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矮牵牛过氧化物酶a:分离、纯化及特性

Petunia peroxidase a: isolation, purification and characteristics.

作者信息

Hendriks T, Wijsman H J, van Loon L C

机构信息

Department of Plant Physiology, Agricultural University, Wageningen, The Netherlands.

出版信息

Eur J Biochem. 1991 Jul 1;199(1):139-46. doi: 10.1111/j.1432-1033.1991.tb16101.x.

DOI:10.1111/j.1432-1033.1991.tb16101.x
PMID:2065669
Abstract

The fast-moving anionic peroxidase isoenzyme variant PRXa was purified from leaves of petunia (Petunia hybrida). Over 1300-fold purification was achieved by subjecting extracellular extracts to two sequential acetone precipitations and resuspending the pellets at pH 5.0 and pH 8.0, respectively, followed by gel filtration and chromatofocusing. The purified enzyme had an absorbance ratio (A405 nm/A280 nm) of 3.6, a molecular mass of about 37 kDa and a pI of 3.8. Three molecular forms with slightly different molecular masses were separated by concanavalin-A--Sepharose affinity chromatography, indicating that these three forms differ in their carbohydrate moieties. The absorption spectrum of PRXa had maxima at 496 and 636 nm and a Soret band at 405 nm. Spectra of compounds I and IV were obtained by titrating a batch of PRXa stored for several months at -20 degrees C with H2O2. The addition of 1 mol H2O2/mol freshly purified PRXa caused the formation of compound II, indicating that freshly isolated PRXa contains a bound hydrogen donor which is lost upon storage. Compound III was obtained from both preparations in the presence of excess H2O2. The pH optimum of PRXa for the reaction with H2O2 and guaiacol was 5.0 and its specific activity 61 mkat/g protein. Among various aromatic compounds, coniferyl alcohol was polymerized by PRXa to presumed lignin-like material. The extracellular localization and high affinity of PRXa for the cinnamic acid derivatives suggest that this isoenzyme functions in the polymerization or cross-linking of lignin in the plant cell wall.

摘要

从矮牵牛(Petunia hybrida)叶片中纯化出快速移动的阴离子过氧化物酶同工酶变体PRXa。通过对细胞外提取物进行两次连续的丙酮沉淀,并分别在pH 5.0和pH 8.0下重悬沉淀,然后进行凝胶过滤和色谱聚焦,实现了超过1300倍的纯化。纯化后的酶的吸光度比(A405 nm/A280 nm)为3.6,分子量约为37 kDa,pI为3.8。通过伴刀豆球蛋白A-琼脂糖亲和色谱分离出三种分子量略有不同的分子形式,表明这三种形式在其碳水化合物部分存在差异。PRXa的吸收光谱在496和636 nm处有最大值,在405 nm处有一个Soret带。通过用H2O2滴定一批在-20℃下储存数月的PRXa,获得了化合物I和IV的光谱。每摩尔新鲜纯化的PRXa加入1摩尔H2O2会导致化合物II的形成,这表明新鲜分离的PRXa含有一个结合的氢供体,该氢供体在储存时会丢失。在过量H2O2存在的情况下,从两种制剂中都获得了化合物III。PRXa与H2O2和愈创木酚反应的最适pH为5.0,其比活性为61 mkat/g蛋白质。在各种芳香族化合物中,松柏醇被PRXa聚合为假定的类木质素物质。PRXa的细胞外定位及其对肉桂酸衍生物的高亲和力表明,这种同工酶在植物细胞壁中木质素的聚合或交联中起作用。

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