Mitochondrial damage causes inflammation via cGAS-STING signaling in ketamine-induced cystitis.

IF 4.8 3区医学 Q2 CELL BIOLOGY

Inflammation Research Pub Date : 2025-01-07 DOI:10.1007/s00011-024-01973-7

Jinji Chen, Shengsheng Liang, Cheng Li, Bowen Li, Mingdong He, Kezhen Li, Weijin Fu, Shenghua Li, Hua Mi

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Abstract

Background: Mitochondrial dysfunction and damage can result in the release of mitochondrial DNA (mtDNA) into the cytoplasm, which subsequently activates the cGAS-STING pathway, promoting the onset of inflammatory diseases. Various factors, such as oxidative stress, viral infection, and drug toxicity, have been identified as inducers of mitochondrial damage. This study aims to investigate the role of mtDNA as a critical inflammatory mediator in the pathogenesis of ketamine (KET)-induced cystitis (KC) through the cGAS-STING pathway.

Methods: To investigate the role of the cGAS-STING pathway in KET-induced cystitis, we assessed the expression of cGAS and STING in rats with KET cystitis. Additionally, we evaluated STING expression in conditionally deficient Simian Virus-transformed Human Uroepithelial Cell Line 1 (SV-HUC-1) cells in vitro. Morphological changes in mitochondria were examined using transmission electron microscopy. We measured intracellular reactive oxygen species (ROS) production through flow cytometry and immunofluorescence techniques. Furthermore, alterations in associated inflammatory factors and cytokines were quantified using real-time quantitative PCR with fluorescence detection.

Results: We observed up-regulation of cGAS and STING expressions in the bladder tissue of rats in the KET group, stimulation with KET also led to increased cGAS and STING levels in SV-HUC-1 cells. Notably, the knockdown of STING inhibited the nuclear translocation of NF-κB p65 and IRF3, resulting in a decrease in the expression of inflammatory cytokines, including IL-6, IL-8, and CXCL10. Additionally, KET induced damage to the mitochondria of SV-HUC-1 cells, facilitating the release of mtDNA into the cytoplasm. This significant depletion of mtDNA inhibited the activation of cGAS-STING pathway, subsequently affecting the expression of NF-κB p65 and IRF3. Importantly, the reintroduction of mtDNA after STING knockdown partially restored the inflammatory response.

Conclusion: Our findings confirmed the activation of the cGAS-STING pathway in KC rats and revealed mitochondrial damage in vitro. These results highlight the involvement of the cGAS-STING pathway in the pathogenesis of KC, suggesting its potential as a therapeutic target for intervention.

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背景：线粒体功能障碍和损伤可导致线粒体 DNA（mtDNA）释放到细胞质中，进而激活 cGAS-STING 通路，促进炎症性疾病的发生。氧化应激、病毒感染和药物毒性等多种因素已被确定为线粒体损伤的诱导因素。本研究旨在通过 cGAS-STING 通路研究 mtDNA 作为关键炎症介质在氯胺酮（KET）诱导的膀胱炎（KC）发病机制中的作用：为了研究 cGAS-STING 通路在 KET 诱导的膀胱炎中的作用，我们评估了 KET 膀胱炎大鼠体内 cGAS 和 STING 的表达。此外，我们还在体外评估了STING在条件性缺失的人泌尿上皮细胞系1（SV-HUC-1）细胞中的表达。我们使用透射电子显微镜检查了线粒体的形态变化。我们通过流式细胞术和免疫荧光技术测量了细胞内活性氧（ROS）的产生。此外，我们还利用荧光检测实时定量 PCR 技术量化了相关炎症因子和细胞因子的变化：结果：我们观察到 KET 组大鼠膀胱组织中 cGAS 和 STING 表达上调，KET 刺激也导致 SV-HUC-1 细胞中 cGAS 和 STING 水平升高。值得注意的是，STING 的敲除抑制了 NF-κB p65 和 IRF3 的核转位，导致炎性细胞因子（包括 IL-6、IL-8 和 CXCL10）的表达减少。此外，KET 还会对 SV-HUC-1 细胞的线粒体造成损伤，促进 mtDNA 释放到细胞质中。这种 mtDNA 的大量消耗抑制了 cGAS-STING 通路的激活，随后影响了 NF-κB p65 和 IRF3 的表达。重要的是，STING敲除后重新引入mtDNA可部分恢复炎症反应：我们的研究结果证实了 KC 大鼠体内 cGAS-STING 通路的激活，并在体外发现了线粒体损伤。这些结果突显了 cGAS-STING 通路参与了 KC 的发病机制，并表明其有可能成为干预治疗的靶点。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Inflammation Research 医学-免疫学

CiteScore

9.90

自引率

1.50%

发文量

134

审稿时长

3-8 weeks

期刊介绍： Inflammation Research (IR) publishes peer-reviewed papers on all aspects of inflammation and related fields including histopathology, immunological mechanisms, gene expression, mediators, experimental models, clinical investigations and the effect of drugs. Related fields are broadly defined and include for instance, allergy and asthma, shock, pain, joint damage, skin disease as well as clinical trials of relevant drugs.

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