STAT2/SLC27A3/PINK1-Mediated Mitophagy Remodeling Lipid Metabolism Contributes to Pazopanib Resistance in Clear Cell Renal Cell Carcinoma.

IF 11 1区 综合性期刊 Q1 Multidisciplinary
Research Pub Date : 2024-11-26 eCollection Date: 2024-01-01 DOI:10.34133/research.0539
Dingheng Lu, Yuxiao Li, Xinyang Niu, Jiazhu Sun, Weitao Zhan, Yuchen Shi, Kai Yu, Suyuelin Huang, Xiaoyan Liu, Liping Xie, Xueyou Ma, Ben Liu
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Solute carrier family 27 member 3 (SLC27A3), highly expressed in lipid-rich tumors like ccRCC, has been associated with poor prognosis. However, the impact of SLC27A3 and the transcription factor complex containing STAT2 on lipid metabolic reprogramming, mitophagy in ccRCC, and their role in TKI resistance remain unexplored. <b>Methods:</b> 786-O to pazopanib resistance was induced by gradient increase of concentration, and the genes related to lipid metabolism were screened by RNA sequencing. Bioinformatics was used to analyze the differential expression of SLC27A3 and its effect on patient prognosis, and to predict the activated pathway in pazopanib-resistant cells. Lipid droplets (LDs) were detected by Red Oil O and BODIPY probe. Micro-targeted lipidomic of acyl-coenzyme A (CoA) and lipid metabolomics were performed to screen potential metabolites of SLC27A3. The differential expression of SLC27A3 was detected in clinical samples. The differential expression of SLC27A3 and its effect on drug resistance of ccRCC tumor were detected in vitro and in vivo<i>.</i> Mitophagy was detected by electron microscopy, Mtphagy probe, and Western blot. The mitochondrial membrane potential (MMP) and reactive oxygen species (ROS) levels were detected by JC-1 and DCF probes. The binding site of the transcription factor complex to the SLC27A3 promoter was detected by dual-luciferase reporter gene assay. <b>Results:</b> SLC27A3, highly expressed in lipid-rich tumors such as ccRCC and glioblastoma, predicts poor prognosis. SLC27A3 expression level also increased in pazopanib-resistant 786-O cells (786-O-PR) with more LD accumulation compared to parental cells. Gene Ontology (GO) and Kyoto Encyclopedia of Genes and Genomes (KEGG) pathway analysis from RNA sequencing showed that PINK1/Parkin-mediated mitophagy pathway was enriched in 786-O-PR. Knockdown of SLC27A3 markedly suppressed LD accumulation and mitophagy, and overcame pazopanib resistance <i>in vitro</i> and <i>in vivo</i>. Moreover, SLC27A3 functions as an acyl-CoA ligase catalyzing the formation of acyl-CoA, which refers to fatty acid oxidation accompanied by ROS production and synthesis of lipid. Overproduced acyl-CoA oxidation in mitochondria resulted in MMP decrease and amounts of ROS production, subsequently triggering PINK1/Parkin-mediated mitophagy. Moreover, mitophagy inhibition led to more ROS accumulation and cell death, indicating that mitophagy can keep ROS at an appropriate level by negative feedback. Mitophagy, simultaneously, prevented fatty acid oxidation in mitochondria by consuming CPT1A, forcing synthesis of triglycerides and cholesterol esters stored in LDs by transforming acyl-CoA, to support ccRCC progression. Besides, we found that STAT2 expression was positively correlated to SLC27A3. 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引用次数: 0

Abstract

