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The Effect of Calcium and Glucose Concentration on Corneal Epithelial Cell Lines Differentiation, Proliferation, and Focal Adhesion Expression

机译:钙和葡萄糖浓度对角膜上皮细胞系分化,增殖和局灶性黏附表达的影响

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It is known that culture media composition can affect cell behavior, morphology, and gene expression. However, in the case of corneal epithelial cells, the combined role of calcium and glucose concentration in media has not previously been examined. In this study, a human immortalized corneal epithelial cell line was used to examine the effect of glucose and calcium concentrations on these cells. Cell metabolic activity, cell growth curve analysis, and relative gene and protein expression of proliferative marker extracellular related kinase (ERK) were used to study proliferation. Corneal epithelial stem cell marker NP63 and mature epithelial marker cytokeratin 3 (CK3) were analyzed by using reverse transcription polymerase chain reaction (RT-PCR) and immunocytochemistry. Focal adhesions were examined by using immunocytochemistry. Cells cultured in both low-glucose, high-calcium (LG-HC) media and high-glucose, low-calcium (HG-LC) media showed similar results in both RT-PCR and immunocytochemistry analysis. NP63 expression was significantly lower and CK3 expression was higher in these groups compared with cells cultured in commercial media. NP63 and CK3 expression was also analyzed by using immunocytochemistry, which confirmed these findings. The high-glucose, high-calcium-fed cells showed the lowest expression of all markers and no gene expression of CK3. This was deemed the most unsuitable media formulation for this cell line. Focal adhesion expression was the lowest in the high-calcium, high-glucose-fed cells, with the most even distribution of this among the commercial media group. Overall, this study showed that varying glucose and calcium concentrations can have significant effects on differentiation, proliferation, focal adhesions, and metabolic activity of this cell line. It seems that an LG-HC and HG-LC formulation were interchangeable with similar proliferative and differentiation effects.
机译:众所周知,培养基成分会影响细胞行为,形态和基因表达。然而,对于角膜上皮细胞,钙和葡萄糖浓度在培养基中的联合作用以前没有被检查过。在这项研究中,人类永生化角膜上皮细胞系用于检查葡萄糖和钙浓度对这些细胞的影响。使用细胞代谢活性,细胞生长曲线分析以及增殖标记物细胞外相关激酶(ERK)的相关基因和蛋白质表达来研究增殖。使用逆转录聚合酶链反应(RT-PCR)和免疫细胞化学分析角膜上皮干细胞标记物NP63和成熟上皮标记物细胞角蛋白3(CK3)。通过使用免疫细胞化学检查局部粘连。在低糖高钙(LG-HC)培养基和高糖低钙(HG-LC)培养基中培养的细胞在RT-PCR和免疫细胞化学分析中均显示相似的结果。与在商业培养基中培养的细胞相比,这些组中的NP63表达明显较低,而CK3表达较高。 NP63和CK3的表达也通过免疫细胞化学分析,证实了这些发现。高糖,高钙喂养的细胞显示所有标记物的最低表达,而CK3则无基因表达。这被认为是该细胞系最不合适的培养基配方。在高钙,高葡萄糖喂养的细胞中,局灶性粘附表达最低,在商业培养基组中分布最均匀。总体而言,这项研究表明,不同的葡萄糖和钙浓度可能对该细胞系的分化,增殖,粘着斑和代谢活性产生重大影响。看来LG-HC和HG-LC制剂可以互换,具有相似的增殖和分化作用。

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