Defining PAH-mediated carcinogenesis in lung: CYP metabolism and B[a]P transport

定义 PAH 介导的肺癌致癌作用：CYP 代谢和 B[a]P 转运

• 批准号: 7406263
• 负责人: Stacy Lynn Gelhaus
• 金额: $ 4.68万
• 依托单位: UNIVERSITY OF PENNSYLVANIA
• 依托单位国家: 美国
• 财政年份: 2007
• 资助国家: 美国
• 起止时间: 2007-09-30 至 2010-09-29
• 项目状态: 已结题
• 来源: https://reporter.nih.gov/project-details/7406263
• 关键词: 2' -deoxyadenosine; ABCB1 gene; ABCC1 gene; Address; Adipose tissue; Amines; Amino Acids; Animals; Area; Aromatic Polycyclic Hydrocarbons; Benz(a)Anthracenes; Benzo(a)pyrene; Binding; Biological; Biological Assay; CYP1A1 gene; CYP3A4 gene; CYP3A5 gene; Cancer Etiology; Carcinogens; Cations; Cattle; Cause of Death; Cell Line; Cell Nucleus; Cells; Characteristics; Coal; CpG Islands; Cultured Cells; Cytochrome P450; Cytochromes; DNA; DNA Adduction; DNA Adducts; DNA Damage; Data; Deoxyguanosine; Development; Dimethyl Sulfoxide; Dioxins; Drug Delivery Systems; Drug Metabolic Detoxication; Environmental Carcinogens; Environmental Pollutants; Enzymes; Epoxide hydrolase; Experimental Models; Exposure to; Family member; Fire - disasters; Food; Garbage; Gases; Genomics; Glutathione; Glutathione S-Transferase; Glycol; Glycoproteins; Guanine; Hepatocyte; Human; Human Milk; Hydrolysis; In Vitro; Individual; Individual Differences; International Agency for Research on Cancer; Itraconazole; Kidney; Link; Liquid Chromatography; Literature; Liver; Lung; Malignant Neoplasms; Malignant neoplasm of lung; Malignant neoplasm of urinary bladder; Mass Spectrum Analysis; Meat; Mediating; Messenger RNA; Metabolic; Metabolic Activation; Metabolic Pathway; Metabolism; Methodology; Methods; Modeling; Monitor; Multidrug Resistance Associated Protein 1; Mus; Mutation; Names; Nature; Null Lymphocytes; Oils; Oxides; P-Glycoprotein; Pathway interactions; Pharmaceutical Preparations; Phase; Play; Point Mutation; Promoter Regions; Protein Isoforms; Protein p53; Proteomics; Public Health; Pyrenes; RNA Interference; Reaction; Reporting; Research; Reverse Transcriptase Polymerase Chain Reaction; Role; Skin; Small Interfering RNA; Smoke; Smoker; Stable Isotope Labeling; TP53 gene; Testing; Tobacco; Tobacco smoke; Toxic effect; Transfection; Transferase; United States; United States Dept. of Health and Human Services; Western Blotting; Wood material; Workplace; adduct; anticancer research; base; benzanthracene; carbonyl reductase (NADPH); carcinogenesis; cigarette smoking; cigarette smoking; cytochrome P450 3A; extracellular; fluoranthene; hepatoma cell; inhibitor/antagonist; insight; lung carcinogenesis; multidrug resistance-associated protein 2; novel; novel therapeutics; prevent; protein expression; pyrene; research study; stable isotope; tobacco exposure; transcription factor

