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生物组织中细胞色素P-448活性的测定。

Determination of cytochrome P-448 activity in biological tissues.

作者信息

Phillipson C E, Godden P M, Lum P Y, Ioannides C, Parke D V

出版信息

Biochem J. 1984 Jul 1;221(1):81-8. doi: 10.1042/bj2210081.

Abstract

Three enzymes used for the determination of cytochrome P-448 activity, namely aryl hydrocarbon hydroxylase, biphenyl 2-hydroxylase and ethoxyresorufin O-de-ethylase, were evaluated with respect to their specificity, sensitivity and inducibility. Purified cytochrome P-448 (LM4), but not cytochrome P-450 (LM2), catalysed the O-de-ethylation of ethoxyresorufin in a reaction that was markedly inhibited by 9-hydroxyellipticine. After the administration of 3-methylcholanthrene to rats all three activities were induced, the extent of induction being highest for ethoxyresorufin O-de-ethylase. Administration of very small doses of benzo[a]pyrene (50 micrograms/kg) to rats to induce cytochrome P-448 specifically increased only the O-de-ethylation of ethoxyresorufin. 3-Hydroxybenzo[a]pyrene, the major metabolite determined by the aryl hydrocarbon hydroxylase assay, undergoes further NADPH-dependent oxygenation leading to loss of fluorescence. On the basis of these observations and those by other workers, we conclude that ethoxyresorufin O-de-ethylase provides the most specific, sensitive and reproducible means of determining cytochrome P-448 activity.

摘要

针对用于测定细胞色素P - 448活性的三种酶,即芳烃羟化酶、联苯2 - 羟化酶和乙氧异吩恶唑酮O - 脱乙基酶,评估了它们的特异性、敏感性和诱导性。纯化的细胞色素P - 448(LM4)而非细胞色素P - 450(LM2)催化乙氧异吩恶唑酮的O - 脱乙基反应,该反应被9 - 羟基玫瑰树碱显著抑制。给大鼠施用3 - 甲基胆蒽后,所有三种活性均被诱导,其中乙氧异吩恶唑酮O - 脱乙基酶的诱导程度最高。给大鼠施用极少量的苯并[a]芘(50微克/千克)以特异性诱导细胞色素P - 448,仅增加了乙氧异吩恶唑酮的O - 脱乙基反应。芳烃羟化酶测定所确定的主要代谢产物3 - 羟基苯并[a]芘会发生进一步的依赖于NADPH的氧化反应,导致荧光丧失。基于这些观察结果以及其他研究人员的观察结果,我们得出结论,乙氧异吩恶唑酮O - 脱乙基酶为测定细胞色素P - 448活性提供了最特异、敏感且可重复的方法。

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