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用丙酮预处理小鼠对微粒体二甲基亚硝胺 -N- 脱甲基酶的刺激作用。

Stimulation of microsomal dimethylnitrosamine-N-demethylase by pretreatment of mice with acetone.

作者信息

Sipes I G, Slocumb M L, Holtzman G

出版信息

Chem Biol Interact. 1978 Jun;21(2-3):155-66. doi: 10.1016/0009-2797(78)90016-9.

Abstract

To further investigate the relationship between in vivo microsomal enzyme modifiers and in vitro dimethylnitrosamine (DMN) metabolism, male C57BL/6J mice were pretreated with acetone or Aroclor 1254, two compounds known to influence DMN-N-demethylase activity. Pretreatment with acetone enhanced the in vitro microsomal activity of DMN-N-demethylase, as measured by formaldehyde production from DMN. Accompanying this acetone-enhanced demethylase activity was an increase in the covalent binding of [14C]DMN to RNA, protein and DNA. Four distinct Km values dependent on the substrate concentration were observed for the N-demethylase present in control microsomes. Only one Km value was observed for the demethylase in microsomes from acetone-treated animals, but it was significantly lower than the lowest Km observed in the control microsomes. At DMN concentrations of 1 and 10 mM, acetone significantly increased N-demethylation of DMN as compared to control, but not at 100 mM DMN. Aroclor 1254 pretreatment repressed DMN-N-demethylase at 1 mM DMN but enhanced it at 100 mM. These results suggest that there may be multiple forms of DMN-N-demethylase which are dependent on DMN concentration and respond differently to modifiers of the microsomal drug-metabolizing enzymes.

摘要

为了进一步研究体内微粒体酶修饰剂与体外二甲基亚硝胺(DMN)代谢之间的关系,对雄性C57BL/6J小鼠用丙酮或多氯联苯1254进行预处理,这两种化合物已知会影响DMN-N-脱甲基酶活性。用丙酮预处理可增强DMN-N-脱甲基酶的体外微粒体活性,通过DMN产生甲醛来测定。伴随着这种丙酮增强的脱甲基酶活性,[14C]DMN与RNA、蛋白质和DNA的共价结合增加。在对照微粒体中存在的N-脱甲基酶观察到四个依赖于底物浓度的不同Km值。在丙酮处理动物的微粒体中,脱甲基酶仅观察到一个Km值,但它显著低于对照微粒体中观察到的最低Km值。在DMN浓度为1和10 mM时,与对照相比,丙酮显著增加了DMN的N-脱甲基作用,但在100 mM DMN时没有。多氯联苯1254预处理在1 mM DMN时抑制DMN-N-脱甲基酶,但在100 mM时增强它。这些结果表明,可能存在多种形式的DMN-N-脱甲基酶,它们依赖于DMN浓度,并且对微粒体药物代谢酶的修饰剂有不同反应。

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