of differentiation proteins were examined. Furthermore, ECM protein productions were also analyzed. From the experiments, we found the topography (roughness) of PCL25 membrane examined by AFM was greater than pure chitosan membrane. FTIR results confirmed the functional groups of C=O bond of PCL. The CECs displayed hexagonal morphology and similar proliferation rate on both PCL25 membrane and TCPS. In addition, the immunofluorescence evidence showed well-localized ZO-1 and Na+/K+ ATPase expression of membrane proteins. ECM protein productions of CECs on PCL were no inferior to TCPS. Moreover, western blot results verified the higher amount of collagen type IV, and reduced TGF-beta 2 expression on PCL25 membrane compared to TCPS substrate. In conclusions, chitosan/PCL blends membrane provided a favorable environment for CECs in terms of ECM compositions, therefore enhancing the growth and differentiation. Accordingly, for CEC tissue engineering applications, PCL 25 might be a suitable alternative for cadaveric cornea transplantation in the near future.
机译:本研究旨在研究角膜内皮细胞(CEC)分化和鉴定使用壳聚糖/聚己内酯(PCL)混合膜来鉴定细胞外基质(ECM)组合物的潜在机制,因此探讨了壳聚糖/ PCL共混物在CEC的组织工程中的潜在使用。我们利用壳聚糖/ PCL共混物命名为PCL25,其由25重量%的PCL组成。通过使用傅里叶变换红外光谱(FTIR)和原子力显微镜(AFM)来确认PCL25的表面特征。与TCP和纯壳聚糖膜相比,在混合物上培养牛CEC。检查细胞附着,增殖,分化表型和分化蛋白表达方面的细胞行为。此外,还分析了ECM蛋白质生产。从实验中,我们发现AFM检查的PCL25膜的形貌(粗糙度)大于纯壳聚糖膜。 FTIR结果证实了PCL的C = O键的官能团。 CEC在PCL25膜和TCP上显示出六边形形态和类似的增殖速率。此外,免疫荧光证据显示出局部局部的ZO-1和膜蛋白的Na + / K + ATP酶的表达。 PCL上CECS的ECM蛋白质制作不低于TCP。此外,与TCPS衬底相比,Western印迹结果验证了较高量的IV型IV型IV,并降低了PCL25膜上的TGF-β2表达。在结论中,壳聚糖/ PCL共混膜在ECM组合物方面为CEC提供了有利的环境,因此增强了生长和分化。因此,对于CEC组织工程应用,PCL 25可能是在不久的将来的尸体角膜移植的合适替代方案。

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