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Trends in the Hydrogen-Deuterium Exchange at the Carbon Centers. Preparation of Internal Standards for Quantitative Analysis by LC-MS.碳中心氢氘交换的趋势。通过 LC-MS 进行定量分析的内标制备。
Molecules. 2021 May 18;26(10):2989. doi: 10.3390/molecules26102989.
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Modular control of l-tryptophan isotopic substitution via an efficient biosynthetic cascade.通过高效的生物合成级联反应对 l-色氨酸同位素取代进行模块化控制。
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The chemo- enzymatic synthesis of labeled l-amino acids and some of their derivatives.标记的L-氨基酸及其某些衍生物的化学酶促合成。
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10
Ancestral Tryptophan Synthase Reveals Functional Sophistication of Primordial Enzyme Complexes.祖先色氨酸合成酶揭示原始酶复合物的功能复杂性。
Cell Chem Biol. 2016 Jun 23;23(6):709-15. doi: 10.1016/j.chembiol.2016.05.009. Epub 2016 Jun 9.

通过双蛋白催化实现氨基酸的位点选择性氘代。

Site-Selective Deuteration of Amino Acids through Dual-Protein Catalysis.

机构信息

Department of Chemistry, University of Wisconsin-Madison, Madison, Wisconsin 53706, United States.

出版信息

J Am Chem Soc. 2022 Apr 27;144(16):7327-7336. doi: 10.1021/jacs.2c00608. Epub 2022 Apr 13.

DOI:10.1021/jacs.2c00608
PMID:35416652
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC10634506/
Abstract

Deuterated amino acids have been recognized for their utility in drug development, for facilitating nuclear magnetic resonance (NMR) analysis, and as probes for enzyme mechanism. Small molecule-based methods for the site-selective synthesis of deuterated amino acids typically involve de novo synthesis of the compound from deuterated precursors. In comparison, enzymatic methods for introducing deuterium offer improved efficiency, operating directly on free amino acids to achieve hydrogen-deuterium (H/D) exchange. However, site selectivity remains a significant challenge for enzyme-mediated deuteration, limiting access to desirable deuteration motifs. Here, we use enzyme-catalyzed deuteration, combined with steady-state kinetic analysis and ultraviolet (UV)-vis spectroscopy to probe the mechanism of a two-protein system responsible for the biosynthesis of l--Ile. We show that an aminotransferase (DsaD) can pair with a small partner protein (DsaE) to catalyze Cα and Cβ H/D exchange of amino acids, while reactions without DsaE lead exclusively to Cα-deuteration. With conditions for improved catalysis, we evaluate the substrate scope for Cα/Cβ-deuteration and demonstrate the utility of this system for preparative-scale, selective labeling of amino acids.

摘要

氘代氨基酸在药物开发、促进核磁共振(NMR)分析以及作为酶机制探针方面具有重要作用。用于选择性合成氘代氨基酸的基于小分子的方法通常涉及从头合成化合物,使用氘代前体。相比之下,引入氘的酶方法可提高效率,直接对游离氨基酸进行操作,实现氢-氘(H/D)交换。然而,对于酶介导的氘化,位点选择性仍然是一个重大挑战,限制了对理想氘化基序的获取。在这里,我们使用酶催化的氘化,结合稳态动力学分析和紫外(UV)可见光谱,研究负责 l-异亮氨酸生物合成的双蛋白系统的机制。我们表明,转氨酶(DsaD)可以与小伴侣蛋白(DsaE)配对,催化氨基酸的 Cα 和 Cβ H/D 交换,而没有 DsaE 的反应则专门导致 Cα 氘化。在改进催化的条件下,我们评估了 Cα/Cβ-氘化的底物范围,并展示了该系统在制备规模、氨基酸选择性标记方面的应用。