Boerman M H, Napoli J L
Department of Biochemistry, School of Medicine and Biomedical Sciences, State University of New York, Buffalo 14214.
J Biol Chem. 1991 Nov 25;266(33):22273-8.
Apo-cellular retinol-binding protein (apoCRBP) activated the hydrolysis of endogenous retinyl esters in rat liver microsomes by a cholate independent retinyl ester hydrolase. A Michaelis-Menten relationship was observed between the apoCRBP concentration and the rate of retinol formation, with half-maximum stimulation at 2.6 +/- 0.6 microM (mean +/- S.D., n = 5). Two other retinol-binding proteins, bovine serum albumin and beta-lactoglobulin, acceptors for the rapid and spontaneous hydration of retinol from membranes, had no effect up to 90 microM. These data suggest activation of the hydrolase by apoCRBP directly, rather than by facilitating removal of retinol from membranes. The hydrolase responding was the cholate-independent/cholate-inhibited retinyl ester hydrolase as shown by: 60% inhibition of the apoCRBP effect by 3 mM cholate; apoCRBP enhancement of retinyl ester hydrolysis in liver microsomes that had no detectable cholate-enhanced activity; inhibition of cholate-dependent, but not apoCRBP-stimulated retinyl ester hydrolysis by rabbit anti-rat cholesteryl esterase. Compared to the rate (mean +/- S.D. of [n] different preparations) supported by 5 microM apoCRBP in liver microsomes of 6.7 +/- 3.7 pmol/min/mg protein [10], microsomes from rat lung, kidney, and testes had endogenous retinyl ester hydrolysis rates of 1.8 +/- 0.3 [5], 0.5 +/- 0.2 [3], and 0.3 +/- 0.2 [5] pmol/min/mg protein, respectively. N-Ethylmaleimide and N-tosyl-L-phenylalanine chloromethyl ketone were potent inhibitors of apoCRBP-stimulated hydrolysis with IC50 values of 0.25 and 0.15 mM, respectively, but phenylmethylsulfonyl fluoride and diisopropyl-fluorophosphate were less effective with IC50 values of 1 mM, indicating the importance of imidazole and sulfhydryl groups to the activity. These data provide evidence of a physiological role for the cholate-independent hydrolase in retinoid metabolism and suggest that apoCRBP is a signal for retinyl ester mobilization.
脱辅基细胞视黄醇结合蛋白(apoCRBP)通过一种不依赖胆酸盐的视黄酯水解酶激活大鼠肝微粒体中内源性视黄酯的水解。在apoCRBP浓度与视黄醇形成速率之间观察到米氏关系,在2.6±0.6微摩尔(平均值±标准差,n = 5)时达到最大刺激的一半。另外两种视黄醇结合蛋白,牛血清白蛋白和β-乳球蛋白,作为视黄醇从膜上快速自发水合的受体,在高达90微摩尔时没有作用。这些数据表明是apoCRBP直接激活水解酶,而不是通过促进视黄醇从膜上的去除。响应的水解酶是不依赖胆酸盐/受胆酸盐抑制的视黄酯水解酶,如下所示:3毫摩尔胆酸盐对apoCRBP的作用有60%的抑制;apoCRBP增强了在没有可检测到的胆酸盐增强活性的肝微粒体中的视黄酯水解;兔抗大鼠胆固醇酯酶抑制了依赖胆酸盐但不抑制apoCRBP刺激的视黄酯水解。与5微摩尔apoCRBP在肝微粒体中支持的速率([n]种不同制剂的平均值±标准差)6.7±3.7皮摩尔/分钟/毫克蛋白质[10]相比,来自大鼠肺、肾和睾丸的微粒体的内源性视黄酯水解速率分别为1.8±0.3[5]、0.5±0.2[3]和0.3±0.2[5]皮摩尔/分钟/毫克蛋白质。N-乙基马来酰亚胺和N-对甲苯磺酰-L-苯丙氨酸氯甲基酮是apoCRBP刺激水解的有效抑制剂,IC50值分别为0.25和0.15毫摩尔,但苯甲基磺酰氟和二异丙基氟磷酸酯效果较差,IC50值为1毫摩尔,表明咪唑和巯基对活性的重要性。这些数据提供了不依赖胆酸盐的水解酶在类视黄醇代谢中的生理作用的证据,并表明apoCRBP是视黄酯动员的信号。
Zotero 插件