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在雌性B6C3F1小鼠中,SKF 525 - A通过诱导细胞色素P - 450 2B来诱导可卡因N - 脱甲基酶、乙氧芴香豆素O - 脱乙基酶和戊氧芴香豆素O - 脱烷基酶的活性。

Skf 525-A induces cocaine N-demethylase, ethoxyresorufin O-deethylase, and pentoxyresorufin O-dealkylase activities by induction of cytochrome p-450 2B in female B6C3F1 mice.

作者信息

Jeong Tae Cheon, Chang Hyeun Wook, Lee Eung Seok, Jeon Tae Won, Jeong Hye Gwang, Holsapple Michael P

机构信息

College of Pharmacy, Yeungnam University, Kyungsan, South Korea.

出版信息

J Toxicol Environ Health A. 2004 Dec;67(23-24):1955-70. doi: 10.1080/15287390490514606.

Abstract

Studies demonstrated that cocaine-induced immunosuppression is mediated by metabolites of cocaine. Although SKF 525-A inhibited cocaine N-demethylation in liver S9 fractions isolated from female B6C3F1 mice, our study showed that pretreatment of mice with SKF 525-A potentiated cocaine-induced suppression of the antibody response to sheep red blood cells. An increase in formaldehyde generation was subsequently shown following incubation of cocaine with the S9 fractions prepared from SKF 525-A-treated mice, indicating the possibility of cytochrome P-450 (CYP) induction. Therefore, the inductive effects of SKF 525-A on CYP enzyme activities and proteins were investigated in female B6C3F1 mice to elucidate the potentiation of cocaine-induced immunosuppression by SKF 525-A. When SKF 525-A was administered at 10, 20, or 40 mg/kg/d intraperitoneally for 7 consecutive days, both ethoxyresorufin O-deethylase and pentoxyresorufin O-dealkylase activities were induced dose-dependently. Furthermore, the induction of enzymatic activity was time dependent. Meanwhile, when the type of isozyme induced by SKF 525-A was analyzed by Western immunoblotting with monospecific anti-CYP 1A and anti-CYP 2B antibodies, only the CYP 2B appeared to be induced. From in vitro inhibition studies with monoclonal antibodies, it was confirmed that the induced activity of ethoxyresorufin O-deethylase by SKF 525-A was due to increased levels of CYP 2B proteins. Our present results provide an explanation for the potentiation of cocaine-induced immunosuppression by repeated exposure to SKF 525-A. Our results also indicate that ethoxyresorufin O-deethylase, a selective substrate for CYP 1A, may also be catalyzed by CYP 2B.

摘要

研究表明,可卡因诱导的免疫抑制是由可卡因的代谢产物介导的。虽然SKF 525 - A抑制了从雌性B6C3F1小鼠分离的肝脏S9组分中可卡因的N - 去甲基化,但我们的研究表明,用SKF 525 - A预处理小鼠可增强可卡因诱导的对绵羊红细胞抗体反应的抑制作用。随后发现,将可卡因与从用SKF 525 - A处理的小鼠制备的S9组分一起孵育后,甲醛生成增加,这表明细胞色素P - 450(CYP)诱导的可能性。因此,在雌性B6C3F1小鼠中研究了SKF 525 - A对CYP酶活性和蛋白质的诱导作用,以阐明SKF 525 - A对可卡因诱导的免疫抑制的增强作用。当以10、20或40 mg/kg/d的剂量连续7天腹腔注射SKF 525 - A时,乙氧异吩恶唑酮O - 脱乙基酶和戊氧异吩恶唑酮O - 脱烷基酶的活性均呈剂量依赖性诱导。此外,酶活性的诱导具有时间依赖性。同时,当用单特异性抗CYP 1A和抗CYP 2B抗体通过Western免疫印迹分析SKF 525 - A诱导的同工酶类型时,似乎只有CYP 2B被诱导。通过单克隆抗体的体外抑制研究证实,SKF 525 - A诱导的乙氧异吩恶唑酮O - 脱乙基酶活性是由于CYP 2B蛋白水平的增加。我们目前的结果为反复暴露于SKF 525 - A增强可卡因诱导的免疫抑制提供了解释。我们的结果还表明,CYP 1A的选择性底物乙氧异吩恶唑酮O - 脱乙基酶也可能由CYP 2B催化。

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