Background: Clear cell renal cell carcinoma (ccRCC) is a prevalent malignant tumor of the urinary system. While tyrosine kinase inhibitors (TKIs) are currently the first-line treatments for advanced/metastatic ccRCC, patients often develop resistance after TKI therapy. Lipid metabolic reprogramming, a hallmark of tumor progression, contributes to acquired drug resistance in various malignant tumors. Mitophagy, a process that maintains mitochondrial homeostasis, aids tumor cells in adapting to microenvironmental changes and consequently developing drug resistance. Solute carrier family 27 member 3 (SLC27A3), highly expressed in lipid-rich tumors like ccRCC, has been associated with poor prognosis. However, the impact of SLC27A3 and the transcription factor complex containing STAT2 on lipid metabolic reprogramming, mitophagy in ccRCC, and their role in TKI resistance remain unexplored. Methods: 786-O to pazopanib resistance was induced by gradient increase of concentration, and the genes related to lipid metabolism were screened by RNA sequencing. Bioinformatics was used to analyze the differential expression of SLC27A3 and its effect on patient prognosis, and to predict the activated pathway in pazopanib-resistant cells. Lipid droplets (LDs) were detected by Red Oil O and BODIPY probe. Micro-targeted lipidomic of acyl-coenzyme A (CoA) and lipid metabolomics were performed to screen potential metabolites of SLC27A3. The differential expression of SLC27A3 was detected in clinical samples. The differential expression of SLC27A3 and its effect on drug resistance of ccRCC tumor were detected in vitro and in vivo. Mitophagy was detected by electron microscopy, Mtphagy probe, and Western blot. The mitochondrial membrane potential (MMP) and reactive oxygen species (ROS) levels were detected by JC-1 and DCF probes. The binding site of the transcription factor complex to the SLC27A3 promoter was detected by dual-luciferase reporter gene assay. Results: SLC27A3, highly expressed in lipid-rich tumors such as ccRCC and glioblastoma, predicts poor prognosis. SLC27A3 expression level also increased in pazopanib-resistant 786-O cells (786-O-PR) with more LD accumulation compared to parental cells. Gene Ontology (GO) and Kyoto Encyclopedia of Genes and Genomes (KEGG) pathway analysis from RNA sequencing showed that PINK1/Parkin-mediated mitophagy pathway was enriched in 786-O-PR. Knockdown of SLC27A3 markedly suppressed LD accumulation and mitophagy, and overcame pazopanib resistance in vitro and in vivo. Moreover, SLC27A3 functions as an acyl-CoA ligase catalyzing the formation of acyl-CoA, which refers to fatty acid oxidation accompanied by ROS production and synthesis of lipid. Overproduced acyl-CoA oxidation in mitochondria resulted in MMP decrease and amounts of ROS production, subsequently triggering PINK1/Parkin-mediated mitophagy. Moreover, mitophagy inhibition led to more ROS accumulation and cell death, indicating that mitophagy can keep ROS at an appropriate level by negative feedback. Mitophagy, simultaneously, prevented fatty acid oxidation in mitochondria by consuming CPT1A, forcing synthesis of triglycerides and cholesterol esters stored in LDs by transforming acyl-CoA, to support ccRCC progression. Besides, we found that STAT2 expression was positively correlated to SLC27A3. Transcriptional factor complex containing STAT2 could bind to the promoter of SLC27A3 mRNA to promote SLC27A3 transcription proved by dual-luciferase reporter assay, which also regulated LD metabolism and activated mitophagy during pazopanib resistance. Conclusion: SLC27A3 is up-regulated in pazopanib-resistant ccRCC and predicts poor prognosis. High expression of SLC27A3 produces excessive metabolites of various long-chain fatty acyl-CoA (12:0-, 16:0-, 17:0-, 20:3-CoA) to enter mitochondria for β-oxidation and produce amounts of ROS activating mitophagy. Subsequent mitophagy/ROS negative feedback controls ROS homeostasis and consumes CPT1A protein within mitochondria to suppress fatty acid β-oxidation, forcing acyl-CoA storage in LDs, mediating pazopanib resistance in ccRCC. Furthermore, STAT2 was identified as a core component of a potential upstream transcriptional factor complex for SLC27A3. Our findings shed new light on the underlying mechanism of SLC27A3 in ccRCC TKI resistance, which may provide a novel therapeutic target for the management of ccRCC.

