a Department of Pharmacology, Manipal College of Pharmaceutical Sciences , Manipal Academy of Higher Education , Manipal , India.
b Oxidative Stress Laboratory, Basic Science Domain , Baker Heart and Diabetes Institute , Melbourne , Australia.
Free Radic Res. 2018 Oct;52(10):1140-1157. doi: 10.1080/10715762.2018.1533636. Epub 2018 Nov 13.
Inflammation is a protective immune response against invading pathogens, however, dysregulated inflammation is detrimental. As the complex inflammatory response involves multiple mediators, including the involvement of reactive oxygen species, concomitantly targeting proinflammatory and antioxidant check-points may be a more rational strategy. We report the synthesis and anti-inflammatory/antioxidant activity of a novel indanedione derivative DMFO. DMFO scavenged reactive oxygen species (ROS) in radical scavenging assays and in lipopolysaccharide (LPS)-stimulated RAW 264.7 macrophages. In acute models of inflammation (carrageenan-induced inflammation in rat paw and air pouch), DMFO effectively reduced paw oedema and leucocyte infiltration with an activity comparable to diclofenac. DMFO stabilised mast cells (MCs) in A23187 and compound 48/80-induced assays. Additionally, DMFO stabilised MCs in an antigen (ovalbumin)-induced MC degranulation model , without affecting serum IgE levels. In a model of chronic immune-mediated inflammation, Freund's adjuvant-induced arthritis, DMFO reduced arthritic score and contralateral paw oedema, and increased the pain threshold with an efficacy comparable to diclofenac but without being ulcerogenic. Additionally, DMFO significantly reduced serum TNFα levels. Mechanistic studies revealed that DMFO reduced proinflammatory genes (IL1β, TNFα, IL6) and protein levels (COX2, MCP1), with a concurrent increase in antioxidant genes (NQO1, haem oxygenase 1 (HO-1), Glo1, Nrf2) and protein (HO-1) in LPS-stimulated macrophages. Importantly, the anti-inflammatory/antioxidant effect on gene expression was absent in primary macrophages isolated from Nrf2 KO mice suggesting an Nrf2-targeted activity, which was subsequently confirmed using siRNA transfection studies in RAW macrophages. Therefore, DMFO is a novel, orally-active, safe (even at 2 g/kg p.o.), a small molecule which targets Nrf2 in ameliorating inflammation.
炎症是一种针对入侵病原体的保护性免疫反应,然而,失调的炎症是有害的。由于复杂的炎症反应涉及多种介质,包括活性氧的参与,同时针对促炎和抗氧化检查点可能是一种更合理的策略。我们报告了一种新型茚二酮衍生物 DMFO 的合成及其抗炎/抗氧化活性。DMFO 在自由基清除测定和脂多糖 (LPS) 刺激的 RAW 264.7 巨噬细胞中清除活性氧 (ROS)。在急性炎症模型(大鼠爪角叉菜胶炎症和气囊)中,DMFO 有效减少爪水肿和白细胞浸润,其活性与双氯芬酸相当。DMFO 在 A23187 和化合物 48/80 诱导的测定中稳定肥大细胞 (MCs)。此外,DMFO 在抗原(卵清蛋白)诱导的 MC 脱颗粒模型中稳定 MC,而不影响血清 IgE 水平。在慢性免疫介导的炎症模型中,弗氏完全佐剂诱导的关节炎,DMFO 降低关节炎评分和对侧爪水肿,并增加疼痛阈值,其疗效与双氯芬酸相当,但无溃疡形成。此外,DMFO 显著降低血清 TNFα 水平。机制研究表明,DMFO 降低促炎基因 (IL1β、TNFα、IL6) 和蛋白水平 (COX2、MCP1),同时增加抗氧化基因 (NQO1、血红素加氧酶 1 (HO-1)、Glo1、Nrf2) 和 LPS 刺激巨噬细胞中的蛋白 (HO-1)。重要的是,在从 Nrf2 KO 小鼠分离的原代巨噬细胞中,对基因表达的抗炎/抗氧化作用缺失,这表明 DMFO 具有 Nrf2 靶向活性,随后使用 RAW 巨噬细胞中的 siRNA 转染研究得到证实。因此,DMFO 是一种新型的、口服活性的、安全的(即使口服 2g/kg 也安全)、小分子,可通过改善炎症来靶向 Nrf2。
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