Vo Vu T A, Tran Le Nhat, Bui Thu Thanh, Lee Han-Woong, Jeong Yangsik
Department of Biochemistry, Wonju College of Medicine, Yonsei University, Wonju, Republic of Korea.
Department of Global Medical Science, Wonju College of Medicine, Yonsei University, Wonju, Republic of Korea.
Cell Mol Biol Lett. 2025 Apr 19;30(1):52. doi: 10.1186/s11658-025-00726-6.
Arginine auxotrophy has been reported in a subset of cancers with inherently defective de novo arginine synthesis. However, the use of arginine deprivation therapy seems to be unequally effective, partially owing to the resistance acquired by cancer cells. Study of underlying factors involved in this response thus becomes of utmost importance. Meanwhile, the function of etoposide-induced 2.4 homolog (EI24) in cancer metabolism, and specifically in arginine metabolism, remains unknown.
EI24 was overexpressed in cancer cells using a doxycycline-inducible system or adenovirus transduction, while siRNA was used to knockdown EI24. Amino acid(s) deprivation medium was exploited with a cell viability assay to check the reliance of cancer cell survival on arginine. Protein expression and activation were examined through western blot and co-immunoprecipitation blot. Furthermore, global and specific protein translation were assessed through the SUnSET assay and polysome fractionation analysis. Gene expression and arginine level were downloaded from public cancer datasets for in silico validation including gene set enrichment and survival analysis to objectively evaluate the association between EI24 and arginine metabolism.
EI24 promoted cancer survival under arginine starvation. Mechanistically, EI24 replenished translation of argininosuccinate synthase 1 (ASS1) by inducing the inactive S-nitrosylated form of phosphatase and tensin homolog (PTEN), leading to release of the phosphoinositide 3-kinase (PI3K)/protein kinase B (AKT) axis. This tumor-promoting action of EI24 could be found in multiple ASS1-deficient cancer cells regardless of p53 status. Furthermore, expression of EI24 was linked to enrichment of arginine metabolism pathway as well as poor survival of patients with cancer across various cancer types, suggesting its role in cancer resistance to arginine deprivation.
This study is the first to report the role of EI24 in promoting cancer survival via translational regulation of the metabolic enzyme ASS1, thus paving a route for further investigation into the link between EI24 and cancer metabolism.
在一部分从头合成精氨酸存在固有缺陷的癌症中,已报道有精氨酸营养缺陷。然而,精氨酸剥夺疗法的使用似乎效果不均,部分原因是癌细胞获得了耐药性。因此,研究参与这种反应的潜在因素变得至关重要。与此同时,依托泊苷诱导的2.4同源物(EI24)在癌症代谢,特别是精氨酸代谢中的功能仍然未知。
使用强力霉素诱导系统或腺病毒转导在癌细胞中过表达EI24,同时使用小干扰RNA(siRNA)敲低EI24。利用氨基酸剥夺培养基和细胞活力测定法来检查癌细胞存活对精氨酸的依赖性。通过蛋白质印迹和免疫共沉淀印迹检测蛋白质表达和激活情况。此外,通过SUnSET测定法和多核糖体分级分析评估整体和特定蛋白质翻译。从公共癌症数据集中下载基因表达和精氨酸水平用于计算机验证,包括基因集富集分析和生存分析,以客观评估EI24与精氨酸代谢之间的关联。
EI24在精氨酸饥饿条件下促进癌细胞存活。机制上,EI24通过诱导磷酸酶和张力蛋白同源物(PTEN)的无活性S-亚硝基化形式来补充精氨琥珀酸合酶1(ASS1)的翻译,从而导致磷酸肌醇3-激酶(PI3K)/蛋白激酶B(AKT)轴的释放。EI24的这种促肿瘤作用在多种ASS1缺陷的癌细胞中均可发现,与p53状态无关。此外,EI24的表达与精氨酸代谢途径的富集以及各种癌症类型患者的不良生存相关,表明其在癌症对精氨酸剥夺的抗性中发挥作用。
本研究首次报道了EI24通过对代谢酶ASS1的翻译调控促进癌细胞存活的作用,从而为进一步研究EI24与癌症代谢之间的联系铺平了道路。
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