4.8 Article

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

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NATURE CHEMISTRY
Volume -, Issue -, Pages -

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NATURE PORTFOLIO
DOI: 10.1038/s41557-023-01252-8

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The tetrazine ligation is a versatile and fast reaction commonly used for bioorthogonal modifications. However, the incorporation of dienophiles in biomolecules has been limited by the need for externally added reagents. This study introduces a novel strategy, called TyrEx cycloaddition, which enables autonomous dienophile generation in bacteria. This technique has been successfully applied for the labeling of proteins and holds potential for various applications.
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-1 s(-1) 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.

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