细胞色素 P450 2E1 依赖性肝内乙醇代谢诱导脂肪酸结合蛋白 4 并导致脂肪变性。
Cytochrome P450 2E1-dependent hepatic ethanol metabolism induces fatty acid-binding protein 4 and steatosis.
机构信息
Department of Surgery, Carolinas Medical Center, Atrium Health, Charlotte, North Carolina, USA.
出版信息
Alcohol Clin Exp Res. 2022 Jun;46(6):928-940. doi: 10.1111/acer.14828. Epub 2022 Apr 17.
BACKGROUND
Hepatic steatosis is an early pathology of alcohol-associated liver disease (ALD). Fatty acid-binding protein-4 (FABP4, a FABP not normally produced in the liver) is secreted by hepatocytes in ALD and stimulates hepatoma proliferation and migration. This study sought to investigate the mechanism[s] by which hepatic ethanol metabolism regulates FABP4 and steatosis.
METHODS
Human hepatoma cells (HepG2/HuH7) and cells stably transfected to express cytochrome P450 2E1 (CYP2E1), were exposed to ethanol in the absence or presence of chlormethiazole (a CYP2E1-inhibitor; CMZ) and/or EX-527 (a sirtuin-1 [SIRT1] inhibitor). The culture medium was analyzed for ethanol metabolism and FABP4 protein abundance. Cells were analyzed for FABP4 mRNA expression, SIRT1 protein abundance, and neutral lipid accumulation. In parallel, cells were analyzed for forkhead box O1 [FOXO1], β-catenin, peroxisome proliferator-activated receptor-α [PPARα], and lipin-1α protein abundance in the absence or presence of ethanol and pharmacological inhibitors of the respective target proteins.
RESULTS
CYP2E1-dependent ethanol metabolism inhibited the amount of SIRT1 protein detected, concomitant with increased FABP4 mRNA expression, FABP4 protein secretion, and neutral lipid accumulation, effects abolished by CMZ. Analysis of pathways associated with lipid oxidation revealed increased FOXO1 nuclear localization and decreased β-catenin, PPARα, and lipin-1α protein levels in CYP2E1-expressing cells in the presence of ethanol. Pharmacological inhibition of SIRT1 mimicked the effects of ethanol, while inhibition of FOXO1 abrogated the effect of ethanol on FABP4 mRNA expression, FABP4 protein secretion, and neutral lipid accumulation in CYP2E1-expressing cells. Pharmacological inhibition of β-catenin, PPARα, or lipin-1α failed to alter the effects of ethanol on FABP4 or neutral lipid accumulation.
CONCLUSION
CYP2E1-dependent ethanol metabolism inhibits SIRT1-FOXO1 signaling, which leads to increased FABP4 mRNA expression, FABP4 protein secretion, and neutral lipid accumulation. These data suggest that FABP4 released from steatotic hepatocytes could play a role in promoting tumor cell expansion in the setting of ALD and represents a potential target for therapeutic intervention.
背景
肝脂肪变性是酒精相关肝病(ALD)的早期病理学改变。脂肪酸结合蛋白 4(FABP4,一种通常不在肝脏中产生的 FABP)在 ALD 中由肝细胞分泌,并刺激肝癌增殖和迁移。本研究旨在探讨肝乙醇代谢调节 FABP4 和脂肪变性的机制。
方法
将人肝癌细胞(HepG2/HuH7)和稳定转染表达细胞色素 P450 2E1(CYP2E1)的细胞暴露于乙醇中,同时存在或不存在氯美噻唑(CYP2E1 抑制剂;CMZ)和/或 EX-527(SIRT1 抑制剂)。分析培养基中的乙醇代谢和 FABP4 蛋白丰度。分析细胞的 FABP4 mRNA 表达、SIRT1 蛋白丰度和中性脂质积累。同时,在存在或不存在乙醇和相应靶蛋白的药理学抑制剂的情况下,分析细胞中叉头框 O1[FOXO1]、β-连环蛋白、过氧化物酶体增殖物激活受体-α[PPARα]和脂联素 1α 的蛋白丰度。
结果
CYP2E1 依赖性乙醇代谢抑制了检测到的 SIRT1 蛋白的量,同时伴随着 FABP4 mRNA 表达、FABP4 蛋白分泌和中性脂质积累的增加,这些作用被 CMZ 所消除。与脂质氧化相关的途径分析显示,在存在乙醇的情况下,CYP2E1 表达细胞中 FOXO1 的核定位增加,β-连环蛋白、PPARα 和脂联素 1α 的蛋白水平降低。SIRT1 的药理学抑制模拟了乙醇的作用,而 FOXO1 的抑制消除了乙醇对 CYP2E1 表达细胞中 FABP4 mRNA 表达、FABP4 蛋白分泌和中性脂质积累的影响。β-连环蛋白、PPARα 或脂联素 1α 的药理学抑制均未能改变乙醇对 FABP4 或中性脂质积累的影响。
结论
CYP2E1 依赖性乙醇代谢抑制 SIRT1-FOXO1 信号通路,导致 FABP4 mRNA 表达、FABP4 蛋白分泌和中性脂质积累增加。这些数据表明,从脂肪变性肝细胞释放的 FABP4 可能在 ALD 中发挥促进肿瘤细胞扩张的作用,是治疗干预的潜在靶点。
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