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在含有从苯巴比妥和β-萘黄酮处理的大鼠中纯化的细胞色素P-450的重组系统中N-亚硝基二烷基胺的脱烷基作用

N-nitrosodialkylamine dealkylation in reconstituted systems containing cytochrome P-450 purified from phenobarbital- and beta-naphthoflavone-treated rats.

作者信息

Kawanishi T, Ohno Y, Takanaka A, Kawano S, Yamazoe Y, Kato R, Omori Y

机构信息

Division of Pharmacology, National Institute of Hygienic Sciences, Tokyo, Japan.

出版信息

Arch Toxicol. 1992;66(2):137-42. doi: 10.1007/BF02342508.

DOI:10.1007/BF02342508
PMID:1605729
Abstract

Five cytochrome P-450 forms were purified from livers of rats pretreated with phenobarbital (PB) or beta-naphthoflavone (BNF), and the oxidative dealkylation of N-nitrosodialkylamines by the reconstituted cytochrome P-450 systems was measured. PB-II (P450IIB1) showed very high N-nitrosomethybutylamine (NMBA) debutylase activity, high NMBA demethylase activity and high N-nitrosomethyl-benzylamine (NMBeA) debenzylase activity, suggesting that the increase following PB treatment in hepatic microsomal NMBA debutylation and NMBeA debenzylation was due to the induction of PB-II. BNF-H (P450IA2) showed very high NMBA debutylase and high NMBeA debenzylase activities, and BNF-L (P450IA1) showed NMBA debutylase and high NMBeA debenzylase activities. These results suggested that the increase by BNF pretreatment in hepatic microsomal NMBA debutylation was due mainly to the induction of BNF-H and in some part to that of BNF-L. PB-II also showed very high dealkylation activity of lipophilic N-nitrosodialkylamines with long alkyl moieties. On the other hand, BNF-H dealkylated N-nitrosodipropylamine (NDPA), N-nitrosomethylbutylamine (NMBA) and N-nitrosoethylbutylamine (NEBA) at higher rates than N-nitrosodibutylamine (NDBA). BNF-L dealkylated NEBA at higher rates than NMBeA and NDBA. These results reveal that substrate specificity of each cytochrome P-450 form in N-nitrosodialkylamine metabolism is different from each other and several forms of cytochrome P-450 support each N-nitrosamine dealkylase activity in mammalians.

摘要

从经苯巴比妥(PB)或β-萘黄酮(BNF)预处理的大鼠肝脏中纯化出5种细胞色素P-450同工酶,并测定了重组细胞色素P-450系统对N-亚硝基二烷基胺的氧化脱烷基作用。PB-II(P450IIB1)表现出非常高的N-亚硝基甲基丁胺(NMBA)脱丁基酶活性、高NMBA脱甲基酶活性和高N-亚硝基甲基苄胺(NMBeA)脱苄基酶活性,这表明PB处理后肝脏微粒体中NMBA脱丁基作用和NMBeA脱苄基作用的增加是由于PB-II的诱导。BNF-H(P450IA2)表现出非常高的NMBA脱丁基酶活性和高NMBeA脱苄基酶活性,而BNF-L(P450IA1)表现出NMBA脱丁基酶活性和高NMBeA脱苄基酶活性。这些结果表明,BNF预处理后肝脏微粒体中NMBA脱丁基作用的增加主要是由于BNF-H的诱导,部分是由于BNF-L的诱导。PB-II对具有长烷基部分的亲脂性N-亚硝基二烷基胺也表现出非常高的脱烷基活性。另一方面,BNF-H对N-亚硝基二丙胺(NDPA)、N-亚硝基甲基丁胺(NMBA)和N-亚硝基乙基丁胺(NEBA)的脱烷基速率高于N-亚硝基二丁胺(NDBA)。BNF-L对NEBA的脱烷基速率高于NMBeA和NDBA。这些结果表明,在N-亚硝基二烷基胺代谢中,每种细胞色素P-450同工酶的底物特异性彼此不同,并且几种形式的细胞色素P-450支持哺乳动物中每种N-亚硝胺脱烷基酶的活性。

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