金属催化的DNA结合剂在活细胞中的解笼作用。
Metal-catalyzed uncaging of DNA-binding agents in living cells.
作者信息
Sánchez Mateo I, Penas Cristina, Vázquez M Eugenio, Mascareñas José L
机构信息
Departamento de Química Orgánica e Centro Singular de Investigación en Química Biolóxica y Materiais Moleculares (CIQUS), Universidade de Santiago de Compostela, 15782 Santiago de Compostela, Spain.
出版信息
Chem Sci. 2014 May 1;2014(5):1901-1907.
Abstract
Attachment of alloc protecting groups to the amidine units of fluorogenic DNA-binding bisbenzamidines or to the amino groups of ethidium bromide leads to a significant reduction of their DNA affinity. More importantly, the active DNA-binding species can be readily regenerated by treatment with ruthenium catalysts in aqueous conditions, even in cell cultures. The catalytic chemical uncaging can be easily monitored by fluorescence microscopy, because the protected products display both different emission properties and cell distribution to the parent compounds.
摘要
将分配保护基团连接到荧光DNA结合双苯甲脒的脒单元上或溴化乙锭的氨基上会导致它们与DNA的亲和力显著降低。更重要的是,即使在细胞培养物中,在水性条件下用钌催化剂处理也可以很容易地再生活性DNA结合物种。催化化学解笼可以通过荧光显微镜轻松监测,因为受保护的产物与母体化合物相比具有不同的发射特性和细胞分布。
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Metal-catalyzed uncaging of DNA-binding agents in living cells.金属催化的DNA结合剂在活细胞中的解笼作用。
Chem Sci. 2014 May 1;2014(5):1901-1907.
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Metal-catalyzed uncaging of DNA-binding agents in living cells†Electronic supplementary information (ESI) available: Synthesis and characterization of the studied molecules and required precursors. NMR, UV, and fluorescence spectra, titrations, control experiments, and detailed procedures for cell uptake and co-staining experiments. See DOI: 10.1039/c3sc53317dClick here for additional data file.金属催化的活细胞中DNA结合剂的光解笼效应†
可获取电子补充信息(ESI):所研究分子及所需前体的合成与表征。核磁共振(NMR)、紫外(UV)和荧光光谱、滴定实验、对照实验以及细胞摄取和共染色实验的详细步骤。见DOI: 10.1039/c3sc53317d
点击此处获取额外数据文件。
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