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氧化应激导致角膜内皮细胞的细胞骨架和紧密连接破裂。

Oxidative Stress Induces a Breakdown of the Cytoskeleton and Tight Junctions of the Corneal Endothelial Cells.

机构信息

Department of Biotechnology, Siddaganga Institute of Technology, Tumakuru, India.

Bio-INvENT Lab, Department of Chemical Engineering, Siddaganga Institute of Technology, Tumakuru, India.

出版信息

J Ocul Pharmacol Ther. 2022 Jan-Feb;38(1):74-84. doi: 10.1089/jop.2021.0037. Epub 2021 Nov 23.

DOI:10.1089/jop.2021.0037
PMID:34818079
Abstract

To investigate the impact of oxidative stress, which is a hallmark of Fuchs dystrophy, on the barrier function of the corneal endothelial cells. Experiments were carried out with cultured bovine and porcine corneal endothelial cells. For oxidative stress, cells were supplemented with riboflavin (Rf) and exposed to UV-A (15-30 min) to induce Type-1 photochemical reactions that release HO. The effect of the stress on the barrier function was assayed by transendothelial electrical resistance (TER) measurement. In addition, the associated changes in the organization of the microtubules, perijunctional actomyosin ring (PAMR), and ZO-1 were evaluated by immunocytochemistry, which was also repeated after direct exposure to HO (100 μM, 1 h). Exposure to HO led to the disassembly of microtubules and the destruction of PAMR. In parallel, the contiguous locus of ZO-1 was disrupted, marking a loss of barrier integrity. Accordingly, a sustained loss in TER was induced when cells in the Rf-supplemented medium were exposed to UV-A. However, the addition of catalase (7,000 U/mL) to rapidly decompose HO limited the loss in TER. Furthermore, the adverse effects on microtubules, PAMR, and ZO-1 were suppressed by including catalase, ascorbic acid (1 mM; 30 min), or pretreatment with p38 MAP kinase inhibitor (SB-203580; 10 μM, 1 h). Acute oxidative stress induces microtubule disassembly by a p38 MAP kinase-dependent mechanism, leading to the destruction of PAMR and loss of barrier function. The response to oxidative stress is reminiscent of the (TNF-α)-induced breakdown of barrier failure in the corneal endothelium.

摘要

为了研究氧化应激对牛和猪眼角膜内皮细胞屏障功能的影响,我们进行了此项实验。氧化应激通过向细胞中添加核黄素(Rf)并使其暴露于 UV-A(15-30 分钟)来诱导产生 1 型光化学反应,从而释放 HO。通过跨内皮电阻(TER)测量来评估应激对屏障功能的影响。此外,通过免疫细胞化学评估微管、周细胞肌动球蛋白环(PAMR)和 ZO-1 的组织结构变化,HO(100μM,1 小时)直接暴露后也进行了重复评估。HO 的暴露导致微管解体和 PAMR 破坏。同时,ZO-1 的连续位置被破坏,标志着屏障完整性的丧失。因此,当富含 Rf 的培养基中的细胞暴露于 UV-A 时,会持续诱导 TER 丧失。然而,添加 7000U/ml 的过氧化氢酶可快速分解 HO,从而限制 TER 的丧失。此外,通过添加过氧化氢酶、抗坏血酸(1mM;30 分钟)或预处理 p38MAP 激酶抑制剂(SB-203580;10μM,1 小时),可抑制对微管、PAMR 和 ZO-1 的不利影响。急性氧化应激通过 p38MAP 激酶依赖性机制诱导微管解体,导致 PAMR 破坏和屏障功能丧失。这种对氧化应激的反应使人联想到 TNF-α 诱导的角膜内皮屏障功能障碍的破坏。

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