从视黄醛合成全反式维甲酸。一种纯化的胞质脱氢酶将与细胞视黄醇结合蛋白（I型）结合的视黄醛识别为底物。

Biosynthesis of all-trans-retinoic acid from retinal. Recognition of retinal bound to cellular retinol binding protein (type I) as substrate by a purified cytosolic dehydrogenase.

作者信息

Posch K C, Burns R D, Napoli J L

机构信息

Department of Biochemistry, School of Medicine and Biomedical Sciences, State University of New York, Buffalo 14214.

出版信息

J Biol Chem. 1992 Sep 25;267(27):19676-82.

PMID:1527087

Abstract

An NAD-dependent rat liver cytosolic dehydrogenase accepted as substrate retinal generated in situ by microsomes from retinol bound to excess CRBP (cellular retinol binding protein, type I). This activity, which was not retained by anion-exchange chromatography at pH 9.15, was designated P1. P1 activity increased 2.5-fold, with no statistically significant change in its K or Hill coefficient, in liver cytosol from rats fed a retinoid-deficient diet. Orally dosed retinoic acid partially suppressed the increase. Activities chromatographically similar to hepatic P1 were observed in cytosols from rat kidney and testes. P1, purified from rat liver cytosol, had a pI of approximately 8.3, migrated as a tetramer (214 kDa) on a Sephadex G-200 column, and had a subunit molecular mass of 55 kDa by sodium dodecyl sulfate-polyacrylamide gel electrophoresis. With free retinal it catalyzed a maximum rate of retinoic acid synthesis of 265 nmol/min/mg of protein and exhibited allosteric kinetics with a K of 0.76 +/- 0.35 microM and a Hill coefficient of 1.5 +/- 0.13 (mean +/- S.D., n = 4). Substrate inhibition was noted with retinal concentrations greater than 6 microM. The purified enzyme not only recognized retinal generated by microsomes as substrate, but also recognized retinal bound to CRBP. The rates of retinoic acid synthesis from CRBP-retinal, with a series of increasing apoCRBP concentrations, exceeded the rates that would be supported by the free retinal present. The CRBP-retinal complex exhibited allosteric kinetics (K, 0.13 microM; Hill coefficient, 1.75; averages of duplicates) in the presence of excess apoCRBP (the ratio total CRBP/total retinal at each concentration of retinal was 2). This enzyme is likely to play a significant role in retinoic acid synthesis in vivo, because it participates in the synthesis of retinoic acid from a physiologically occurring form of retinol (holoCRBP), reflects retinoid status, and is distributed in extrahepatic tissues in addition to liver. These results also suggest a novel role for CRBP in retinoid metabolism, facilitating the conversion of retinal into retinoic acid.

摘要

一种依赖烟酰胺腺嘌呤二核苷酸（NAD）的大鼠肝脏胞质脱氢酶，可将与过量细胞视黄醇结合蛋白I（CRBP）结合的视黄醇经微粒体原位生成的视黄醛作为底物。这种在pH 9.15时不能被阴离子交换色谱保留的活性被命名为P1。在喂食类维生素A缺乏饮食的大鼠肝脏胞质中，P1活性增加了2.5倍，其米氏常数（K）或希尔系数无统计学显著变化。口服给予的视黄酸部分抑制了这种增加。在大鼠肾脏和睾丸的胞质中观察到色谱行为与肝脏P1相似的活性。从大鼠肝脏胞质中纯化得到的P1，其等电点约为8.3，在葡聚糖凝胶G - 200柱上以四聚体（214 kDa）形式迁移，通过十二烷基硫酸钠 - 聚丙烯酰胺凝胶电泳测得其亚基分子量为55 kDa。对于游离视黄醛，它催化视黄酸合成的最大速率为265 nmol/（min·mg蛋白），表现出别构动力学，米氏常数K为0.76±0.35 μM，希尔系数为1.5±0.13（平均值±标准差，n = 4）。当视黄醛浓度大于6 μM时会出现底物抑制现象。纯化后的酶不仅将微粒体生成的视黄醛识别为底物，还能识别与CRBP结合的视黄醛。在一系列不断增加的脱辅基CRBP浓度下，从CRBP - 视黄醛合成视黄酸的速率超过了游离视黄醛所支持的速率。在存在过量脱辅基CRBP（在每个视黄醛浓度下总CRBP/总视黄醛的比例为2）的情况下，CRBP - 视黄醛复合物表现出别构动力学（K为0.13 μM；希尔系数为1.75；重复测量平均值）。这种酶可能在体内视黄酸合成中发挥重要作用，因为它参与从生理形式的视黄醇（全反式视黄醇结合蛋白，holoCRBP）合成视黄酸，反映类维生素A状态，并且除肝脏外还分布于肝外组织。这些结果还提示CRBP在类维生素A代谢中具有新的作用，即促进视黄醛转化为视黄酸。