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11-氧化甾体的代谢。肝脏制剂的体外代谢。

Metabolism of 11-oxygenated steroids. Metabolism in vitro by preparations of liver.

作者信息

Bush I E, Hunter S A, Meigs R A

出版信息

Biochem J. 1968 Mar;107(2):239-58. doi: 10.1042/bj1070239.

Abstract
  1. The isolation and partial purification of 11beta-hydroxy steroid dehydrogenase from rat and guinea-pig liver microsomes has been achieved by conventional methods. 2. The efficiency of different 11-oxygenated steroids as substrates has been examined. The relative efficiencies confirm in the main the stereochemical theory of the enzyme-coenzyme-substrate complex that was proposed earlier on the basis of studies in vivo. Delta(4)-3-Ketones and 5alpha-hydrogen steroids are readily metabolized by the enzyme. 5beta-Hydrogen steroids and Delta(4)-3-ketones with certain large alpha-substituents are metabolized to a limited extent or not at all. Halogen substitution in the 9alpha-position enhances the rate of reduction of 11-ketones but blocks the oxidation of the related 11beta-ols. 3. 9alpha-Fluorocortisol is a competitive inhibitor of the oxidation of cortisol, but 9alpha-fluorocortisone is reduced at five to ten times the initial velocity of cortisone. 4. 11beta-Hydroxy steroid dehydrogenase activity has been found in liver microsomes of rat, guinea pig, rabbit and calf. 5. Relative substrate efficiencies and K(m) values are similar in whole (debris-free) homogenates, washed microsomes and acetone-dried powders of washed microsomes. 6. A variety of conditions have been examined for the observation of 11beta-hydroxy steroid dehydrogenase activity. NADP(H) is an efficient and NAD(H) a very poor coenzyme for the reaction.
摘要
  1. 已通过常规方法从大鼠和豚鼠肝脏微粒体中分离并部分纯化了11β-羟基类固醇脱氢酶。2. 研究了不同11-氧化类固醇作为底物的效率。相对效率在很大程度上证实了先前基于体内研究提出的酶-辅酶-底物复合物的立体化学理论。Δ(4)-3-酮和5α-氢类固醇很容易被该酶代谢。5β-氢类固醇和带有某些大α-取代基的Δ(4)-3-酮仅在有限程度上被代谢或根本不被代谢。9α-位的卤素取代提高了11-酮的还原速率,但阻断了相关11β-醇的氧化。3. 9α-氟皮质醇是皮质醇氧化的竞争性抑制剂,但9α-氟可的松的还原速度是可的松初始速度的五到十倍。4. 在大鼠、豚鼠、兔子和小牛的肝脏微粒体中发现了11β-羟基类固醇脱氢酶活性。5. 相对底物效率和K(m)值在全(无碎片)匀浆、洗涤过的微粒体和洗涤过的微粒体的丙酮干粉中相似。6. 已研究了多种观察11β-羟基类固醇脱氢酶活性的条件。NADP(H)是该反应的有效辅酶,而NAD(H)是非常差的辅酶。

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