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利用小分子荧光传感器按需可视化细胞内隔室化的镁。

Visualizing Compartmentalized Cellular Mg on Demand with Small-Molecule Fluorescent Sensors.

机构信息

Department of Chemistry, New York University , New York, New York 10003, United States.

出版信息

J Am Chem Soc. 2016 Nov 9;138(44):14639-14649. doi: 10.1021/jacs.6b07927. Epub 2016 Oct 26.

DOI:10.1021/jacs.6b07927
PMID:27750004
Abstract

The study of intracellular metal ion compartmentalization and trafficking involved in cellular processes demands sensors with controllable localization for the measurement of organelle-specific levels of cations with subcellular resolution. We introduce herein a new two-step strategy for in situ anchoring and activation of a fluorescent Mg sensor within an organelle of choice, using a fast fluorogenic reaction between a tetrazine-functionalized pro-sensor, Mag-S-Tz, and a strained bicyclononyne conjugated to a genetically encoded HaloTag fusion protein of known cellular localization. Protein conjugation does not affect the metal-binding properties of the o-aminophenol-N,N,O-triacetic acid (APTRA)-based fluorescent indicator, which displays a dissociation constant K = 3.1 mM suitable for the detection of low millimolar concentrations of chelatable Mg typical of the intracellular environment. We demonstrate the application of our sensing system for the ratiometric detection of Mg in target organelles in HEK 293T cells, providing the first direct comparison of subcellular pools of the metal without interfering signal from other compartments. Activation of the fluorescence in situ through a fluorogenic conjugation step effectively constrains the fluorescence signal to the locale of interest, thus improving the spatial resolution in imaging applications and eliminating the need for washout of mislocalized sensor. The labeling strategy is fully compatible with live cell imaging, and provides a valuable tool for tracking changes in metal distribution that to date have been an unsolved mystery in magnesium biology.

摘要

研究细胞内金属离子区室化和运输在细胞过程中所涉及的问题,需要具有可控定位的传感器,以测量亚细胞分辨率下细胞器中特定阳离子的水平。我们在此引入了一种新的两步策略,用于在细胞器内原位锚定和激活荧光 Mg 传感器,该策略利用四嗪功能化前体传感器 Mag-S-Tz 与固定在已知细胞定位的基因编码 HaloTag 融合蛋白上的应变双环壬炔之间的快速荧光反应。蛋白质偶联不会影响基于邻氨基酚-N,N,O-三乙酸(APTRA)的荧光指示剂的金属结合特性,该指示剂的解离常数 K = 3.1 mM,适用于检测典型细胞内环境中可螯合 Mg 的低毫摩尔浓度。我们展示了我们的传感系统在 HEK 293T 细胞中靶细胞器中 Mg 的比率检测中的应用,提供了对金属亚细胞池的首次直接比较,而不会干扰其他隔室的信号。通过荧光反应性偶联步骤原位激活荧光,有效地将荧光信号限制在感兴趣的位置,从而提高成像应用中的空间分辨率,并消除对错误定位传感器的冲洗需求。该标记策略与活细胞成像完全兼容,为跟踪金属分布的变化提供了有价值的工具,迄今为止,金属生物学中的这一变化一直是未解之谜。

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