Hareland W A, Crawford R L, Chapman P J, Dagley S
J Bacteriol. 1975 Jan;121(1):272-85. doi: 10.1128/jb.121.1.272-285.1975.
The enzyme 4-hydroxyphenylacetate, NAD(P)H:oxygen oxidoreductase (1-hydroxylating) (EC 1.14.13 ...; 4-hydroxyphenylacetate 1-monooxygenase; referred to here as 4-HPA 1-hydroxylase) was induced in Pseudomonas acidovorans when 4-hydroxyphenylacetate (4-PHA) was utilized as carbon source for growth; homogentisate and maleylacetoacetate were intermediates in the degradation of 4-HPA. A preparation of the hydroxylase that was free from homogentisate dioxygenase and could be stored at 4 C in the presence of dithioerythritol with little loss of activity was obtained by ultracentrifuging cell extracts; but when purified 18-fold by affinity chromatography the enzyme became unstable. Flavin adenine dinucleotide and Mg2+ ions were required for full activity. 4-HPA 1-hydrocylase was inhibited by KCl, which was uncompetitive with 4-HPA. Values of Ki determined for inhibitors competitive with 4-HPA were 17 muM dl-4-hydroxymandelic acid, 43 muM 3,4-dihydroxyphenylacetic acid, 87 muM 4-hydroxy-3-methylphenylacetic acid, and 440 muM 4-hydroxyphenylpropionic acid. Apparent Km values for substrates of 4-HPA 1-hydroxylase were 31 muM 4-HPA, 67 muM oxygen, 95 muM reduced nicotinamide adenine dinucleotide (NADH); AND 250 muM reduced nicotinamide adenine dinucleotide phosphate (NADPH). The same maximum velocity was given by NADH and NADPH. A chemical synthesis is described for 2-deutero-4-hydroxyphenylacetic acid. This compound was enzymatically hydroxylated with retention of half the deuterium in the homogentisic acid formed. Activity as substrate or inhibitor of 4-HPA 1-hydroxylase was shown only by those analogues of 4-HPA that possessed a hydroxyl group substituent at C-4 of the benze nucleus. A mechanism is suggested that accounts for this structural requirement and also for the observation that when 4-hydroxyphenoxyacetic acid was attacked by the enzyme, hydroquinone was formed by release of the side chain, probably as glycolic acid. Only one enantiometer of racemic 4-hydroxyhydratropic acid was attacked by 4-HPA 1-hydroxylase; the product, alpha-methylhomogentisic acid (2-(2,5-dihydroxyphenyl)-propionic acid), exhibited optical activity. This observation suggests that, during its shift from C-1 to C-2 of the nucleus, the side chain of the substrate remains bound to a site on the enzyme while a conformational change of the protein permits the necessary movement of the benzene ring.
当食酸假单胞菌利用4-羟基苯乙酸(4-PHA)作为生长碳源时,会诱导产生4-羟基苯乙酸、NAD(P)H:氧氧化还原酶(1-羟化)(EC 1.14.13...;4-羟基苯乙酸1-单加氧酶,本文中称为4-HPA 1-羟化酶);尿黑酸和马来酰乙酰乙酸是4-HPA降解过程中的中间产物。通过对细胞提取物进行超速离心,获得了一种不含尿黑酸双加氧酶的羟化酶制剂,该制剂在二硫赤藓糖醇存在下可于4℃保存,活性损失很小;但通过亲和层析纯化18倍后,该酶变得不稳定。黄素腺嘌呤二核苷酸和Mg2+离子是充分发挥活性所必需的。4-HPA 1-羟化酶受到KCl的抑制,KCl对4-HPA无竞争性。与4-HPA竞争性抑制剂的Ki值分别为:17μM dl-4-羟基扁桃酸、43μM 3,4-二羟基苯乙酸、87μM 4-羟基-3-甲基苯乙酸和440μM 4-羟基苯丙酸。4-HPA 1-羟化酶底物的表观Km值分别为:31μM 4-HPA、67μM氧气、95μM还原型烟酰胺腺嘌呤二核苷酸(NADH)和250μM还原型烟酰胺腺嘌呤二核苷酸磷酸(NADPH)。NADH和NADPH给出相同的最大反应速度。描述了2-氘代-4-羟基苯乙酸的化学合成方法。该化合物经酶促羟化后,在形成的尿黑酸中保留了一半的氘。只有那些在苯核C-4位具有羟基取代基的4-HPA类似物才表现出作为4-HPA 1-羟化酶底物或抑制剂的活性。提出了一种机制来解释这种结构要求,以及当4-羟基苯氧基乙酸被该酶作用时,通过侧链释放形成对苯二酚(可能是乙醇酸)的观察结果。外消旋4-羟基氢化阿托酸只有一种对映体被4-HPA 1-羟化酶作用;产物α-甲基尿黑酸(2-(2,5-二羟基苯基)-丙酸)表现出光学活性。这一观察结果表明,在底物从核的C-1位转移到C-2位的过程中,底物的侧链仍与酶上的一个位点结合,而蛋白质的构象变化允许苯环进行必要的移动。
