Key Laboratory of Experimental Marine Biology, Institute of Oceanology, Chinese Academy of Sciences, Qingdao, China.
Laboratory for Marine Biology and Biotechnology, Qingdao National Laboratory for Marine Science and Technology, Qingdao, China.
FASEB J. 2019 Sep;33(9):10089-10103. doi: 10.1096/fj.201802619RR. Epub 2019 Jun 14.
Sorafenib is a multikinase inhibitor that is effective in treating advanced liver cancer. Although its mechanism of action through several established cancer-related protein kinase targets is well-characterized, sorafenib induces variable responses among human tumors, and the cause for this variation is yet unknown. To investigate the underlying mechanisms, we applied mass spectrometry-based proteomic analysis to Huh7.5 human liver cancer cells and found that sorafenib significantly affected the expression of the key lipogenic enzymes, especially stearoyl coenzyme A desaturase 1 (SCD1), in these cells. Given that SCD1 catalyzes the most crucial and rate-limiting step in the synthesis of monounsaturated fatty acids (FAs), we performed a lipidomic analysis, which showed a dramatically altered lipid profile in sorafenib-treated cells. Detection and analysis of free FAs showed that the levels of monounsaturated FAs, including oleate, were significantly decreased in those cells treated by sorafenib. Addition of oleate protected liver cancer cells from sorafenib-induced death and alleviated the abnormalities of mitochondrial morphology and function caused by the drug. Treatment with sorafenib suppressed ATP production, resulting in AMPK activation phosphorylation. Further secondary effects included reduction of the levels of sterol regulatory element-binding protein 1 (SREBP1) and the phosphorylation of mammalian target of rapamycin (mTOR) in liver cancer cells. These effects were partly abolished in the presence of compound C (an AMPK inhibitor) and ATP and adenosine, and SREBP1c overexpression also could be resistant to the effects of sorafenib, suggesting that the sorafenib-induced reduction in cell viability was mediated by the ATP-AMPK-mTOR-SREBP1 signaling pathway. Taken together, our results suggest that sorafenib's anticancer activity in liver cancer cells is based on the inhibition of ATP production, SCD1 expression, and monounsaturated FA synthesis. In addition, the decreased monounsaturated FA synthesis further triggered the more serious reduction of ATP production in sorafenib-treated cells. To our knowledge, this is the first evidence that sorafenib disrupts lipogenesis and triggers liver cancer cell death by targeting SCD1 through the ATP-AMPK-mTOR-SREBP1 pathway.-Liu, G., Kuang, S., Cao, R., Wang, J., Peng, Q., Sun, C. Sorafenib kills liver cancer cells by disrupting SCD1-mediated synthesis of monounsaturated fatty acids the ATP-AMPK-mTOR- SREBP1 signaling pathway.
索拉非尼是一种多激酶抑制剂,可有效治疗晚期肝癌。虽然其通过几种已确定的与癌症相关的蛋白激酶靶点发挥作用的机制已得到很好的描述,但索拉非尼在人类肿瘤中引起的反应各不相同,而这种变化的原因尚不清楚。为了研究潜在的机制,我们应用基于质谱的蛋白质组学分析方法对 Huh7.5 人肝癌细胞进行了分析,发现索拉非尼显著影响了关键的生脂酶的表达,特别是硬脂酰辅酶 A 去饱和酶 1(SCD1)。鉴于 SCD1 催化单不饱和脂肪酸(FA)合成中最关键和限速的步骤,我们进行了脂质组学分析,结果显示索拉非尼处理的细胞中的脂质谱发生了显著改变。检测和分析游离 FA 表明,在索拉非尼处理的细胞中,单不饱和 FA(包括油酸)的水平明显降低。添加油酸可保护肝癌细胞免受索拉非尼诱导的死亡,并减轻药物引起的线粒体形态和功能异常。索拉非尼处理会抑制 ATP 产生,导致 AMPK 激活和磷酸化。进一步的次级效应包括降低固醇调节元件结合蛋白 1(SREBP1)的水平和肝癌细胞中雷帕霉素(mTOR)的磷酸化。在存在化合物 C(一种 AMPK 抑制剂)和 ATP 和腺苷的情况下,这些作用部分被消除,SREBP1c 过表达也可以抵抗索拉非尼的作用,表明索拉非尼诱导的细胞活力降低是由 ATP-AMPK-mTOR-SREBP1 信号通路介导的。总之,我们的结果表明,索拉非尼在肝癌细胞中的抗癌活性是基于抑制 ATP 产生、SCD1 表达和单不饱和 FA 合成。此外,单不饱和 FA 合成的减少进一步触发了索拉非尼处理的细胞中 ATP 产生的更严重减少。据我们所知,这是第一个证据表明,索拉非尼通过靶向 SCD1 破坏脂肪生成并通过 ATP-AMPK-mTOR-SREBP1 途径触发肝癌细胞死亡。-刘,G.,匡,S.,曹,R.,王,J.,彭,Q.,孙,C. 索拉非尼通过靶向 SCD1 破坏单不饱和脂肪酸合成并通过 ATP-AMPK-mTOR-SREBP1 信号通路杀死肝癌细胞。
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