Huang Yang, Wu Chengyang, Lu Anjing, Wang Jingzhe, Liang Jian, Sun Han, Yang Liqing, Duan Shixiang, Berezin Andrey A, Wu Chuanliu, Zhang Bo, Wu Yi-Lin, Tsai Yu-Hsuan
School of Basic Medical Sciences, Capital Medical University, Beijing 100069, China.
Institute of Molecular Physiology, Shenzhen Bay Laboratory, Shenzhen 518132, China.
J Am Chem Soc. 2025 Jan 15;147(2):1612-1623. doi: 10.1021/jacs.4c11701. Epub 2025 Jan 3.
Small-molecule fluorophores are invaluable tools for fluorescence imaging. However, means for their covalent conjugation to the target proteins limit applications in multicolor imaging. Here, we identify 2-[(alkylhio)(ryl)ethylene]alononitrile (TAMM) molecules reacting with 1,2-aminothiol at a labeling rate over 10 M s through detailed mechanistic investigation. The fast TAMM molecules and mild reaction conditions enable site-specific labeling of surface proteins in not only cell lines but also primary neurons and living mice. The combination of genetic code expansion and sequence-specific proteolytic cleavage enables selective modification of three different cell surface proteins through iterative TAMM condensation. TAMM condensation is also compatible with Cu-catalyzed azide-alkyne cycloaddition and tetrazine ligation for four-color fluorescent labeling, reaching the maximum available colors of conventional confocal microscopes. Thus, bioconjugation chemistry is no longer the limiting factor for multiplex cell surface protein imaging.
小分子荧光团是荧光成像中非常重要的工具。然而,将它们与目标蛋白共价结合的方法限制了其在多色成像中的应用。在此,我们通过详细的机理研究确定了2-[(烷基硫基)(芳基)乙烯]丙二腈(TAMM)分子与1,2-氨基硫醇以超过10 M⁻¹ s⁻¹的标记速率发生反应。快速的TAMM分子和温和的反应条件不仅能够对细胞系中的表面蛋白进行位点特异性标记,还能对原代神经元和活体小鼠进行标记。遗传密码扩展和序列特异性蛋白水解切割相结合,能够通过迭代TAMM缩合对三种不同的细胞表面蛋白进行选择性修饰。TAMM缩合还与铜催化的叠氮化物-炔烃环加成反应和四嗪连接反应兼容,可用于四色荧光标记,达到了传统共聚焦显微镜的最大可用颜色数。因此,生物共轭化学不再是多重细胞表面蛋白成像的限制因素。
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