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白腐真菌黄孢原毛平革菌中木质素酶-I和过氧化物酶-M2的比较

Comparison of ligninase-I and peroxidase-M2 from the white-rot fungus Phanerochaete chrysosporium.

作者信息

Paszczyński A, Huynh V B, Crawford R

出版信息

Arch Biochem Biophys. 1986 Feb 1;244(2):750-65. doi: 10.1016/0003-9861(86)90644-2.

DOI:10.1016/0003-9861(86)90644-2
PMID:3080953
Abstract

Ligninase-I (Mr 42,000-43,000; carbohydrate, 21%) and peroxidase-M2 (Mr 45,000-47,000; carbohydrate, 17%), two representative, hydrogen peroxide-dependent extracellular enzymes produced by ligninolytic cultures of the white-rot fungus Phanerochaete chrysosporium BKM-F-1767, were purified and their properties compared. Spectroscopic studies showed that both native enzymes are heme proteins containing protoporphyrin IX. EPR spectroscopy indicated that iron ions are coordinated with the enzymes' prosthetic groups as high-spin ferriheme complexes. We confirmed reports of others that the ligninase-hydrogen peroxide complex (activated enzyme) reverts to its native state on addition of dithionite or one of the enzyme's substrates (e.g., veratryl alcohol); however, we found that the peroxidase-M2-hydrogen peroxide complex required Mn2+ ions to accomplish a similar cycle. The peroxidase oxidized Mn2+ to a higher oxidation state, and the oxidized Mn acted as a diffusible catalyst able to oxidize numerous organic substrates. Unlike ligninase-I which is found free extracellularly, peroxidase-M2 appears to be associated closely with the fungal mycelium. In its peroxidatic reactions, ligninase-I oxidizes a variety of nonphenolic and phenolic lignin model compounds. In the presence of Mn2+, peroxidase-M2 oxidizes numerous phenolic compounds, especially syringyl (3,5-dimethoxy-4-hydroxyphenyl) and vinyl side-chain substituted substrates. Also, the peroxidase-Mn2+ system (without hydrogen peroxide) expresses oxidase activity against NADPH, GSH, dithiothreitol, and dihydroxymaleic acid, forming hydrogen peroxide at the expense of oxygen. Both enzymes were believed to play roles in lignin degradation, and these are discussed.

摘要

木质素酶-I(分子量42,000 - 43,000;碳水化合物含量21%)和过氧化物酶-M2(分子量45,000 - 47,000;碳水化合物含量17%)是白腐真菌黄孢原毛平革菌(Phanerochaete chrysosporium)BKM-F-1767木质素分解培养物产生的两种典型的、依赖过氧化氢的胞外酶,对它们进行了纯化并比较了其特性。光谱研究表明,两种天然酶都是含有原卟啉IX的血红素蛋白。电子顺磁共振光谱表明,铁离子作为高自旋铁血红素复合物与酶的辅基配位。我们证实了其他人的报道,即木质素酶-过氧化氢复合物(活化酶)在加入连二亚硫酸盐或酶的一种底物(如藜芦醇)后会恢复到其天然状态;然而,我们发现过氧化物酶-M2-过氧化氢复合物需要Mn2+离子来完成类似的循环。过氧化物酶将Mn2+氧化到更高的氧化态,氧化后的Mn作为一种可扩散的催化剂,能够氧化多种有机底物。与细胞外游离存在的木质素酶-I不同,过氧化物酶-M2似乎与真菌菌丝体紧密相关。在其过氧化物反应中,木质素酶-I氧化多种非酚类和酚类木质素模型化合物。在Mn2+存在的情况下,过氧化物酶-M2氧化多种酚类化合物,尤其是丁香基(3,5-二甲氧基-4-羟基苯基)和乙烯基侧链取代的底物。此外,过氧化物酶-Mn2+体系(无过氧化氢)对NADPH、谷胱甘肽、二硫苏糖醇和二羟基马来酸表现出氧化酶活性,以氧气为代价形成过氧化氢。两种酶都被认为在木质素降解中起作用,并对此进行了讨论。

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