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鉴定白杨质连蛋白过氧化物酶中酪氨酸 74 和 177 为底物氧化位点

Identification of Tyr74 and Tyr177 as substrate oxidation sites in cationic cell wall-bound peroxidase from Populus alba L.

机构信息

Department of Forest and Forest Products Sciences, Kyushu University, Fukuoka, Japan.

出版信息

FEBS J. 2012 Jan;279(2):348-57. doi: 10.1111/j.1742-4658.2011.08429.x. Epub 2011 Dec 9.

DOI:10.1111/j.1742-4658.2011.08429.x
PMID:22099451
Abstract

Cationic cell wall-bound peroxidase (CWPO-C) has the capability to oxidize sinapyl alcohol, ferrocytochrome c, and synthetic lignin polymers, unlike most peroxidases that have been characterized in flowering plants, such as horseradish peroxidase and Arabidopsis thaliana peroxidase A2. It has been suggested that the oxidation site is located on the CWPO-C surface, and homology modeling and chemically modified CWPO-C studies suggest that Tyr74 and/or Tyr177 are possible participants in the catalytic site. The present study clarifies the importance of these Tyr residues for substrate oxidation, using recombinant CWPO-C and recombinant mutant CWPO-C with phenylalanine substitution(s) for tyrosine. Such recombinant proteins, produced in Escherichia coli as inclusion bodies, were successfully refolded to yield the active form, and purified recombinant protein solutions exhibited typical spectra of high-spin ferric protein and displayed H(2) O(2) -dependent oxidation of guaiacol, 2,6-dimethoxyphenol, and syringaldazine. Measurement of peroxidase activity with these guaiacyl and syringyl compounds as reducing substrates indicated that a single mutation, Y74F or Y177F, resulted in substantial loss of oxidation activity (∼ 40-60% and 82%, respectively). Also, over 95% of the oxidation activity was lost with a double mutation, Y74F/Y177F. These results indicated that Tyr74 and Tyr177, rather than the heme pocket, play a central role in the oxidation of these substrates. This is the first report of active residues on an enzyme surface being identified in a plant peroxidase. This study also suggests that sinapyl alcohol incorporation into lignin is performed by a peroxidase that generates Tyr radicals on its surface.

摘要

阳离子细胞壁结合过氧化物酶 (CWPO-C) 具有氧化丁香醇、亚铁细胞色素 c 和合成木质素聚合物的能力,这与已在开花植物中表征的大多数过氧化物酶(如辣根过氧化物酶和拟南芥过氧化物酶 A2)不同。有人提出,氧化部位位于 CWPO-C 表面,同源建模和化学修饰 CWPO-C 研究表明 Tyr74 和/或 Tyr177 可能是催化部位的参与者。本研究使用重组 CWPO-C 和重组突变 CWPO-C(用苯丙氨酸取代酪氨酸),阐明了这些 Tyr 残基对底物氧化的重要性。这些重组蛋白作为包涵体在大肠杆菌中产生,成功地重折叠为活性形式,并且纯化的重组蛋白溶液表现出典型的高自旋铁蛋白光谱,并显示 H(2)O(2)依赖性氧化愈创木酚、2,6-二甲氧基苯酚和愈创木酚嗪。用这些愈创木基和丁香基化合物作为还原底物测量过氧化物酶活性表明,单个突变(Y74F 或 Y177F)导致氧化活性显著丧失(分别约为 40-60%和 82%)。此外,双突变(Y74F/Y177F)导致超过 95%的氧化活性丧失。这些结果表明 Tyr74 和 Tyr177 而不是血红素口袋在这些底物的氧化中起核心作用。这是首次在植物过氧化物酶中鉴定酶表面上的活性残基的报道。本研究还表明,木质素中丁香醇的掺入是由在其表面产生 Tyr 自由基的过氧化物酶完成的。

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