DESCRIPTION (provided by applicant): In this proposed research, benzo[a]pyrene (B[a]P) and it's metabolites, will be used as model compounds to determine the major metabolic pathways of PAHs in lung carcinogenesis. It is generally accepted that cytochrome P4501A1, CYP1A1, is primarily responsible for the metabolism of B[a]P to 7,8-dihydroxy-9,10- epoxy-7,8,9,10-tetrahydrobenzo[a]pyrene (B[a]PDE), the ultimate DNA-adduct forming, carcinogenic reactive metabolite; thus connecting CYP1A1 to the toxicological effects of this environmental carcinogen. DNA-adduct formation has been detected at CpG islands located in the promoter region of the tumor suppressor p53. Inactivation of p53 by point mutations is seen in over 40% of all cancers. However, in preliminary research using H358, human bronchoalveolar lung cells, it was found that DNA-adduct levels were higher in non-treated CYP1A1/1B1 null cells compared to H358 cells in which CYP1A1 expression was induced with 2, 3, 7, 8-tetrachlorodibenzo-p-dioxin (TCDD). This data correlates with literature results of CYP1A1 KO mice stuides in which it was determined that CYP1A1 conferred a protective rather than a toxic effect. This is indicative of the metabolic activity of another CYP in the metabolism of B[a]P. Several other CYP enzymes are capable of catalyzing this metabolism. Preliminary data has also indicated that TCDD may have an effect on the transport of B[a]P-reactive metabolites. It is known that TCDD is able to induce several of the ABCC drug transporter family members; therefore, explaining why less DNA-adduct formation is observed in lung cells pretreated with TCDD . This proposal, which has two aims, will identify the predominate CYP responsible for B[a]P metabolism in the lung and determine the role of B[a]PDE transporters in DNA-adduct formation in lung cells. A stable isotope dilution LC-MRM/MS method, previously developed, will be used for DNA-adduct quantification. DNA-adduct levels will be correlated to mRNA and protein expression determined by RT-PCR and a novel quantitative proteomics method, SI LAC. CYPs including 1A1, 1B1, 1A2, 2B6, 2E1, 2J2, 3A4, and 3A5 will be investigated. DNA-adduct formation will also be monitored in lung cells in which drug transporter expression has been inhibited by siRNA. Continuing research in this area will provide exciting new therapeutic strategies (drug targets) that can be employed to prevent PAH-mediated DNA damage. Relevance to public health: Cigarette smoke is known to cause 90% of lung cancer, but only 10% of smokers develop lung cancer. Examination of alternative CYP metabolism and B[a]PDE transport in lung cells will provide an experimental model to explore whether inter-individual differences in CYP metabolism and transport contribute to these phenomenon.

描述（由申请人提供）：本拟研究以苯并[a]芘（B[a]P）及其代谢物为模型化合物，确定多环芳烃在肺癌发生中的主要代谢途径。一般认为，细胞色素P4501A1 （CYP1A1）主要负责B[a]P代谢为7,8-二羟基-9,10-环氧-7,8,9,10-四氢苯并[a]芘（B[a]PDE），最终形成dna加合物，致癌反应代谢物；从而将CYP1A1与这种环境致癌物的毒理学效应联系起来。dna加合物的形成在位于肿瘤抑制因子p53启动子区域的CpG岛上被检测到。在超过40%的癌症中，p53因点突变而失活。然而，在对H358人支气管肺泡肺细胞的初步研究中发现，与2,3,7,8 -四氯二苯并-对二恶英（TCDD）诱导CYP1A1表达的H358细胞相比，未处理的CYP1A1/ 1b1空细胞的dna加合物水平更高。这一数据与CYP1A1 KO小鼠研究的文献结果相关联，其中确定CYP1A1具有保护作用而不是毒性作用。这表明另一种CYP在B[a]P的代谢中具有代谢活性。其他几种CYP酶也能催化这种代谢。初步数据还表明，TCDD可能对B[a] p反应性代谢物的转运有影响。众所周知，TCDD能够诱导几种ABCC药物转运体家族成员；因此，解释了为什么在经TCDD预处理的肺细胞中观察到较少的dna加合物形成。该提案有两个目的，将确定肺中负责B[a]P代谢的主要CYP，并确定B[a]PDE转运体在肺细胞dna加合物形成中的作用。先前开发的稳定同位素稀释LC-MRM/MS方法将用于dna加合物的定量。dna加合物水平将通过RT-PCR和一种新的定量蛋白质组学方法SI LAC测定mRNA和蛋白质的表达。CYPs包括1A1、1B1、1A2、2B6、2E1、2J2、3A4和3A5。在药物转运体表达被siRNA抑制的肺细胞中，dna加合物的形成也将被监测。该领域的持续研究将提供令人兴奋的新治疗策略（药物靶点），可用于预防多环芳烃介导的DNA损伤。与公共卫生的相关性：众所周知，90%的肺癌是由吸烟引起的，但只有10%的吸烟者患肺癌。对肺细胞中CYP代谢和B[a]PDE转运的检测将提供一个实验模型，以探索CYP代谢和转运的个体间差异是否导致了这些现象。