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首页> 外文期刊>Archives of Biochemistry and Biophysics >The role of cysteine 160 in thiamine diphosphate binding of the Calvin-Benson-Bassham cycle transketolase of Rhodobacter sphaeroides
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The role of cysteine 160 in thiamine diphosphate binding of the Calvin-Benson-Bassham cycle transketolase of Rhodobacter sphaeroides

机译:半胱氨酸160在硫代二磷酸硫胺素结合中的作用(球菌红球菌Calvin-Benson-Bassham循环转酮醇酶)

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The transketolase gene (cbbT) that encodes the Calvin-Benson-Bassham pathway transketolase (CbbT) of Rhodobacter sphaeroides was overexpressed in Escherichia coli and the recombinant protein purified to homogeneity. Like other transketolases, R. sphaeroides CbbT was found to be inactivated in the presence of oxygen. At its optimal pH of 7.8, CbbT displays a specific activity of 37 U/mg, a K-R5P of 949 muM, a K-xu5p of 11 muM, and a K-ThDP of 1.8 muM. Cysteine 160, equivalent to Cys159 of the yeast enzyme, is found within the active site and is loosely conserved amongst several sources of transketolase. To investigate the role of cysteine 160 found in the active site of R. sphaeroides CbbT, this residue was targeted for mutagenesis. Cys160 was changed to alanine, serine, aspartate, and glutamate. To compare the effect of these mutations on ThDP binding, spectral techniques were employed in addition to analysis by enzymatic activity. Fluorescence quenching was used to measure both equilibrium binding constants as well as first order rates of binding. The results of these studies indicated that Cys160 played an important and substantial role in cofactor binding, revealing the importance of this loosely conserved residue. In addition, the Cys160 mutants did not appear to alter oxygen-mediated inactivation. (C) 2004 Elsevier Inc. All rights reserved.
机译:编码球形球形红球菌的Calvin-Benson-Bassham途径转酮醇酶(CbbT)的转酮醇酶基因(cbbT)在大肠杆菌中过表达,重组蛋白纯化至均一。像其他转酮酶一样,发现球形红球菌CbbT在氧气存在下被灭活。在其最佳pH值为7.8时,CbbT的比活性为37 U / mg,K-R5P为949μM,K-xu5p为11μM,K-ThDP为1.8μM。在活性位点发现与酵母酶的Cys159等效的半胱氨酸160,在转酮醇酶的几种来源中松散保守。为了调查在球形红球菌CbbT的活性位点中发现的半胱氨酸160的作用,将该残基用于诱变。 Cys160更改为丙氨酸,丝氨酸,天冬氨酸和谷氨酸。为了比较这些突变对ThDP结合的影响,除了通过酶活性进行分析外,还采用了光谱技术。荧光猝灭用于测量平衡结合常数以及结合的一级速率。这些研究的结果表明,Cys160在辅因子结合中起着重要而实质的作用,揭示了这种松散保守的残基的重要性。另外,Cys160突变体似乎没有改变氧介导的失活。 (C)2004 Elsevier Inc.保留所有权利。

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