Engineering the cofactor specificity of an alcohol dehydrogenase via single mutations or insertions distal to the 2′-phosphate group of NADP(H)

K. Solanki, Walaa Abdallah, S. Banta
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引用次数: 12

Abstract

There have been many reports exploring the engineering of the cofactor specificity of aldo-keto reductases (AKRs), as this class of proteins is ubiquitous and exhibits many useful activities. A common approach is the mutagenesis of amino acids involved in interactions with the 2'-phosphate group of NADP(H) in the cofactor binding pocket. We recently performed a 'loop-grafting' approach to engineer the substrate specificity of the thermostable alcohol dehydrogenase D (AdhD) from Pyrococcus furiosus and we found that a loop insertion after residue 211, which is on the back side of the cofactor binding pocket, could also alter cofactor specificity. Here, we further explore this approach by introducing single point mutations and single amino acid insertions at the loop insertion site. Six different mutants of AdhD were created by either converting glycine 211 to cysteine or serine or by inserting alanine, serine, glycine or cysteine between the 211 and 212 residues. Several mutants gained activity with NADP+ above the wild-type enzyme. And remarkably, it was found that all of the mutants investigated resulted in some degree of reversal of cofactor specificity in the oxidative direction. These changes were generally a result of changes in conformations of the ternary enzyme/cofactor/substrate complexes as opposed to changes in affinities or binding energies of the cofactors. This study highlights the role that amino acids which are distal to the cofactor binding pocket but are involved in substrate interactions can influence cofactor specificity in AdhD, and this strategy should translate to other AKR family members.
通过单次突变或插入NADP(H)的2 ' -磷酸基远端来设计乙醇脱氢酶的辅助因子特异性
由于醛酮还原酶(AKRs)这类蛋白普遍存在并表现出许多有用的活性,因此已经有许多报道探索了辅助因子特异性的工程设计。一种常见的方法是诱变与辅助因子结合袋中NADP(H)的2'-磷酸基团相互作用的氨基酸。我们最近进行了一种“环接枝”方法来设计来自发热焦球菌的耐热性醇脱氢酶D (AdhD)的底物特异性,我们发现在辅因子结合袋背面的残基211后插入环也可以改变辅因子特异性。在这里,我们通过在环插入位点引入单点突变和单氨基酸插入来进一步探索这种方法。通过将甘氨酸211转化为半胱氨酸或丝氨酸,或在211和212残基之间插入丙氨酸、丝氨酸、甘氨酸或半胱氨酸,产生了六种不同的AdhD突变体。一些突变体获得了野生型酶以上NADP+的活性。值得注意的是,研究发现所有的突变体都导致了氧化方向上辅因子特异性的某种程度的逆转。这些变化通常是由于三元酶/辅因子/底物复合物构象的变化,而不是辅因子的亲和力或结合能的变化。这项研究强调了辅助因子结合袋远端但参与底物相互作用的氨基酸在AdhD中影响辅助因子特异性的作用,这种策略应该适用于其他AKR家族成员。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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