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Biochemical and physiological characterization of a tau class glutathione transferase from rice (Oryza sativa)

机译:水稻tau类谷胱甘肽转移酶的生化和生理特性

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摘要

The classical phase II detoxification glutathione transferases (GSTs) are key metabolic enzymes that catalyze the conjugation of glutathione to various electrophilic compounds. A tau class GST gene (OsGSTU17) was cloned from rice, which encodes a protein of 223 amino acid residues with a calculated molecular mass of 25.18 kDa. The recombinant OsGSTU17 formed a homodimer protein and showed GSH-conjugating activity with various xenobiotics. Kinetic analysis with respect to NBD-Cl as substrate revealed a K-m of 0.324 mM and V-max of 0.219 mu mol/min per mg of protein. The enzyme had a maximum activity at pH 7.5, and a high thermal stability with 81% of its initial activity at 55 degrees C for 15 min. Site-directed mutagenesis revealed that Ser15 in the N-terminal domain is a critical catalytic residue, responsible for stabilisation of the thiolate anion of enzyme-bound glutathione. OsGSTU17 mRNA was expressed in different tissues of rice, both above and below ground. The relative transcript levels of OsGSTU17 mRNA varied significantly among the tissues in response to CDNB, hydrogen peroxide and atrazine treatments, indicating the gene has diverse regulation mechanisms in response to abiotic stresses.
机译:经典的II期解毒谷胱甘肽转移酶(GST)是催化谷胱甘肽与各种亲电化合物结合的关键代谢酶。从水稻中克隆出tau类GST基因(OsGSTU17),该基因编码223个氨基酸残基的蛋白质,计算分子量为25.18 kDa。重组OsGSTU17形成了同型二聚体蛋白,并显示了与各种异源生物的GSH结合活性。关于作为底物的NBD-Cl的动力学分析表明,每mg蛋白质的K-m为0.324mM,V-max为0.219μmol/ min。该酶在pH 7.5时具有最大活性,并具有很高的热稳定性,在55摄氏度下15分钟的初始活性为其初始活性的81%。定点诱变显示,N末端结构域中的Ser15是关键的催化残基,负责稳定酶结合的谷胱甘肽的硫醇根阴离子。 OsGSTU17 mRNA在水稻不同组织中在地面以上和地下均表达。响应CDNB,过氧化氢和at去津处理,组织中OsGSTU17 mRNA的相对转录水平显着变化,表明该基因具有响应非生物胁迫的多种调控机制。

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