多氯联苯在环境性肝病小鼠模型中改变肝 m6A mRNA 甲基化。
Polychlorinated biphenyls alter hepatic m6A mRNA methylation in a mouse model of environmental liver disease.
机构信息
Department of Biochemistry & Molecular Genetics, University of Louisville School of Medicine, Louisville, KY, 40292, USA.
University of Louisville Center for Integrative Environmental Health Sciences (CIEHS), USA; University of Louisville Hepatobiology and Toxicology Center, USA; The University of Louisville Superfund Research Center, USA; Division of Gastroenterology, Hepatology & Nutrition, Department of Medicine, University of Louisville School of Medicine, USA.
出版信息
Environ Res. 2023 Jan 1;216(Pt 3):114686. doi: 10.1016/j.envres.2022.114686. Epub 2022 Oct 28.
Exposure to polychlorinated biphenyls (PCBs) has been associated with liver injury in human cohorts and with nonalcoholic steatohepatitis (NASH) in mice fed a high fat diet (HFD). N (6)-methyladenosine (m6A) modification of mRNA regulates transcript fate, but the contribution of m6A modification on the regulation of transcripts in PCB-induced steatosis and fibrosis is unknown. This study tested the hypothesis that PCB and HFD exposure alters the levels of m6A modification in transcripts that play a role in NASH in vivo. Male C57Bl6/J mice were fed a HFD (12 wks) and administered a single oral dose of Aroclor1260, PCB126, or Aroclor1260 + PCB126. Genome-wide identification of m6A peaks was accomplished by m6A mRNA immunoprecipitation sequencing (m6A-RIP) and the mRNA transcriptome identified by RNA-seq. Exposure of HFD-fed mice to Aroclor1260 decreased the number of m6A peaks and m6A-containing genes relative to PCB vehicle control whereas PCB126 or the combination of Aroclor1260 + PCB126 increased m6A modification frequency. ∼41% of genes had one m6A peak and ∼49% had 2-4 m6A peaks. 117 m6A peaks were common in the four experimental groups. The Aroclor1260 + PCB126 exposure group showed the highest number (52) of m6A-peaks. qRT-PCR confirmed enrichment of m6A-containing fragments of the Apob transcript with PCB exposure. A1cf transcript abundance, m6A peak count, and protein abundance was increased with Aroclor1260 + PCB126 co-exposure. Irrespective of the PCB type, all PCB groups exhibited enriched pathways related to lipid/lipoprotein metabolism and inflammation through the m6A modification. Integrated analysis of m6A-RIP-seq and mRNA-seq identified 242 differentially expressed genes (DEGs) with increased or reduced number of m6A peaks. These data show that PCB exposure in HFD-fed mice alters the m6A landscape offering an additional layer of regulation of gene expression affecting a subset of gene responses in NASH.
多氯联苯 (PCBs) 的暴露已被证明与人类队列中的肝损伤以及高脂饮食 (HFD) 喂养的小鼠中非酒精性脂肪性肝炎 (NASH) 有关。mRNA 的 N (6)-甲基腺苷 (m6A) 修饰调节转录本的命运,但 m6A 修饰对 PCB 诱导的脂肪变性和纤维化中调节转录本的作用尚不清楚。本研究检验了这样一个假设,即 PCB 和 HFD 暴露改变了体内 NASH 中起作用的转录本的 m6A 修饰水平。雄性 C57Bl6/J 小鼠喂食 HFD(12 周)并给予单次口服 Aroclor1260、PCB126 或 Aroclor1260+PCB126。通过 m6A mRNA 免疫沉淀测序 (m6A-RIP) 进行全基因组 m6A 峰鉴定,并通过 RNA-seq 鉴定 mRNA 转录组。与 PCB 载体对照相比,HFD 喂养的小鼠暴露于 Aroclor1260 会降低 m6A 峰和 m6A 含量基因的数量,而 PCB126 或 Aroclor1260+PCB126 的组合则增加 m6A 修饰频率。约 41%的基因有一个 m6A 峰,约 49%的基因有 2-4 个 m6A 峰。在四个实验组中共有 117 个 m6A 峰。Aroclor1260+PCB126 暴露组显示出最高数量(52)的 m6A 峰。qRT-PCR 证实了 PCB 暴露时 Apob 转录物中 m6A 含量片段的富集。随着 Aroclor1260+PCB126 共同暴露,A1cf 转录物丰度、m6A 峰计数和蛋白丰度增加。无论 PCB 类型如何,所有 PCB 组都表现出富含与脂质/脂蛋白代谢和炎症相关的途径,这是通过 m6A 修饰实现的。m6A-RIP-seq 和 mRNA-seq 的综合分析确定了 242 个差异表达基因(DEGs),它们的 m6A 峰数量增加或减少。这些数据表明,HFD 喂养的小鼠中 PCB 的暴露改变了 m6A 图谱,为影响 NASH 中基因反应子集的基因表达提供了额外的调节层。
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