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首页> 外文期刊>Pharmacological research: The official journal of The Italian Pharmacological Society >Nrf2 activators modulate oxidative stress responses and bioenergetic profiles of human retinal epithelial cells cultured in normal or high glucose conditions
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Nrf2 activators modulate oxidative stress responses and bioenergetic profiles of human retinal epithelial cells cultured in normal or high glucose conditions

机译:Nrf2激活剂调节在正常或高葡萄糖条件下培养的人视网膜上皮细胞的氧化应激反应和生物能谱

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摘要

Retinal pigment epithelial cells exert an important supporting role in the eye and develop adaptive responses to oxidative stress or high glucose. levels, as observed during diabetes. Endogenous antioxidant defences are mainly regulated by Nrf2, a transcription factor that is activated by naturally-derived and electrophilic compounds. Here we investigated the effect of the Nrf2 activators dimethylfumarate (DMF) and carnosol on antioxidant pathways, oxygen consumption rate and wound healing in human retinal pigment epithelial cells (ARPE-19) cultured in medium containing normal (NG, 5 mM) or high (HG, 25 mM) glucose levels. We also assessed wound healing using an in vivo corneal epithelial injury model. We found that Nrf2 nuclear translocation and heme oxygenase activity increased in ARPE cells treated with 10 mu M DMF or carnosol irrespective of glucose culture conditions. However, HG rendered retinal cells more sensitive to regulators of glutathione synthesis or inhibition and caused a decrease of both cellular and mitochondrial reactive oxygen species. Culture in HG also reduced ATP production and mitochondrial function as measured with the Seahorse XF analyzer and electron microscopy analysis revealed morphologically damaged mitochondria. Acute treatment with DMF or carnosol did not restore mitochondrial function in HG cells; conversely, the compounds reduced cellular maximal respiratory and reserve capacity, which were completely prevented by N-acetylcysteine thus suggesting the involvement of thiols in this effect. Interestingly, the scratch assay showed that wound closure was faster in cells cultured in HG than NG and was accelerated by carnosol. This effect was reversed by an inhibitor of heme oxygenase activity. Moreover, topical application of carnosol to the cornea of diabetic rats significantly accelerated wound healing. In summary, these data indicate that culture of retinal epithelial cells in HG does not affect the activation of the Nrf2/heme oxygenase axis but influences other crucial oxidative and mitochondrial-dependent cellular functions. The additional effect on wound closure suggests that results obtained in in vitro experimental settings need to be carefully evaluated in the context of the glucose concentrations used in cell culture. (C) 2015 Elsevier Ltd. All rights reserved.
机译:视网膜色素上皮细胞在眼睛中发挥重要的支持作用,并发展对氧化应激或高葡萄糖的适应性反应。糖尿病期间观察到的血脂水平。内源性抗氧化剂防御主要受Nrf2调节,Nrf2是一种由天然和亲电子化合物激活的转录因子。在这里,我们研究了Nrf2激活剂富马酸二甲酯(DMF)和鼠尾草酚对在正常(NG,5 mM)或高(NG)培养基中培养的人视网膜色素上皮细胞(ARPE-19)的抗氧化途径,耗氧率和伤口愈合的影响。 HG,25 mM)葡萄糖水平。我们还使用体内角膜上皮损伤模型评估了伤口愈合情况。我们发现,在10μMDMF或鼠尾草酚处理的ARPE细胞中,无论葡萄糖培养条件如何,Nrf2核易位和血红素加氧酶活性均增加。然而,HG使视网膜细胞对谷胱甘肽合成或抑制的调节剂更敏感,并导致细胞和线粒体活性氧的减少。用Seahorse XF分析仪测量,HG中的培养也降低了ATP的产生和线粒体功能,电子显微镜分析揭示了形态受损的线粒体。 DMF或鼠尾草酚的急性治疗不能恢复HG细胞的线粒体功能。相反,该化合物降低了细胞的最大呼吸和储备能力,这被N-乙酰半胱氨酸完全阻止,因此表明硫醇参与了这种作用。有趣的是,刮擦试验表明,在HG中培养的细胞中伤口闭合比NG更快,并且被鼠尾草酚加速。这种作用被血红素加氧酶活性的抑制剂逆转。此外,向糖尿病大鼠的角膜局部施用鼠尾草酚可显着加速伤口愈合。总之,这些数据表明在HG中视网膜上皮细胞的培养不会影响Nrf2 /血红素加氧酶轴的激活,但会影响其他关键的氧化和线粒体依赖性细胞功能。对伤口闭合的附加作用表明,需要在细胞培养中使用的葡萄糖浓度的背景下仔细评估在体外实验环境中获得的结果。 (C)2015 Elsevier Ltd.保留所有权利。

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