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一种可去甲基化切换的适体设计能够对具有能量自给和结构整合特征的mA去甲基化酶FTO进行无滞后监测。

A Demethylation-Switchable Aptamer Design Enables Lag-Free Monitoring of mA Demethylase FTO with Energy Self-Sufficient and Structurally Integrated Features.

作者信息

Shi Yakun, Lei Yutian, Chen Meng, Ma Hansu, Shen Taorong, Zhang Yanfei, Huang Xing, Ling Wanxuan, Liu Si-Yang, Pan Yihang, Dai Zong, Xu Yuzhi

机构信息

Guangdong Provincial Key Laboratory of Sensing Technology and Biomedical Instrument, School of Biomedical Engineering, Shenzhen Campus of Sun Yat-Sen University, Sun Yat-Sen University, Shenzhen 518107, China.

Guangdong Provincial Key Laboratory of Digestive Cancer Research, Precision Medicine Center, The Seventh Affiliated Hospital, Sun Yat-Sen University, Shenzhen 518107, China.

出版信息

J Am Chem Soc. 2024 Dec 18;146(50):34638-34650. doi: 10.1021/jacs.4c12884. Epub 2024 Dec 4.

DOI:10.1021/jacs.4c12884
PMID:39628311
Abstract

Cellular context profiling of modification effector proteins is critical for an in-depth understanding of their biological roles in RNA -methyladenosine (mA) modification regulation and function. However, challenges still remain due to the high context complexities, which call for a versatile toolbox for accurate live-cell monitoring of effectors. Here, we propose a demethylation-switchable aptamer sensor engineered with a site-specific mA (DSA-mA) for lag-free monitoring of the mA demethylase FTO activity in living cells. As a proof of concept, a DNA aptamer against adenosine triphosphate (ATP) is selected to construct the DSA-mA model, as the "universal energy currency" role of ATP could guarantee the equally fast and spontaneous conformation change of DSA-mA sensor upon demethylation and ATP binding in living organisms, thus enabling sensitive monitoring of FTO activity with neither time delay nor recourse to extra supply of substances. This ATP-driven DSA-mA design facilitates biomedical research, including live-cell imaging, inhibitor screening, single-cell tracking of dynamic FTO nuclear translocation upon starvation stimuli, FTO characterization in a biomimetic heterotypic three-dimensional (3D) multicellular spheroid model, as well as the first report on the in vivo imaging of FTO activity. This strategy provides a simple yet versatile toolbox for clinical diagnosis, drug discovery, therapeutic evaluation, and biological study of RNA demethylation.

摘要

对修饰效应蛋白进行细胞背景分析,对于深入了解其在RNA甲基腺苷(mA)修饰调控和功能中的生物学作用至关重要。然而,由于背景复杂性高,挑战依然存在,这就需要一个多功能工具箱来对效应蛋白进行准确的活细胞监测。在此,我们提出一种用位点特异性mA设计的去甲基化可切换适配体传感器(DSA-mA),用于在活细胞中无延迟地监测mA去甲基化酶FTO的活性。作为概念验证,选择一种针对三磷酸腺苷(ATP)的DNA适配体来构建DSA-mA模型,因为ATP的“通用能量货币”作用能够保证DSA-mA传感器在活生物体中去甲基化和ATP结合后,其构象能以同样快速且自发的方式发生变化,从而能够对FTO活性进行灵敏监测,既无时间延迟,也无需额外供应物质。这种由ATP驱动的DSA-mA设计有助于生物医学研究,包括活细胞成像、抑制剂筛选、饥饿刺激下FTO核转位的单细胞动态追踪、在仿生异型三维(3D)多细胞球体模型中对FTO的表征,以及关于FTO活性体内成像的首次报道。该策略为RNA去甲基化的临床诊断、药物发现、治疗评估及生物学研究提供了一个简单而多功能的工具箱。

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