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A sulfonium tethered peptide ligand rapidly and selectively modifies protein cysteine in vicinity

机译:sulf拴的肽配体可快速选择性地修饰附近的蛋白质半胱氨酸

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摘要

Significant efforts have been invested to develop site-specific protein modification methodologies in the past two decades. In most cases, a reactive moiety was installed onto ligands with the sole purpose of reacting with specific residues in proteins. Herein, we report a unique peptide macrocyclization method via the bis-alkylation between methionine and cysteine to generate cyclic peptides with significantly enhanced stability and cellular uptake. Notably, when the cyclized peptide ligand selectively recognizes its protein target with a proximate cysteine, a rapid nucleophilic substitution could occur between the protein Cys and the sulfonium center on the peptide to form a conjugate. The conjugation reaction is rapid, facile and selective, triggered solely by proximity. The high target specificity is further proved in cell lysate and hints at its further application in activity based protein profiling. This method enhances the peptide's biophysical properties and generates a selective ligand-directed reactive site for protein modification and fulfills multiple purposes by one modification. This proof-of-concept study reveals its potential for further broad biological applications.
机译:在过去的二十年中,已经投入了大量的精力来开发位点特异性的蛋白质修饰方法。在大多数情况下,仅将反应性部分安装在配体上即可与蛋白质中的特定残基反应。在本文中,我们报告了一种独特的肽大环化方法,该方法通过蛋氨酸和半胱氨酸之间的双烷基化来生成具有显着增强的稳定性和细胞摄取能力的环状肽。值得注意的是,当环化的肽配体选择性地用近半胱氨酸识别其蛋白质靶标时,在蛋白质Cys和肽上的center中心之间可能发生快速的亲核取代,形成结合物。共轭反应是快速,容易和选择性的,仅由邻近性触发。高靶点特异性在细胞裂解物中得到进一步证明,并暗示了其在基于活性的蛋白谱分析中的进一步应用。该方法增强了肽的生物物理特性,并生成了选择性配体导向的反应位点,用于蛋白质修饰,并通过一种修饰实现了多种目的。这项概念验证研究揭示了其在进一步广泛的生物学应用中的潜力。

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