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通过差速离心和钙聚集制备的微粒体中的UDP葡萄糖醛酸基转移酶和混合功能氧化酶活性。

UDP glucuronosyltransferase and mixed function oxidase activity in microsomes prepared by differential centrifugation and calcium aggregation.

作者信息

Aitio A, Vainio H

出版信息

Acta Pharmacol Toxicol (Copenh). 1976;39(5):555-61. doi: 10.1111/j.1600-0773.1976.tb03205.x.

Abstract

Microsomes were prepared from the liver, kidney and lung of phenobarbital or 20-methylcholanthrene treated and control rats with the conventional ultracentrifugation and calcium aggregation methods. The two methods were compared as to the yield of microsomal protein, amount of cytochrome P-450/448 and activity of UDP-GLUCURONOSYLTRANSFERASE, BENZOPYRENE HYDROXYLASE AND P-NITROANISOLE O-demethylase. The absolute amount of cytochrome P-450/448 (nmol/g wet weight), as well as the enzymatic activities dependent on it (nmol produced/g wet weight) did not differ significantly in any tissue of either treated or control animals nor did that of UDPglucuronosyltransferase. However, the ultracentrifugation method resulted in a slightly smaller yield of the hepatic microsomal protein and a correspondingly higher yield of cytochrome P-450/448 per mg protein as well as higher specific enzymatic activities of both the consecutive drug biotransformation reactions studied. The specific activity of UDPglucuronosyltransferase in digitonin treated microsomes was twice as high in the conventional microsomes as in the calcium aggregated microsomes; no differences was found in the trypsin treated microsomes. The specific activity of the hepatic benzpyrene hydroxylase of the benzpyrene treated animals in the calcium harvested microsomes was 55 per cent of that in the ultracentrifugated microsomes.

摘要

采用传统超速离心法和钙聚集法,从经苯巴比妥或20-甲基胆蒽处理的大鼠以及对照大鼠的肝脏、肾脏和肺中制备微粒体。比较了这两种方法在微粒体蛋白产量、细胞色素P-450/448含量以及UDP-葡糖醛酸基转移酶、苯并芘羟化酶和对硝基苯甲醚O-脱甲基酶活性方面的差异。无论是处理组还是对照组动物的任何组织中,细胞色素P-450/448的绝对量(nmol/g湿重)以及依赖于它的酶活性(nmol生成/g湿重),与UDP-葡糖醛酸基转移酶的情况一样,均无显著差异。然而,超速离心法导致肝微粒体蛋白产量略低,相应地每毫克蛋白中细胞色素P-450/448的产量较高,同时所研究的连续药物生物转化反应的比酶活性也较高。在洋地黄皂苷处理的微粒体中,UDP-葡糖醛酸基转移酶的比活性在传统微粒体中是钙聚集微粒体中的两倍;在胰蛋白酶处理的微粒体中未发现差异。在钙聚集微粒体中,经苯并芘处理的动物肝脏苯并芘羟化酶的比活性是超速离心微粒体中的55%。

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