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一种酪氨酸羟化酶/多巴氧化酶比率异常高的酪氨酸酶。

A tyrosinase with an abnormally high tyrosine hydroxylase/dopa oxidase ratio.

作者信息

Hernández-Romero Diana, Sanchez-Amat Antonio, Solano Francisco

机构信息

Department of Genetics and Microbiology, University of Murcia, Spain.

出版信息

FEBS J. 2006 Jan;273(2):257-70. doi: 10.1111/j.1742-4658.2005.05038.x.

DOI:10.1111/j.1742-4658.2005.05038.x
PMID:16403014
Abstract

The sequencing of the genome of Ralstonia solanacearum[Salanoubat M, Genin S, Artiguenave F, et al. (2002) Nature 415, 497-502] revealed several genes that putatively code for polyphenol oxidases (PPOs). This soil-borne pathogenic bacterium withers a wide range of plants. We detected the expression of two PPO genes (accession numbers NP_518458 and NP_519622) with high similarity to tyrosinases, both containing the six conserved histidines required to bind the pair of type-3 copper ions at the active site. Generation of null mutants in those genes by homologous recombination mutagenesis and protein purification allowed us to correlate each gene with its enzymatic activity. In contrast with all tyrosinases so far studied, the enzyme NP_518458 shows higher monophenolase than o-diphenolase activity and its initial activity does not depend on the presence of l-dopa cofactor. On the other hand, protein NP_519622 is an enzyme with a clear preference to oxidize o-diphenols and only residual monophenolase activity, behaving as a catechol oxidase. These catalytic characteristics are discussed in relation to two other characteristics apart from the six conserved histidines. One is the putative presence of a seventh histidine which interacts with the carboxy group on the substrate and controls the preference for carboxylated and decarboxylated substrates. The second is the size of the residue isosteric with the aromatic F261 reported in sweet potato catechol oxidase which acts as a gate to control accessibility to CuA at the active site.

摘要

青枯雷尔氏菌的基因组测序[萨拉努巴特M、热南S、阿蒂盖纳夫F等(2002年)《自然》415卷,497 - 502页]揭示了几个可能编码多酚氧化酶(PPO)的基因。这种土壤传播的病原菌会使多种植物枯萎。我们检测到两个与酪氨酸酶高度相似的PPO基因(登录号NP_518458和NP_519622)的表达,这两个基因在活性位点都含有结合一对3型铜离子所需的六个保守组氨酸。通过同源重组诱变在这些基因中产生无效突变体并进行蛋白质纯化,使我们能够将每个基因与其酶活性相关联。与迄今为止研究的所有酪氨酸酶不同,酶NP_518458的单酚酶活性高于邻二酚酶活性,并且其初始活性不依赖于L - 多巴辅因子的存在。另一方面,蛋白质NP_519622是一种明显偏好氧化邻二酚且只有残余单酚酶活性的酶,表现为儿茶酚氧化酶。除了六个保守组氨酸外,还结合另外两个特征对这些催化特性进行了讨论。一个是推测存在第七个组氨酸,它与底物上的羧基相互作用并控制对羧化和脱羧底物的偏好。另一个是与甘薯儿茶酚氧化酶中报道的芳香族F261等排的残基大小,它作为一个门控来控制活性位点处铜A的可及性。

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