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首页> 外文期刊>Applied Microbiology >Fusion of a Flavin-Based Fluorescent Protein to Hydroxynitrile Lyase from Arabidopsis thaliana Improves Enzyme Stability
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Fusion of a Flavin-Based Fluorescent Protein to Hydroxynitrile Lyase from Arabidopsis thaliana Improves Enzyme Stability

机译:基于黄素的荧光蛋白与拟南芥中的羟基腈裂解酶融合提高了酶的稳定性

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Hydroxynitrile lyase from Arabidopsis thaliana ( At HNL) was fused to different fluorescent reporter proteins. Whereas all fusion constructs retained enzymatic activity and fluorescence in vivo and in vitro , significant differences in activity and pH stability were observed. In particular, flavin-based fluorescent reporter (FbFP) fusions showed almost 2 orders of magnitude-increased half-lives in the weakly acidic pH range compared to findings for the wild-type enzyme. Analysis of the quaternary structure of the respective FbFP- At HNL fusion proteins suggested that this increased stability is apparently caused by oligomerization mediated via the FbFP tag. Moreover, the increased stability of the fusion proteins enabled the efficient synthesis of ( R )-mandelonitrile in an aqueous-organic two-phase system at a pH of <5. Remarkably, ( R )-mandelonitrile synthesis is not possible using wild-type At HNL under the same conditions due to the inherent instability of this enzyme below pH 5. The fusion strategy presented here reveals a surprising means for the stabilization of enzymes and stresses the importance of a thorough in vitro characterization of in vivo -employed fluorescent fusion proteins.
机译:将来自拟南芥的羟基腈裂解酶(位于HNL)与不同的荧光报告蛋白融合。尽管所有融合构建体在体内和体外均保留酶活性和荧光,但观察到活性和pH稳定性存在显着差异。特别是,与野生型酶的发现相比,基于黄素的荧光报告基因(FbFP)融合物在弱酸性pH范围内显示出半衰期延长了将近2个数量级。对各个FbFP-At HNL融合蛋白的四级结构的分析表明,这种增加的稳定性显然是由通过FbFP标签介导的寡聚引起的。而且,融合蛋白的增加的稳定性使得能够在pH <5的水-有机两相系统中有效地合成(R)-扁桃腈。值得注意的是,由于该酶在pH低于5时固有的不稳定性,因此在相同条件下无法使用野生型At HNL合成(R)-扁桃腈。此处提出的融合策略揭示了一种令人惊讶的稳定酶方法,并强调体内荧光融合蛋白的全面体外表征的重要性。

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