Department of Anesthesiology, the 988th Hospital of Joint Logistic Support Force of Chinese People's Liberation Army, Zhengzhou 450042, Henan, China.
Department of Rheumatology and Immunology, Shanghai Changzheng Hospital, Second Affiliated Hospital of Naval Medical University, Shanghai, 200003, China.
Int Immunopharmacol. 2024 Feb 15;128:111474. doi: 10.1016/j.intimp.2023.111474. Epub 2024 Jan 6.
Hepatic ischemia-reperfusion injury (IRI) typically manifests during subtotal hepatectomy and inflicts substantial damage to liver function in the perioperative period. Although the central role of cGAS-STING-mediated immune inflammation in hepatocyte damage during hepatic IRI is acknowledged, the precise regulatory mechanisms remain elusive. The current study aims to elucidate how Sirt3 inhibition activates the cGAS-STING pathway and exacerbates hepatocyte damage in hepatic IRI. We established both in vivo and in vitro models by creating hepatic IRI mice model and subjecting AML-12 hepatocyte cell lines to oxygen-glucose deprivation/reperfusion (OGD/R). Hepatic IRI compromised liver and mitochondrial function while elevating cytosolic mitochondrial DNA (mtDNA) levels in hepatocytes. Additionally, both in vivo hepatic IRI and in vitro OGD/R induced increased phosphorylation and activation of cGAS, STING, and IRF3, accompanied by heightened levels of pro-inflammatory factors, including TNF-α, IL-1β, and type I interferon (IFN-β). Importantly, knockdown of cGAS or STING through siRNA effectively attenuated hepatic IRI-induced inflammation and ameliorated liver function in both experimental settings, underscoring the dynamic involvement of the cGAS-STING pathway in hepatic IRI-induced inflammation. Furthermore, we observed a significant reduction in Sirt3 expression following hepatic IRI, both in vivo and in vitro. Then we generated Sirt3-deficient mice and applied Sirt3 knockdown in AML-12 hepatocytes. Notably, Sirt3 deficiency led to increased phosphorylation and activation of cGAS, STING, and IRF3, coupled with elevated TNF-α, IL-1β, and IFN-β levels in both in vivo and in vitro conditions. Moreover, upon silencing various downstream targets of Sirt3, such as transcription factors Sp1, Pu1, and p65, we observed that specifically knocking down p65 in AML-12 hepatocytes reduced cGAS mRNA levels. Co-immunoprecipitation assays confirmed a direct interaction between Sirt3 and p65. The absence of Sirt3 significantly increased nuclear translocation of p65 in mice, whereas Sirt3 knockdown in AML-12 hepatocytes heightened nuclear translocation of p65. ChIP-PCR assays demonstrated that Sirt3 deficiency notably enhanced the binding of p65 to two cGAS promoters, ultimately promoting cGAS transcription. Collectively, our results underscored that inhibition of Sirt3 activates the cGAS-STING pathway to aggravate hepatocyte damage by increasing cytosolic mtDNA and promoting nuclear translocation of p65 to promote cGAS transcription in hepatic IRI. These findings hold promise for potential therapeutic interventions in hepatic IRI by targeting the Sirt3-cGAS-STING axis, offering new avenues for the development of clinical strategies to mitigate liver damage during the perioperative period.
肝缺血再灌注损伤(IRI)通常在部分肝切除术中表现出来,并在围手术期对肝功能造成严重损害。尽管 cGAS-STING 介导的免疫炎症在肝 IRI 期间肝细胞损伤中的核心作用已得到认可,但确切的调节机制仍不清楚。本研究旨在阐明 Sirt3 抑制如何激活 cGAS-STING 途径并加剧肝 IRI 中的肝细胞损伤。我们通过建立肝 IRI 小鼠模型和使 AML-12 肝细胞系经历氧葡萄糖剥夺/再灌注(OGD/R)来建立体内和体外模型。肝 IRI 损害了肝脏和线粒体功能,同时增加了肝细胞中胞质线粒体 DNA(mtDNA)水平。此外,体内肝 IRI 和体外 OGD/R 均诱导 cGAS、STING 和 IRF3 的磷酸化和激活增加,并伴有促炎因子 TNF-α、IL-1β 和 I 型干扰素(IFN-β)水平升高。重要的是,通过 siRNA 敲低 cGAS 或 STING 可有效减轻两种实验模型中肝 IRI 诱导的炎症并改善肝功能,突出了 cGAS-STING 途径在肝 IRI 诱导的炎症中的动态作用。此外,我们观察到在体内和体外肝 IRI 后 Sirt3 的表达均显著降低。然后,我们生成了 Sirt3 缺陷型小鼠并在 AML-12 肝细胞中应用 Sirt3 敲低。值得注意的是,Sirt3 缺陷导致 cGAS、STING 和 IRF3 的磷酸化和激活增加,并伴有体内和体外条件下 TNF-α、IL-1β 和 IFN-β 水平升高。此外,在沉默 Sirt3 的各种下游靶标(如转录因子 Sp1、Pu1 和 p65)后,我们观察到仅在 AML-12 肝细胞中敲低 p65 可降低 cGAS mRNA 水平。免疫共沉淀实验证实了 Sirt3 和 p65 之间的直接相互作用。Sirt3 缺失显著增加了小鼠中 p65 的核易位,而 AML-12 肝细胞中 Sirt3 的敲低增加了 p65 的核易位。ChIP-PCR 实验表明,Sirt3 缺失显著增强了 p65 与两个 cGAS 启动子的结合,最终促进了 cGAS 转录。总之,我们的结果强调了 Sirt3 的抑制通过增加胞质 mtDNA 并促进核易位来激活 cGAS-STING 途径,从而加剧肝细胞损伤,以促进 cGAS 转录,从而在肝 IRI 中加重肝细胞损伤。这些发现为通过靶向 Sirt3-cGAS-STING 轴治疗肝 IRI 提供了希望,为减轻围手术期肝损伤的临床策略的发展提供了新途径。
