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利用内源性β-氨基酸亲双烯体通过四嗪连接进行位点特异性生物正交蛋白质标记。

Site-specific bioorthogonal protein labelling by tetrazine ligation using endogenous β-amino acid dienophiles.

作者信息

Richter Daniel, Lakis Edgars, Piel Jörn

机构信息

Institute of Microbiology, Eidgenössische Technische Hochschule (ETH) Zürich, Zürich, Switzerland.

出版信息

Nat Chem. 2023 Oct;15(10):1422-1430. doi: 10.1038/s41557-023-01252-8. Epub 2023 Jul 3.

Abstract

The tetrazine ligation is an inverse electron-demand Diels-Alder reaction widely used for bioorthogonal modifications due to its versatility, site specificity and fast reaction kinetics. A major limitation has been the incorporation of dienophiles in biomolecules and organisms, which relies on externally added reagents. Available methods require the incorporation of tetrazine-reactive groups by enzyme-mediated ligations or unnatural amino acid incorporation. Here we report a tetrazine ligation strategy, termed TyrEx (tyramine excision) cycloaddition, permitting autonomous dienophile generation in bacteria. It utilizes a unique aminopyruvate unit introduced by post-translational protein splicing at a short tag. Tetrazine conjugation occurs rapidly with a rate constant of 0.625 (15) M s and was applied to produce a radiolabel chelator-modified Her2-binding Affibody and intracellular, fluorescently labelled cell division protein FtsZ. We anticipate the labelling strategy to be useful for intracellular studies of proteins, as a stable conjugation method for protein therapeutics, as well as other applications.

摘要

四嗪连接反应是一种逆电子需求的狄尔斯-阿尔德反应,因其多功能性、位点特异性和快速反应动力学而被广泛用于生物正交修饰。一个主要限制是亲双烯体在生物分子和生物体中的掺入,这依赖于外部添加的试剂。现有的方法需要通过酶介导的连接或非天然氨基酸掺入来引入与四嗪反应的基团。在此,我们报告了一种四嗪连接策略,称为酪胺切除(TyrEx)环加成反应,它允许在细菌中自主生成亲双烯体。该策略利用了通过翻译后蛋白质剪接在短标签处引入的独特氨基丙酮酸单元。四嗪结合反应迅速发生,速率常数为0.625(15)M⁻¹s⁻¹,并被应用于生产放射性标记螯合剂修饰的Her2结合亲和体和细胞内荧光标记的细胞分裂蛋白FtsZ。我们预计这种标记策略将有助于蛋白质的细胞内研究,作为蛋白质治疗药物的稳定偶联方法,以及用于其他应用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7706/10533398/bcbbbabb484d/41557_2023_1252_Fig1_HTML.jpg

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