Gilmour R, Goodhew C F, Pettigrew G W, Prazeres S, Moura J J, Moura I
Department of Preclinical Veterinary Sciences, Royal (Dick) School of Veterinary Studies, University of Edinburgh, Summerhall, U.K.
Biochem J. 1994 Jun 15;300 ( Pt 3)(Pt 3):907-14. doi: 10.1042/bj3000907.
In work that is complementary to our investigation of the spectroscopic features of the cytochrome c peroxidase from Paracoccus denitrificans [Gilmour, Goodhew, Pettigrew, Prazeres, Moura and Moura (1993) Biochem. J. 294, 745-752], we have studied the kinetics of oxidation of cytochrome c by this enzyme. The enzyme, as isolated, is in the fully oxidized form and is relatively inactive. Reduction of the high-potential haem at pH 6 with ascorbate results in partial activation of the enzyme. Full activation is achieved by addition of 1 mM CaCl2. Enzyme activation is associated with formation of a high-spin state at the oxidized low-potential haem. EGTA treatment of the oxidized enzyme prevents activation after reduction with ascorbate, while treatment with EGTA of the reduced, partially activated, form abolishes the activity. We conclude that the active enzyme is a mixed-valence form with the low-potential haem in a high-spin state that is stabilized by Ca2+. Dilution of the enzyme results in a progressive loss of activity, the extent of which depends on the degree of dilution. Most of the activity lost upon dilution can be recovered after reconcentration. The M(r) of the enzyme on molecular-exclusion chromatography is concentration-dependent, with a shift to lower values at lower concentrations. Values of M(r) obtained are intermediate between those of a monomer (39,565) and a dimer. We propose that the active form of the enzyme is a dimer which dissociates at high dilution to give inactive monomers. From the activity of the enzyme at different dilutions, a KD of 0.8 microM can be calculated for the monomerdimer equilibrium. The cytochrome c peroxidase oxidizes horse ferrocytochrome c with first-order kinetics, even at high ferrocytochrome c concentrations. The maximal catalytic-centre activity ('turnover number') under the assay conditions used is 62,000 min-1, with a half-saturating ferrocytochrome c concentration of 3.3 microM. The corresponding values for the Paracoccus cytochrome c-550 (presumed to be the physiological substrate) are 85,000 min-1 and 13 microM. However, in this case, the kinetics deviate from first-order progress curves at all ferrocytochrome c concentrations. Consideration of the periplasmic environment in Paracoccus denitrificans leads us to propose that the enzyme will be present as the fully active dimer supplied with saturating ferrocytochrome c-550.
在与我们对反硝化副球菌细胞色素c过氧化物酶光谱特征的研究互补的工作中[吉尔摩、古德休、佩蒂格鲁、普拉泽雷斯、莫拉和莫拉(1993年)《生物化学杂志》294卷,745 - 752页],我们研究了该酶氧化细胞色素c的动力学。分离得到的酶处于完全氧化形式,相对无活性。在pH 6时用抗坏血酸还原高电位血红素会导致酶部分活化。加入1 mM氯化钙可实现完全活化。酶的活化与氧化态低电位血红素形成高自旋态有关。用乙二醇双(2 - 氨基乙基醚)四乙酸(EGTA)处理氧化态酶可防止用抗坏血酸还原后活化,而用EGTA处理还原的、部分活化的形式则会消除活性。我们得出结论,活性酶是一种混合价形式,低电位血红素处于高自旋态,由Ca²⁺稳定。酶的稀释会导致活性逐渐丧失,丧失程度取决于稀释程度。稀释后丧失的大部分活性在重新浓缩后可以恢复。分子排阻色谱法测得的酶的相对分子质量(M(r))与浓度有关,在较低浓度时向较低值偏移。测得的M(r)值介于单体(39,565)和二聚体之间。我们提出酶的活性形式是二聚体,在高稀释度下会解离成无活性的单体。根据酶在不同稀释度下的活性,可以计算出单体 - 二聚体平衡的解离常数(KD)为0.8 μM。细胞色素c过氧化物酶以一级动力学氧化马亚铁细胞色素c,即使在高铁细胞色素c浓度较高时也是如此。在所使用的测定条件下,最大催化中心活性(“周转数”)为62,000 min⁻¹,半饱和高铁细胞色素c浓度为3.3 μM。反硝化副球菌细胞色素c - 550(推测为生理底物)的相应值为85,000 min⁻¹和13 μM。然而,在这种情况下,所有高铁细胞色素c浓度下的动力学都偏离一级反应进程曲线。考虑到反硝化副球菌的周质环境,我们提出该酶将以与饱和细胞色素c - 550结合的完全活性二聚体形式存在。
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