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白藜芦醇靶向MDM2/P53/PUMA轴抑制葡聚糖硫酸钠诱导的溃疡性结肠炎小鼠结肠细胞凋亡

Resveratrol targeting MDM2/P53/PUMA axis to inhibit colonocyte apoptosis in DSS-induced ulcerative colitis mice.

作者信息

Tang Rui, Jiang Ling, Ji Quan, Kang Pengyuan, Liu Yuan, Miao Pengyu, Xu Xiaofan, Tang Mingxi

机构信息

Department of Pathology, Yaan People's Hospital, Yaan, China.

School of Basic Medical Sciences, Southwest Medical University, Luzhou, China.

出版信息

Front Pharmacol. 2025 Apr 30;16:1572906. doi: 10.3389/fphar.2025.1572906. eCollection 2025.

Abstract

BACKGROUND

Resveratrol, a naturally occurring polyphenolic compound found in grapes, berries, and traditional medicinal plants like Polygonum cuspidatum, has been used for centuries in traditional medicine systems for its anti-inflammatory, antioxidant, and cardioprotective properties. Ulcerative colitis (UC), a chronic inflammatory bowel disease, is characterized by intestinal barrier disruption due to excessive colonocyte apoptosis, leading to increased permeability and inflammation. Targeting apoptosis is a critical therapeutic strategy for UC.

AIM OF THE STUDY

This study aims to investigate the therapeutic potential of Resveratrol in ulcerative colitis (UC) by targeting excessive colonocyte apoptosis and intestinal barrier dysfunction. Specifically, we seek to elucidate the mechanisms through which Resveratrol modulates apoptosis-related pathways and evaluate its efficacy in restoring intestinal homeostasis and mitigating UC progression in both and models.

MATERIALS AND METHODS

We used dextran sulfate sodium (DSS) to induce UC in a mouse model. Colonic damage was assessed through colonic length measurement, histological examination, and immunofluorescence staining. Single-cell sequencing was employed to explore changes in the colonic immune microenvironment and cellular signaling pathways after Resveratrol treatment. , colonocytes isolated from healthy mouse colonic tissue were exposed to TGF-β to induce apoptosis. DNA fragmentation, mitochondrial membrane potential, and annexin V/propidium iodide staining were used to assess apoptosis. Additionally, we employed an Adeno-Associated Virus system to overexpress MDM2 in the colon and evaluate its protective role in DSS-induced UC.

RESULTS

Resveratrol treatment effectively repaired colonic damage in the UC mouse model by significantly increasing colon length, reducing inflammatory cell infiltration, and mitigating mucosal injury. Single-cell sequencing revealed that Resveratrol primarily targeted colonocytes, decreasing genes related to apoptosis and the P53 pathway. , Resveratrol reduced DNA fragmentation, apoptotic cell populations, and increased mitochondrial membrane potential in a dose-dependent manner. Furthermore, Resveratrol increased MDM2 expression, inhibiting P53 and downstream pro-apoptotic signaling. Nutlin-3a, an MDM2 inhibitor, reversed the anti-apoptotic effects of Resveratrol. Overexpression of MDM2 in the colon protected against DSS-induced damage.

CONCLUSION

Resveratrol is an effective treatment for DSS-induced UC, primarily by inhibiting excessive apoptosis in colonocytes through the MDM2/P53/PUMA axis. MDM2 presents a promising therapeutic target for UC treatment.

摘要

背景

白藜芦醇是一种天然存在的多酚化合物,存在于葡萄、浆果以及虎杖等传统药用植物中,几个世纪以来,它因其抗炎、抗氧化和心脏保护特性而被用于传统医学体系。溃疡性结肠炎(UC)是一种慢性炎症性肠病,其特征是由于结肠细胞过度凋亡导致肠道屏障破坏,进而导致通透性增加和炎症。针对细胞凋亡是UC的关键治疗策略。

研究目的

本研究旨在通过针对过度的结肠细胞凋亡和肠道屏障功能障碍来研究白藜芦醇在溃疡性结肠炎(UC)中的治疗潜力。具体而言,我们试图阐明白藜芦醇调节凋亡相关途径的机制,并评估其在恢复肠道稳态和减轻UC在体内和体外模型中进展方面的疗效。

材料与方法

我们使用葡聚糖硫酸钠(DSS)在小鼠模型中诱导UC。通过测量结肠长度、组织学检查和免疫荧光染色来评估结肠损伤。采用单细胞测序来探索白藜芦醇治疗后结肠免疫微环境和细胞信号通路的变化。此外,从健康小鼠结肠组织中分离出的结肠细胞暴露于转化生长因子-β(TGF-β)以诱导细胞凋亡。使用DNA片段化、线粒体膜电位和膜联蛋白V/碘化丙啶染色来评估细胞凋亡。另外,我们采用腺相关病毒系统在结肠中过表达MDM2,并评估其在DSS诱导的UC中的保护作用。

结果

白藜芦醇治疗通过显著增加结肠长度、减少炎症细胞浸润和减轻粘膜损伤,有效修复了UC小鼠模型中的结肠损伤。单细胞测序显示,白藜芦醇主要靶向结肠细胞,减少与细胞凋亡和P53途径相关的基因。此外,白藜芦醇以剂量依赖的方式减少DNA片段化、凋亡细胞群体并增加线粒体膜电位。此外,白藜芦醇增加MDM2表达,抑制P53及其下游促凋亡信号。MDM2抑制剂Nutlin-3a逆转了白藜芦醇的抗凋亡作用。结肠中MDM2的过表达对DSS诱导的损伤具有保护作用。

结论

白藜芦醇是DSS诱导的UC的有效治疗方法,主要通过MDM2/P53/PUMA轴抑制结肠细胞中的过度凋亡。MDM2是UC治疗中一个有前景的治疗靶点。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3dd7/12075554/86addc269164/fphar-16-1572906-g001.jpg

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