STAT2/SLC27A3/PINK1介导的丝裂吞噬重塑脂质代谢是透明细胞肾细胞癌帕唑帕尼耐药的原因。
背景:透明细胞肾细胞癌(ccRCC)是一种常见的泌尿系统恶性肿瘤。虽然酪氨酸激酶抑制剂(TKIs)是目前治疗晚期/转移性ccRCC的一线药物,但患者在接受TKI治疗后往往会产生耐药性。脂质代谢重编程是肿瘤进展的一个标志,也是各种恶性肿瘤产生获得性耐药性的原因之一。线粒体吞噬是维持线粒体平衡的过程,有助于肿瘤细胞适应微环境变化,从而产生耐药性。溶质运载家族 27 成员 3(SLC27A3)在富含脂质的肿瘤(如 ccRCC)中高表达,与预后不良有关。然而,SLC27A3和含有STAT2的转录因子复合物对脂质代谢重编程、ccRCC中的有丝分裂以及它们在TKI耐药性中的作用的影响仍有待探索。方法:通过梯度增加浓度诱导 786-O 对帕唑帕尼耐药,并通过 RNA 测序筛选与脂质代谢相关的基因。利用生物信息学分析SLC27A3的差异表达及其对患者预后的影响,并预测帕唑帕尼耐药细胞中的激活途径。红油O和BODIPY探针检测脂滴(LDs)。通过酰辅酶A(CoA)微靶脂质组学和脂质代谢组学筛选SLC27A3的潜在代谢物。在临床样本中检测到了 SLC27A3 的差异表达。在体外和体内检测了SLC27A3的差异表达及其对ccRCC肿瘤耐药性的影响。通过电子显微镜、Mtphagy探针和Western印迹检测了线粒体吞噬。用 JC-1 和 DCF 探针检测线粒体膜电位(MMP)和活性氧(ROS)水平。通过双荧光素酶报告基因检测转录因子复合物与 SLC27A3 启动子的结合位点。结果SLC27A3在富含脂质的肿瘤(如ccRCC和胶质母细胞瘤)中高表达,可预测不良预后。与亲代细胞相比,帕唑帕尼耐药的786-O细胞(786-O-PR)中SLC27A3的表达水平也有所升高,并有更多的LD积累。基因本体(GO)和京都基因组百科全书(KEGG)通路分析显示,786-O-PR中富含PINK1/Parkin介导的有丝分裂通路。敲除SLC27A3能显著抑制LD积累和有丝分裂,并克服帕唑帕尼在体外和体内的耐药性。此外,SLC27A3还具有酰基-CoA连接酶的功能,可催化酰基-CoA的形成。线粒体中过度产生的酰基-CoA 氧化会导致 MMP 减少和 ROS 产生,进而引发 PINK1/Parkin 介导的有丝分裂。此外,抑制有丝分裂会导致更多的 ROS 积累和细胞死亡,这表明有丝分裂可以通过负反馈将 ROS 保持在适当的水平。同时,有丝分裂可通过消耗CPT1A阻止线粒体中的脂肪酸氧化,迫使甘油三酯和胆固醇酯通过转化酰基-CoA合成储存在LD中的脂肪酸,从而支持ccRCC的进展。此外,我们还发现 STAT2 的表达与 SLC27A3 呈正相关。双荧光素酶报告实验证明,含有STAT2的转录因子复合物可与SLC27A3 mRNA的启动子结合,促进SLC27A3的转录,这也调节了帕唑帕尼耐药期间的LD代谢并激活了有丝分裂。结论SLC27A3在帕唑帕尼耐药的ccRCC中上调,可预测不良预后。SLC27A3的高表达会产生过多的各种长链脂肪酰基-CoA(12:0-、16:0-、17:0-、20:3-CoA)代谢产物进入线粒体进行β氧化,并产生大量的ROS激活有丝分裂。随后的有丝分裂/ROS 负反馈控制着 ROS 的平衡,并消耗线粒体中的 CPT1A 蛋白以抑制脂肪酸的 β 氧化,从而迫使酰基-CoA 储存在 LD 中,介导了帕唑帕尼对 ccRCC 的耐药性。此外,还发现 STAT2 是 SLC27A3 潜在上游转录因子复合物的核心成分。我们的研究结果揭示了SLC27A3在ccRCC TKI耐药中的潜在机制,这可能为治疗ccRCC提供一个新的治疗靶点。
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
Research
Research Multidisciplinary-Multidisciplinary
CiteScore
13.40
自引率
3.60%
发文量
0
审稿时长
14 weeks
期刊介绍: Research serves as a global platform for academic exchange, collaboration, and technological advancements. This journal welcomes high-quality research contributions from any domain, with open arms to authors from around the globe. Comprising fundamental research in the life and physical sciences, Research also highlights significant findings and issues in engineering and applied science. The journal proudly features original research articles, reviews, perspectives, and editorials, fostering a diverse and dynamic scholarly environment.
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