cGAS regulates metabolic reprogramming independently of STING pathway in colorectal cancer

IF 3.3 3区 生物学 Q3 CELL BIOLOGY Experimental cell research Pub Date : 2024-11-01 DOI:10.1016/j.yexcr.2024.114316
Fan Wang , Chao Jiang , Hong-Xia Hui , Ming-Yue Tao , Hai-Xiao Wang , Yuan Sun , Jing Zhu
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Abstract

Background

Cyclic GMP-AMP synthase (cGAS) is widely acknowledged for detecting cytosolic chromatin fragments and triggering innate immune responses through the production of the second messenger cGAMP, which subsequently activates the adaptor protein STING. However, the role of cGAS in regulating metabolic reprogramming independently of STING activation has not yet been explored.

Methods

Gene set enrichment pathway analysis (GSEA) based on TCGA transcriptomics, combined with Seahorse metabolic analysis of CRC cell lines and human normal colonic mucosa cell line FHC, was performed to profile the metabolic features in CRC. cGAS doxycycline- (dox) inducible knockout (iKO) CRC sublines were generated to investigate the role of cGAS in CRC. Transcriptome and proteome data from COAD cohorts were utilized to evaluate the RNA and protein expression levels of cGAS in COAD tissues and normal colon tissues. Overall survival information of patients with COAD was used to evaluate the prognostic value of cGAS expression. Colony formation assays were conducted to evaluate the clonogenicity of CRC cells under different situations. Flow cytometry detecting the signal of fluorogenic reactive oxygen species (ROS) probes was performed to evaluate the total cellular and mitochondrial oxidative stress level in CRC cells. A propidium iodide (PI) staining assay was used to evaluate the cell death level in CRC cells. Quantitative PCR (qPCR) was conducted to detect the RNA level of STING pathway downstream target genes. Mass spectrometry was used for the identification of novel binding partners of cGAS in CRC cells. Co-immunoprecipitation (co-IP) was conducted to confirm the interaction between cGAS and NDUFA4L2.

Results

By integrating metabolic pathway analysis based on TCGA transcriptomics with Seahorse metabolic analysis of a panel CRC cell lines and the human normal colonic mucosa cell line FHC, we demonstrated that CRC cells exhibit typical characteristics of metabolic reprogramming, characterized by a shift from oxidative phosphorylation (OXPHOS) to glycolysis. We found that cGAS is critical for CRC cells to maintain this metabolic switch. Specifically, the suppression of cGAS through siRNA-mediated knockdown or doxycycline-inducible knockout reversed this metabolic switch, resulting in increased OXPHOS activity, elevated production of OXPHOS byproduct reactive oxygen species (ROS), and consequently caused oxidative stress. This disruption induced oxidative stress, ultimately resulting in cell death and reduced cell viability. Moreover, significant upregulation of cGAS in CRC tissues and cell lines and its association with poor prognosis in CRC patients was observed. Subsequently, we demonstrated that the role of cGAS in regulating metabolic reprogramming does not rely on the canonical cGAS-STING pathway. Co-immunoprecipitation combined with mass spectrometry identified NDUFA4L2 as a novel interactor of cGAS. Subsequent functional experiments, including mitochondrial respiration and oxidative stress assays, demonstrated that cGAS plays a crucial role in sustaining elevated levels of NDUFA4L2 protein expression. The increased expression of NDUFA4L2 is essential for cGAS-mediated regulation of metabolic reprogramming and cell survival in CRC cells.

Conclusion

cGAS regulates metabolic reprogramming and promotes cell survival in CRC cells through its interaction with NDUFA4L2, independently of the canonical cGAS-STING pathway.
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cGAS 可独立于 STING 通路调控结直肠癌的代谢重编程。
背景:人们普遍认为环GMP-AMP合成酶(cGAS)可检测细胞染色质片段,并通过产生第二信使cGAMP触发先天性免疫反应,进而激活适配蛋白STING。然而,cGAS 在 STING 激活之外调节代谢重编程的作用尚未得到探讨:方法:基于TCGA转录组学的基因组富集通路分析(Gene set enrichment pathway analysis,GSEA),结合对CRC细胞系和人类正常结肠粘膜细胞系FHC的Seahorse代谢分析,分析了CRC的代谢特征。利用 COAD 队列中的转录组和蛋白质组数据评估了 cGAS 在 COAD 组织和正常结肠组织中的 RNA 和蛋白质表达水平。利用 COAD 患者的总体生存信息评估 cGAS 表达的预后价值。通过集落形成试验评估不同情况下 CRC 细胞的克隆性。检测荧光活性氧探针信号的流式细胞术用于评估 CRC 细胞的总细胞和线粒体氧化应激水平。碘化丙啶(PI)染色法用于评估 CRC 细胞的细胞死亡水平。定量 PCR(qPCR)检测 STING 通路下游靶基因的 RNA 水平。质谱法用于鉴定 cGAS 在 CRC 细胞中的新型结合伙伴。共免疫沉淀(co-immunoprecipitation,co-IP)证实了cGAS与NDUFA4L2之间的相互作用:通过将基于 TCGA 转录组学的代谢通路分析与对 CRC 细胞系和人类正常结肠粘膜细胞系 FHC 的海马代谢分析相结合,我们发现 CRC 细胞表现出典型的代谢重编程特征,即从氧化磷酸化(OXPHOS)转向糖酵解。我们发现,cGAS 对 CRC 细胞维持这种代谢转换至关重要。具体来说,通过 siRNA 介导的基因敲除或强力霉素诱导的基因敲除抑制 cGAS,可逆转这种代谢转换,导致 OXPHOS 活性增加、OXPHOS 副产物活性氧(ROS)生成增加,从而引起氧化应激。这种破坏诱导了氧化应激,最终导致细胞死亡和细胞活力降低。此外,还观察到 cGAS 在 CRC 组织和细胞系中明显上调,并与 CRC 患者的不良预后有关。随后,我们证明了cGAS在调节代谢重编程中的作用并不依赖于典型的cGAS-STING途径。共免疫沉淀结合质谱鉴定出 NDUFA4L2 是 cGAS 的新型互作因子。随后进行的功能实验(包括线粒体呼吸和氧化应激实验)证明,cGAS 在维持 NDUFA4L2 蛋白表达水平的升高中起着至关重要的作用。结论:cGAS通过与NDUFA4L2的相互作用调控CRC细胞的代谢重编程并促进细胞存活,而不依赖于典型的cGAS-STING通路。
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
Experimental cell research
Experimental cell research 医学-细胞生物学
CiteScore
7.20
自引率
0.00%
发文量
295
审稿时长
30 days
期刊介绍: Our scope includes but is not limited to areas such as: Chromosome biology; Chromatin and epigenetics; DNA repair; Gene regulation; Nuclear import-export; RNA processing; Non-coding RNAs; Organelle biology; The cytoskeleton; Intracellular trafficking; Cell-cell and cell-matrix interactions; Cell motility and migration; Cell proliferation; Cellular differentiation; Signal transduction; Programmed cell death.
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