SARS-CoV-2 病毒穿孔蛋白通过线粒体通透性转换孔激活 NLRP3 炎症小体。
SARS-COV-2 viroporins activate the NLRP3-inflammasome by the mitochondrial permeability transition pore.
机构信息
Center for Mitochondrial and Epigenomic Medicine, Division of Human Genetics, The Children's Hospital of Philadelphia, Philadelphia, PA, United States.
Department of biology, University of Pennsylvania, Philadelphia, PA, United States.
出版信息
Front Immunol. 2023 Feb 20;14:1064293. doi: 10.3389/fimmu.2023.1064293. eCollection 2023.
BACKGROUND
Compared to healthy controls, severe COVID19 patients display increased levels of activated NLRP3-inflammasome (NLRP3-I) and interleukin (IL)-1β. SARS-CoV-2 encodes viroporin proteins E and Orf3a(2-E+2-3a) with homologs to SARS-CoV-1, 1-E+1-3a, which elevate NLRP3-I activation; by an unknown mechanism. Thus, we investigated how 2-E+2-3a activates the NLRP3-I to better understand the pathophysiology of severe COVID-19.
METHODS
We generated a polycistronic expression-vector co-expressing 2-E+2-3a from a single transcript. To elucidate how 2-E+2-3a activates the NLRP3-I, we reconstituted the NLRP3-I in 293T cells and used THP1-derived macrophages to monitor the secretion of mature IL-1β. Mitochondrial physiology was assessed using fluorescent microscopy and plate reader assays, and the release of mitochondrial DNA (mtDNA) was detected from cytosolic-enriched fractions using Real-Time PCR.
RESULTS
Expression of 2-E+2-3a in 293T cells increased cytosolic Ca++ and elevated mitochondrial Ca++, taken up through the MCUi11-sensitive mitochondrial calcium uniporter. Increased mitochondrial Ca++ stimulated NADH, mitochondrial reactive oxygen species (mROS) production and the release of mtDNA into the cytosol. Expression of 2-E+2-3a in NLRP3-I reconstituted 293T cells and THP1-derived macrophages displayed increased secretion of IL-1β. Increasing mitochondrial antioxidant defenses via treatment with MnTBAP or genetic expression of mCAT abolished 2-E+2-3a elevation of mROS, cytosolic mtDNA levels, and secretion of NLRP3-activated-IL-1β. The 2-E+2-3a-induced release of mtDNA and the secretion of NLRP3-activated-IL-1β were absent in cells lacking mtDNA and blocked in cells treated with the mitochondrial-permeability-pore(mtPTP)-specific inhibitor NIM811.
CONCLUSION
Our findings revealed that mROS activates the release of mitochondrial DNA via the NIM811-sensitive mitochondrial-permeability-pore(mtPTP), activating the inflammasome. Hence, interventions targeting mROS and the mtPTP may mitigate the severity of COVID-19 cytokine storms.
背景
与健康对照组相比,严重 COVID19 患者的活化 NLRP3-炎症小体(NLRP3-I)和白细胞介素(IL)-1β水平升高。SARS-CoV-2 编码的 viroporin 蛋白 E 和 Orf3a(2-E+2-3a)与 SARS-CoV-1 的 1-E+1-3a 具有同源性,它们可通过未知机制升高 NLRP3-I 的激活。因此,我们研究了 2-E+2-3a 如何激活 NLRP3-I,以更好地了解严重 COVID-19 的病理生理学。
方法
我们从单个转录本生成了一个共表达 2-E+2-3a 的多顺反子表达载体。为了阐明 2-E+2-3a 如何激活 NLRP3-I,我们在 293T 细胞中重建了 NLRP3-I,并使用 THP1 衍生的巨噬细胞来监测成熟的 IL-1β 的分泌。使用荧光显微镜和板读数仪评估线粒体生理学,并使用实时 PCR 从细胞溶质浓缩部分检测线粒体 DNA(mtDNA)的释放。
结果
293T 细胞中 2-E+2-3a 的表达增加了细胞溶质 Ca++,并通过 MCUi11 敏感的线粒体钙单向转运体升高了线粒体 Ca++。增加的线粒体 Ca++刺激 NADH、线粒体活性氧(mROS)的产生,并将 mtDNA 释放到细胞质中。在 NLRP3-I 重建的 293T 细胞和 THP1 衍生的巨噬细胞中表达 2-E+2-3a 可增加 IL-1β 的分泌。通过用 MnTBAP 处理或通过基因表达 mCAT 增加线粒体抗氧化防御,可消除 2-E+2-3a 升高的 mROS、细胞质 mtDNA 水平和 NLRP3 激活的-IL-1β 的分泌。缺乏 mtDNA 的细胞中不存在 2-E+2-3a 诱导的 mtDNA 释放和 NLRP3 激活的-IL-1β 的分泌,并且在用线粒体通透性孔(mtPTP)特异性抑制剂 NIM811 处理的细胞中被阻断。
结论
我们的研究结果表明,mROS 通过 NIM811 敏感的线粒体通透性孔(mtPTP)激活线粒体 DNA 的释放,从而激活炎症小体。因此,靶向 mROS 和 mtPTP 的干预措施可能减轻 COVID-19 细胞因子风暴的严重程度。
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