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大鼠肝脏微粒体的视黄醇酯化作用。脂肪酰基辅酶A:视黄醇酰基转移酶的证据。

Retinol esterification by rat liver microsomes. Evidence for a fatty acyl coenzyme A: retinol acyltransferase.

作者信息

Ross A C

出版信息

J Biol Chem. 1982 Mar 10;257(5):2453-9.

PMID:7061433
Abstract

To explore the nature of retinyl ester synthesis by liver microsomes, membranes prepared from rat or cat liver were incubated under various conditions with [3H] retinol dispersed in dimethyl sulfoxide. When [3H]retinol, buffer, and microsomes were incubated together (basal conditions), some [3H]retinol esterification was consistently observed. However, the rate of esterification could be increased 6- to 11-fold by addition of either palmitoyl-CoA (100 microM) or a fatty acyl CoA-generating system. To determine whether the fatty acid used to esterify [3H]retinol under basal conditions might be derived from an endogenous pool of fatty acyl-CoA associated with the microsomal preparation, microsomes were pretreated at pH 7.4 with 0.5 M hydroxylamine, a reagent that reacts with coenzyme A thioesters to form hydroxamates. This pretreatment reduced the basal reaction by 69%. However, hydroxylamine-treated microsomes still retained acyltransferase activity, as shown by a 24- to 40-fold increase in retinyl ester synthesis after addition of palmitoyl-CoA. When microsomes were incubated with both [3H]retinol and [14C]palmitoyl-CoA of known specific radioactivities, the ratio of 14C to 3H in newly synthesized retinyl palmitate was essentially equal to that of its putative substrates, indicating that [14C]palmitate did not undergo significant isotope dilution prior to acylation of [3H]retinol. These experiments provide direct evidence for retinol esterification catalyzed by a microsomal acyl-CoA:retinol acyltransferase and indirect evidence for a pool of fatty acyl-CoA in isolated liver microsomes that is available to react with [3H]retinol to form esterified retinol.

摘要

为了探究肝微粒体合成视黄酯的本质,将从大鼠或猫肝脏制备的膜在各种条件下与分散于二甲基亚砜中的[3H]视黄醇一起孵育。当[3H]视黄醇、缓冲液和微粒体一起孵育时(基础条件),始终能观察到一些[3H]视黄醇的酯化现象。然而,通过添加棕榈酰辅酶A(100微摩尔)或脂肪酸辅酶A生成系统,酯化速率可提高6至11倍。为了确定在基础条件下用于酯化[3H]视黄醇的脂肪酸是否可能源自与微粒体制备相关的内源性脂肪酸辅酶A池,微粒体在pH 7.4下用0.5 M羟胺进行预处理,羟胺是一种与辅酶A硫酯反应形成异羟肟酸的试剂。这种预处理使基础反应降低了69%。然而,经羟胺处理的微粒体仍保留酰基转移酶活性,如添加棕榈酰辅酶A后视黄酯合成增加24至40倍所示。当微粒体与已知比放射性的[3H]视黄醇和[14C]棕榈酰辅酶A一起孵育时,新合成的棕榈酸视黄酯中14C与3H的比率基本等于其假定底物的比率,表明[14C]棕榈酸在[3H]视黄醇酰化之前未发生明显的同位素稀释。这些实验为微粒体酰基辅酶A:视黄醇酰基转移酶催化的视黄醇酯化提供了直接证据,并为分离的肝微粒体中可与[3H]视黄醇反应形成酯化视黄醇的脂肪酸辅酶A池提供了间接证据。

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