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铜(II)在pH值影响下向无锌牛红细胞超氧化物歧化酶的空锌结合位点迁移。

pH-dependent migration of copper(II) to the vacant zinc-binding site of zinc-free bovine erythrocyte superoxide dismutase.

作者信息

Valentine J S, Pantoliano M W, McDonnell P J, Burger A R, Lippard S J

出版信息

Proc Natl Acad Sci U S A. 1979 Sep;76(9):4245-9. doi: 10.1073/pnas.76.9.4245.

Abstract

Bovine erythrocyte superoxide dismutase (Cu(2)Zn(2)SODase; superoxide:superoxide oxidoreductase, EC 1.15.1.1) consists of two identical subunits each containing Cu(2+) and Zn(2+) in close proximity. We describe here electron spin resonance (ESR) and visible absorption spectroscopic studies of the zinc-free derivative of this protein, Cu(2)E(2)SODase (E = empty) over the pH range 6-10. The ESR spectrum of the zinc-free protein at 77 K is markedly pH dependent. At pH < 8.0 the ESR spectrum is axial in appearance. At pH > 8.0, the lineshape becomes increasingly distorted with increasing pH until, at pH = 9.5, the spectrum is very broad and resembles that of the four-copper derivative Cu(2)Cu(2)SODase and of model imidazolate-bridged binuclear Cu(II) complexes. ESR spectra at 30 degrees C are also consistent with formation of Cu(II)-Im-Cu(II). A plot of changes in the signal amplitude of g perpendicular for Cu(2)E(2)SODase as a function of pH gives an apparent pK(a) of 8.2 for the transition. The long-wavelength absorption with lambda(max) = 700 nm characteristic of Cu(2)E(2)SODase shifts with increasing pH to 800 nm and the resulting visible spectrum is identical to that of Cu(2)Cu(2)SODase. All of the above-mentioned spectroscopic changes induced by additions of NaOH are reversed when the pH is decreased with HNO(3), although the approach to equilibrium is slow in the latter case. The results of these experiments are consistent with a reversible, pH-dependent migration of Cu(2+) from the native copper site of one subunit of the zinc-free protein to the empty zinc site of another subunit. By contrast, native protein, Cu(2)Zn(2)SODase, and the four-copper protein, Cu(2)Cu(2)SODase, show no variation in visible or ESR spectral properties in this pH range. Some previous results concerning the activity of Cu(2)E(2)SODase and its thermal stability are reexamined in light of these new findings.

摘要

牛红细胞超氧化物歧化酶(Cu(2)Zn(2)SOD酶;超氧化物:超氧化物氧化还原酶,EC 1.15.1.1)由两个相同的亚基组成,每个亚基都含有紧密相邻的Cu(2+)和Zn(2+)。我们在此描述了该蛋白质的无锌衍生物Cu(2)E(2)SOD酶(E = 空)在pH值6 - 10范围内的电子自旋共振(ESR)和可见吸收光谱研究。无锌蛋白质在77 K时的ESR光谱明显依赖于pH值。在pH < 8.0时,ESR光谱呈轴向。在pH > 8.0时,随着pH值升高,谱线形状越来越扭曲,直到在pH = 9.5时,光谱非常宽,类似于四铜衍生物Cu(2)Cu(2)SOD酶和咪唑桥联双核Cu(II)配合物模型的光谱。30℃时的ESR光谱也与Cu(II)-Im-Cu(II)的形成一致。以Cu(2)E(2)SOD酶垂直g值信号幅度变化对pH值作图,得到该转变的表观pK(a)为8.2。Cu(2)E(2)SOD酶特征性的λ(max) = 700 nm的长波长吸收随着pH值升高向800 nm移动,所得可见光谱与Cu(2)Cu(2)SOD酶的相同。当用HNO(3)降低pH值时,添加NaOH引起的上述所有光谱变化都可逆转,尽管在后一种情况下达到平衡的过程较慢。这些实验结果与Cu(2+)从无锌蛋白质一个亚基的天然铜位点向另一个亚基的空锌位点进行可逆的、pH值依赖性迁移一致。相比之下,天然蛋白质Cu(2)Zn(2)SOD酶和四铜蛋白质Cu(2)Cu(2)SOD酶在该pH范围内的可见或ESR光谱性质没有变化。根据这些新发现,重新审视了一些先前关于Cu(2)E(2)SOD酶活性及其热稳定性的结果。

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