人细胞色素P450(CYP)参与AQ4N(一种缺氧激活的蒽醌二N - 氧化物前药)的还原代谢。
Involvement of human cytochromes P450 (CYP) in the reductive metabolism of AQ4N, a hypoxia activated anthraquinone di-N-oxide prodrug.
作者信息
Raleigh S M, Wanogho E, Burke M D, McKeown S R, Patterson L H
机构信息
Department of Pharmaceutical Sciences, De Montfort University, Leicester, United Kingdom.
出版信息
Int J Radiat Oncol Biol Phys. 1998 Nov 1;42(4):763-7. doi: 10.1016/s0360-3016(98)00308-3.
PURPOSE
To establish the role of the human cytochromes P450 (CYPs) in the reductive metabolism of the novel anthraquinone di-N-oxide prodrug AQ4N.
METHODS AND MATERIALS
Metabolism of AQ4N was conducted in a panel of 17 human phenotyped liver microsomes. AQ4N and metabolites were detected by reverse phase isocratic HPLC. CYP inhibitors and Spearman rank correlation were used to determine the significance of AQ4N metabolism versus specific CYP activity and/or expression.
RESULTS
Anaerobic metabolism of AQ4N to the 2-electron reduction product, AQM, and the 4-electron reduced tertiary amine, AQ4, occurred in all 17 human liver microsome preparations. The range (+/- SE) for total AQ4N turnover was 14.26 +/- 1.43 nmol/incubate (highest) to 3.65 +/- 1.05 nmol/incubate (lowest). Metabolism was not detected in the absence of NADPH or microsomes. In aerobic incubates, AQM was less than 4% of anaerobic values whereas AQ4 was undetectable. CYP-mediated metabolism of AQ4N was inhibited completely by ketoconazole (KET) and carbon monoxide (CO), two global inhibitors of CYP-mediated metabolism. AQ4N metabolism correlated significantly with probes for CYP 3A, specifically benzoxylresorufin O-dealkylation [r(s) = 0.70,p <0.01] and tamoxifen N-demethylation (r(s) = 0.85, p < 0.01), but not with probes for CYPs 2C, 2D, and 1A. CYP 3A involvement was confirmed by the use of the CYP 3A specific inhibitor, triacetyloleandomycin (TAO), which repressed the formation of AQM to 13% of the uninhibited value and abolished completely the formation of AQ4. Alpha-naphthoflavone (ANF), an inhibitor of CYP 2C and 1A, had no significant effect on AQ4N metabolism.
CONCLUSIONS
These data suggest that the human CYP 3A enzymes can contribute to the reductive metabolism of AQ4N. CYP 3A enzymes are highly expressed in a broad spectrum of human cancers. The results show that AQ4N requires anaerobic conditions for CYP 3A-mediated reduction and hence this subfamily of enzymes is likely to selectively activate AQ4N in hypoxic tumors.
目的
确定人细胞色素P450(CYPs)在新型蒽醌二氮氧化物前药AQ4N的还原代谢中的作用。
方法和材料
在17种经表型鉴定的人肝微粒体中进行AQ4N的代谢研究。通过反相等度高效液相色谱法检测AQ4N及其代谢产物。使用CYP抑制剂和Spearman等级相关性分析来确定AQ4N代谢与特定CYP活性和/或表达之间的关系。
结果
在所有17种人肝微粒体制剂中均发生了AQ4N的厌氧代谢,生成2电子还原产物AQM和4电子还原的叔胺AQ4。AQ4N总周转率的范围(±标准误)为14.26±1.43 nmol/孵育(最高)至3.65±1.05 nmol/孵育(最低)。在没有NADPH或微粒体的情况下未检测到代谢。在需氧孵育中,AQM低于厌氧值的4%,而AQ4未检测到。酮康唑(KET)和一氧化碳(CO)这两种CYP介导代谢的全局抑制剂可完全抑制AQ4N的CYP介导代谢。AQ4N代谢与CYP 3A的探针显著相关,特别是苯氧基试卤灵O-脱烷基化[r(s)=0.70,p<0.01]和他莫昔芬N-去甲基化(r(s)=0.85,p<0.01),但与CYP 2C、2D和1A的探针无关。使用CYP 3A特异性抑制剂三乙酰竹桃霉素(TAO)证实了CYP 3A的参与,TAO将AQM的形成抑制至未抑制值的13%,并完全消除了AQ4的形成。α-萘黄酮(ANF),一种CYP 2C和1A的抑制剂,对AQ4N代谢没有显著影响。
结论
这些数据表明人CYP 3A酶可参与AQ4N的还原代谢。CYP 3A酶在多种人类癌症中高度表达。结果表明AQ4N需要厌氧条件才能进行CYP 3A介导的还原,因此该酶亚家族可能在缺氧肿瘤中选择性激活AQ4N。
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