The protoporphyrin-apoperoxidase complex as a horseradish peroxidase analog

N.N. Ugarova, A.P. Savitski, I.V. Berezin
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引用次数: 34

Abstract

Similarity of the protein tertiary structures of the native horseradish peroxidase (donor: hydrogen-peroxide oxidoreductase, EC 1.11.1.7) and protoporphyrin-apoperoxidase complex has been shown on the basis of identity of the tryptophan fluorescence parameter at pH 2.0–8.0 and of the circular dichroism spectra of the two proteins. Absorption and fluorescence spectra have been obtained for protoporphyrin in the complex in the pH range 7.0–1.6. A shift in the apparent pK by 4 units has been observed for protonation of the protoporphyrin pyrrolic ring in the complex. From this shift, the dielectric constant has been evaluated for the heme pocket of the peroxidase (approx. 20). Fluorescence quantum yield of protoporphyrin in the complex increased with pH decreasing from 5.0 to 3.5, whereas the spectrum pattern and fluorescence lifetime did not change. The ions, I and [Fe(CN)6]−4, peroxidase substrates, did not quench the protoporphyrin fluorescence in the complex at about neutral pH, whereas the quenching markedly enhanced with lowering pH. The bimolecular constant for the I-quenching of the porphyrin fluorescence in the complex showed a pH-dependence similar to that of the bimolecular rate constant for the reaction of peroxidase compound I with I. A mechanism for I oxidation at an acid pH in the presence of peroxidase has been proposed.

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原卟啉-过氧化物酶复合物是一种辣根过氧化物酶类似物
根据色氨酸在pH 2.0 ~ 8.0的荧光参数和两种蛋白的圆二色性光谱的一致性,表明了天然辣根过氧化物酶(供体:过氧化氢氧化还原酶,EC 1.11.1.7)和原卟啉-过氧化物酶复合物的蛋白质三级结构的相似性。在pH 7.0 ~ 1.6范围内获得了配合物中原卟啉的吸收光谱和荧光光谱。在配合物中原卟啉吡啶环的质子化过程中,表观pK发生了4个单位的变化。从这一变化,已经评估了介电常数为过氧化物酶的血红素袋(约。20). 配合物中原卟啉的荧光量子产率随pH从5.0降低到3.5而增加,而光谱模式和荧光寿命没有变化。过氧化物酶底物离子I−和[Fe(CN)6]−4在中性pH下不猝灭配合物中的原卟啉荧光,而随着pH的降低,猝灭作用明显增强。配合物中卟啉荧光的I−猝灭双分子常数与过氧化物酶化合物I与I−反应的双分子速率常数具有类似的pH依赖性。提出了一种在酸性pH下过氧化物酶存在下的I−氧化机制。
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