Wolgel S A, Dege J E, Perkins-Olson P E, Jaurez-Garcia C H, Crawford R L, Münck E, Lipscomb J D
Department of Biochemistry, University of Minnesota, Minneapolis 55455.
J Bacteriol. 1993 Jul;175(14):4414-26. doi: 10.1128/jb.175.14.4414-4426.1993.
Protocatechuate 2,3-dioxygenase (2,3-PCD) from Bacillus macerans JJ1b has been purified to homogeneity for the first time. The enzyme catalyzes proximal extradiol ring cleavage of protocatechuate (PCA) with the attendant incorporation of both atoms of oxygen from O2. The holoenzyme has a mass of 143 +/- 7 kDa as determined by ultracentrifugation and other techniques. It is composed of four apparently identical subunits with M(r)s of 35,500, each containing one iron atom. Mössbauer spectroscopy of 57Fe-enriched enzyme showed that the irons are indistinguishable and are high spin (S = 2) Fe2+ in both the uncomplexed and substrate-bound enzyme. However, the quadrupole splitting, delta EQ, and isomer shift, delta, of the Mössbauer spectrum changed from delta EQ = 2.57 mm/s and delta = 1.29 mm/s to delta EQ = 2.73 mm/s and delta = 1.19 mm/s upon PCA binding to the enzyme, showing that the iron environment is altered when substrate is present. The enzyme was also found to bind variable and substoichiometric amounts of Mn2+, but this metal could be removed without loss of activity or stability. The inherently electron paramagnetic resonance (EPR)-silent Fe2+ of the enzyme reversibly bound nitric oxide to produce an EPR-active species (g = 4.11, 3.95; S = 3/2). The specific activity of the enzyme was found to be correlated with the amount of the S = 3/2 species formed, showing that activity is dependent on Fe2+. Anaerobic addition of substrates to the enzyme-nitric oxide complex significantly altered the EPR spectrum, suggesting that substrates bind to or near the iron. The enzyme was inactivated by reagents that oxidize the Fe2+, such as H2O2 and K3FE(CN)6; full activity was restored after reduction of the iron by ascorbate. Steady-state kinetic data were found to be consistent with an ordered bi-uni mechanism in which the organic substrate must add to 2,3-PCD before O2. The enzyme has the broadest substrate range of any of the well-studied catecholic dioxygenases. All substrates have vicinal hydroxyl groups on the aromatic ring except 4-NH2-3-hydroxybenzoate. This is the first substrate lacking vicinal hydroxyl groups reported for catecholic extradiol dioxygenases. 2,3-PCD is the final member of the PCA dioxygenase family to be purified. It is compared with other members of this family as well as other catecholic dioxygenases.
来自浸麻芽孢杆菌JJ1b的原儿茶酸2,3-双加氧酶(2,3-PCD)首次被纯化至同质。该酶催化原儿茶酸(PCA)的近端间位二醇环裂解,并伴随从O₂中摄取氧的两个原子。通过超速离心和其他技术测定,全酶的质量为143±7 kDa。它由四个明显相同的亚基组成,亚基的相对分子质量为35,500,每个亚基含有一个铁原子。对富含⁵⁷Fe的酶进行穆斯堡尔光谱分析表明,在未结合底物和结合底物的酶中,铁无法区分,且均为高自旋(S = 2)的Fe²⁺。然而,当PCA与酶结合后,穆斯堡尔光谱的四极分裂δEQ和同质异能位移δ从δEQ = 2.57 mm/s和δ = 1.29 mm/s变为δEQ = 2.73 mm/s和δ = 1.19 mm/s,表明当底物存在时铁的环境发生了改变。还发现该酶能结合可变的、亚化学计量的Mn²⁺,但去除这种金属不会导致活性或稳定性丧失。该酶内在的电子顺磁共振(EPR)沉默的Fe²⁺可逆地结合一氧化氮,产生一个EPR活性物种(g = 4.11, 3.95;S = 3/2)。发现该酶的比活性与形成的S = 3/2物种的量相关,表明活性依赖于Fe²⁺。向酶 - 一氧化氮复合物中厌氧添加底物会显著改变EPR光谱,表明底物与铁结合或在铁附近结合。该酶会被氧化Fe²⁺的试剂如H₂O₂和K₃Fe(CN)₆失活;用抗坏血酸将铁还原后可恢复全部活性。稳态动力学数据与有序的双单机制一致,即有机底物必须在O₂之前添加到2,3-PCD中。在所有已深入研究的儿茶酚双加氧酶中,该酶具有最宽的底物范围。除了4-NH₂-3-羟基苯甲酸外,所有底物在芳环上都有邻位羟基。这是报道的第一种缺乏邻位羟基的儿茶酚间位二醇双加氧酶底物。2,3-PCD是PCA双加氧酶家族中最后一个被纯化的成员。它与该家族的其他成员以及其他儿茶酚双加氧酶进行了比较。
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