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来自假单胞菌属菌株CBS 3的4-氯苯乙酸3,4-双加氧酶组分B的纯化及某些性质

Purification and some properties of component B of the 4-chlorophenylacetate 3,4-dioxygenase from Pseudomonas species strain CBS 3.

作者信息

Schweizer D, Markus A, Seez M, Ruf H H, Lingens F

出版信息

J Biol Chem. 1987 Jul 5;262(19):9340-6.

PMID:3036855
Abstract

4-Chlorophenylacetate 3,4-dioxygenase system from Pseudomonas sp. CBS 3 consists of two protein components, a red-brown iron-sulfur protein (component A) which functions as dioxygenase and an orange-colored reductase (component B). Component B was purified by a five-step procedure. Criterion of purity was sodium dodecyl sulfate-polyacrylamide gel electrophoresis, which also showed that the protein consists of one polypeptide species with a molecular weight of 35,000. With gel chromatography on Sephadex G-100 also, a molecular weight of 35,000 was found for the native enzyme, suggesting a monomeric structure for the reductase enzyme. The isoelectric point was determined as pH 4.8. The visible absorption spectrum of the homogeneous protein exhibits maxima at 336, 394, and 458 nm. One mol of FMN, 2.1 mol of iron, and 1.7 mol of acid-labile sulfide were found in one mol of component B. The EPR-spectrum of the reduced form of the enzyme (with NADH) showed two types of signals. The signal at g values of 2.03, 1.94, and 1.90 was assigned to an iron-sulfur cluster of the [2Fe-2S]-type. The properties of the other signal type at g = 2.004 are characteristic of flavosemiquinone radical which does not show coupling to an other paramagnetic center. The apparent Km values for 2,6-dichlorophenolindophenol, cytochrome c, and NADH were calculated from Lineweaver-Burk plots as 6.3, 2.3, and 32 microM, respectively. Inhibitors of the reductase are metal-chelating reagents and sulfhydryl-inhibiting compounds. Component B reduces several redox compounds: 2,6-dichlorophenolindophenol, potassium hexacyanoferrat III, cytochrome c, methylene blue, and nitro blue tetrazolium.

摘要

来自假单胞菌属CBS 3的4-氯苯乙酸3,4-双加氧酶系统由两种蛋白质组分组成,一种是起双加氧酶作用的红棕色铁硫蛋白(组分A),另一种是橙色还原酶(组分B)。组分B通过五步程序进行纯化。纯度标准是十二烷基硫酸钠-聚丙烯酰胺凝胶电泳,该电泳还表明该蛋白质由一种分子量为35,000的多肽组成。通过Sephadex G-100凝胶色谱法也发现天然酶的分子量为35,000,这表明还原酶为单体结构。测定其等电点为pH 4.8。该纯蛋白质的可见吸收光谱在336、394和458 nm处有最大值。在1摩尔组分B中发现1摩尔FMN、2.1摩尔铁和1.摩尔酸不稳定硫化物。该酶还原形式(与NADH一起)的EPR光谱显示出两种类型的信号。g值为2.03、1.94和1.90处的信号归因于[2Fe-2S]型铁硫簇。g = 2.004处另一种信号类型的性质是黄素半醌自由基的特征,该自由基不显示与其他顺磁中心的偶联。根据Lineweaver-Burk图计算,2,6-二氯酚靛酚、细胞色素c和NADH的表观Km值分别为6.3、2.3和32 microM。还原酶的抑制剂是金属螯合剂和巯基抑制化合物。组分B可还原几种氧化还原化合物:2,6-二氯酚靛酚、铁氰化钾III、细胞色素c、亚甲蓝和硝基蓝四唑。

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