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Coupling Bioorthogonal Chemistries with Artificial Metabolism: Intracellular Biosynthesis of Azidohomoalanine and Its Incorporation into Recombinant Proteins

机译:生物正交化学与人工代谢的耦合:叠氮高丙氨酸的细胞内生物合成及其并入重组蛋白。

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摘要

In this paper, we present a novel, “single experiment” methodology based on genetic engineering of metabolic pathways for direct intracellular production of non-canonical amino acids from simple precursors, coupled with expanded genetic code. In particular, we engineered the intracellular biosynthesis of l-azidohomoalanine from O-acetyl-l-homoserine and NaN3, and achieved its direct incorporation into recombinant target proteins by AUG codon reassignment in a methionine-auxotroph E. coli strain. In our system, the host’s methionine biosynthetic pathway was first diverted towards the production of the desired non-canonical amino acid by exploiting the broad reaction specificity of recombinant pyridoxal phosphate-dependent O-acetylhomoserine sulfhydrylase from Corynebacterium glutamicum. Then, the expression of the target protein barstar, accompanied with efficient l-azidohomoalanine incorporation in place of l-methionine, was accomplished. This work stands as proof-of-principle and paves the way for additional work towards intracellular production and site-specific incorporation of biotechnologically relevant non-canonical amino acids directly from common fermentable sources.
机译:在本文中,我们基于代谢途径的遗传工程提出了一种新颖的“单一实验”方法,可从简单的前体直接在细胞内生产非规范氨基酸,并结合扩展的遗传密码。特别是,我们设计了由O-乙酰基-1-高丝氨酸和NaN3合成L-叠氮高丙氨酸的细胞内生物合成,并通过甲硫氨酸营养缺陷型大肠杆菌菌株中的AUG密码子重分配将其直接掺入重组靶蛋白中。在我们的系统中,宿主的蛋氨酸生物合成途径首先通过利用谷氨酸棒状杆菌重组磷酸吡ido醛依赖性O-乙酰高丝氨酸巯基酶的广泛反应特异性而转向了所需的非规范氨基酸的生产。然后,完成了目标蛋白barstar的表达,并伴有有效的l-叠氮高丙氨酸取代l-蛋氨酸的掺入。这项工作是原则性的证明,为直接从常见的可发酵来源直接向细胞内生产和生物技术相关的非规范氨基酸的位点特异性结合铺平了道路。

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