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莫林补充剂调节 UPR 的 PERK 分支,并减轻实验大鼠结肠中 1,2-二甲基肼诱导的血管生成和氧化应激。

Morin supplementation modulates PERK branch of UPR and mitigates 1,2-dimethylhydrazine-induced angiogenesis and oxidative stress in the colon of experimental rats.

机构信息

School of Chemical and Biotechnology, SASTRA Deemed University, Thanjavur, India.

Department of Biochemistry and Biotechnology, Faculty of Science, Annamalai University, Annamalai Nagar, India.

出版信息

Toxicol Mech Methods. 2020 May;30(4):306-315. doi: 10.1080/15376516.2020.1727596. Epub 2020 Feb 20.

DOI:10.1080/15376516.2020.1727596
PMID:32028820
Abstract

Angiogenesis, disturbance in redox homeostasis, and deregulated redox signaling are considered as common hallmarks of cancer progression and chemo resistance. In this context, PERK (protein kinase PKR-like ER kinase) branch of the unfolded protein response (UPR), an adaptive mechanism triggered by endoplasmic reticulum (ER) stress to cope with protein misfolding and perturbed proteostasis, has shown to regulate angiogenesis and oxidative stress. This study aimed to investigate the impact of morin, a poly phenolic compound from the family of on PERK-Nrf2-VEGF axis in experimental rats challenged with the colon specific procarcinogen 1,2-dimethylhydrazine (DMH). Male albino Wistar rats were randomized into four groups ( = 6) viz., control, morin control, DMH control, and DMH administered rats treated with morin. Immunohistochemical analysis of colonic cross-section revealed that DMH alone administered rats showed significantly increased expression of Nrf2 predominantly in the cytoplasm. Angiogenic growth factors viz., VEGF, PDGF, and bFGF are also shown to be increased in the DMH alone administered tumor bearing rats as compared to control. Significant downregulation was also observed in the downstream targets of Nrf2 such as hemeoxygenase 1 (HO1), glutathione peroxidase 2 (GPX2), thioredoxin (TRXN), glutathione S transferase (GST), and uridine glucuronyl transferase (UGT) as evidenced by the qPCR analysis. Immunoblot analysis revealed that onset of oxidative stress and angiogenesis in the colon of DMH alone administered rats were due to downregulation of pPERK along with its downstream targets such as peIF2α and CHOP. Supplementation of morin reversed the DMH-induced alterations and suppresses oxidative stress and angiogenesis via PERK phosphorylation.

摘要

血管生成、氧化还原稳态失调和失调的氧化还原信号转导被认为是癌症进展和化疗耐药的共同特征。在这种情况下,未折叠蛋白反应 (UPR) 的 PERK(蛋白激酶 PKR 样内质网激酶)分支是一种适应性机制,由内质网 (ER) 应激触发,以应对蛋白质错误折叠和蛋白质稳态失调,已显示可调节血管生成和氧化应激。本研究旨在研究 morin(多酚家族的一种化合物)对实验大鼠中 PERK-Nrf2-VEGF 轴的影响,这些大鼠受到结肠特异性前致癌物 1,2-二甲基肼 (DMH) 的挑战。雄性白化 Wistar 大鼠随机分为四组(每组 6 只):对照组、morin 对照组、DMH 对照组和 DMH 给药大鼠用 morin 治疗。对结肠切片的免疫组织化学分析表明,单独给予 DMH 的大鼠表现出 Nrf2 的表达明显增加,主要在细胞质中。血管生成生长因子,如 VEGF、PDGF 和 bFGF,在单独给予 DMH 的肿瘤荷瘤大鼠中也显示出增加,与对照组相比。通过 qPCR 分析还观察到 Nrf2 的下游靶标如血红素加氧酶 1 (HO1)、谷胱甘肽过氧化物酶 2 (GPX2)、硫氧还蛋白 (TRXN)、谷胱甘肽 S 转移酶 (GST) 和尿苷葡萄糖醛酸转移酶 (UGT) 的显著下调。免疫印迹分析表明,单独给予 DMH 的大鼠结肠中氧化应激和血管生成的发生是由于 pPERK 及其下游靶标如 peIF2α 和 CHOP 的下调。morin 的补充逆转了 DMH 诱导的改变,并通过 PERK 磷酸化抑制氧化应激和血管生成。

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