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口腔癌发生过程中乙醇和4-硝基喹啉-1-氧化物诱导的表观遗传和氧化应激标志物的鉴定

Identification of Ethanol and 4-Nitroquinoline-1-Oxide Induced Epigenetic and Oxidative Stress Markers During Oral Cavity Carcinogenesis.

作者信息

Urvalek Alison M, Osei-Sarfo Kwame, Tang Xiao-Han, Zhang Tuo, Scognamiglio Theresa, Gudas Lorraine J

机构信息

Department of Pharmacology, Weill Cornell Medical College, New York, New York.

Genomics Resources Core Facility, Weill Cornell Medical College, New York, New York.

出版信息

Alcohol Clin Exp Res. 2015 Aug;39(8):1360-72. doi: 10.1111/acer.12772.

Abstract

BACKGROUND

Head and neck squamous cell carcinoma (HNSCC) is a cancer that is characterized by its high morbidity and mortality rates. While tobacco use and alcohol consumption are 2 major contributing factors for HNSCC carcinogenesis, how the combination of tobacco and alcohol increases HNSCC risk is not understood.

METHODS

We combined the 4-nitroquinoline-1-oxide (4-NQO) oral carcinogenesis and Meadows-Cook alcohol mouse models to elucidate the molecular events and to identify the novel biomarkers associated with oral cancer development.

RESULTS

By genome-wide RNA-seq of tongue samples (3 mice per group), we identified changes in transcripts that mediate alcohol metabolism and oxidative stress (Aldh2, Aldh1a3, Adh1, Adh7, and Cyp2a5) in mice treated with 4-NQO followed by ethanol (4-NQO/EtOH) as compared to the vehicle control/untreated (V.C./Untr.) samples. We measured major, global increases in specific histone acetylation and methylation epigenetic marks (H3K27ac, H3K9/14ac, H3K27me3, and H3K9me3) in the oral cavities of V.C./EtOH, 4-NQO/Untr., and 4-NQO/EtOH treatment groups compared to the V.C./Untr. group. We detected changes in histone epigenetic marks near regulatory regions of genes involved in ethanol metabolism by chromatin immunoprecipitation. For instance, the Aldh2 promoter showed increased H3K27me3 marks, and Aldh2 mRNA levels were reduced by 10-fold in 4NQO/EtOH versus V.C./Untr. tongue samples. 4-NQO/EtOH treatment also caused increases in markers of oxidative stress, including 4-HNE, MCT4/SLC16a3, and TOM20, as measured by immunohistochemistry.

CONCLUSIONS

We delineate a mechanism by which 4-NQO and ethanol can regulate gene expression during the development of HNSCC and suggest that histone epigenetic marks and oxidative stress markers could be the novel biomarkers and targets for the prevention of HNSCC.

摘要

背景

头颈部鳞状细胞癌(HNSCC)是一种发病率和死亡率都很高的癌症。虽然吸烟和饮酒是HNSCC致癌的两个主要促成因素,但烟草和酒精的联合使用如何增加HNSCC风险尚不清楚。

方法

我们将4-硝基喹啉-1-氧化物(4-NQO)口腔致癌模型和梅多斯-库克酒精小鼠模型相结合,以阐明分子事件,并识别与口腔癌发生相关的新型生物标志物。

结果

通过对舌样本(每组3只小鼠)进行全基因组RNA测序,我们发现与载体对照/未处理(V.C./未处理)样本相比,在用4-NQO处理后再用乙醇处理(4-NQO/乙醇)的小鼠中,介导酒精代谢和氧化应激的转录本(Aldh2、Aldh1a3、Adh1、Adh7和Cyp2a5)发生了变化。与V.C./未处理组相比,我们在V.C./乙醇、4-NQO/未处理和4-NQO/乙醇处理组的口腔中检测到特定组蛋白乙酰化和甲基化表观遗传标记(H3K27ac、H3K9/14ac、H3K27me3和H3K9me3)总体上有显著增加。通过染色质免疫沉淀,我们检测到参与乙醇代谢的基因调控区域附近的组蛋白表观遗传标记发生了变化。例如,Aldh2启动子显示H3K27me3标记增加,与V.C./未处理的舌样本相比,4NQO/乙醇处理组中Aldh2 mRNA水平降低了10倍。通过免疫组织化学检测,4-NQO/乙醇处理还导致氧化应激标志物增加,包括4-HNE、MCT4/SLC16a3和TOM20。

结论

我们阐述了一种4-NQO和乙醇在HNSCC发生过程中调节基因表达的机制,并表明组蛋白表观遗传标记和氧化应激标志物可能是预防HNSCC的新型生物标志物和靶点。

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