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用于病毒RNA体内成像的近红外荧光蛋白核酸模拟物的开发及开启式荧光

Development of Near-Infrared Nucleic Acid Mimics of Fluorescent Proteins for In Vivo Imaging of Viral RNA with Turn-On Fluorescence.

作者信息

Zhang Jiaheng, Li Huiyi, Lin Bin, Luo Xingyu, Yin Peng, Yi Ting, Xue Binbin, Zhang Xiao-Lian, Zhu Haizhen, Nie Zhou

机构信息

State Key Laboratory of Chemo/Biosensing and Chemometrics, College of Chemistry and Chemical Engineering, Hunan Provincial Key Laboratory of Biomacromolecular Chemical Biology, Hunan University, Changsha 410082, People's Republic of China.

Institute of Pathogen Biology and Immunology of College of Biology, State Key Laboratory of Chemo/Biosensing and Chemometrics, Hunan University, Changsha 410082, People's Republic of China.

出版信息

J Am Chem Soc. 2021 Nov 24;143(46):19317-19329. doi: 10.1021/jacs.1c04577. Epub 2021 Nov 11.

DOI:10.1021/jacs.1c04577
PMID:34762804
Abstract

GFP-like fluorescent proteins and their molecular mimics have revolutionized bioimaging research, but their emissions are largely limited in the visible to far-red region, hampering the in vivo applications in intact animals. Herein, we structurally modulate GFP-like chromophores using a donor-acceptor-acceptor (D-A-A') molecular configuration to discover a set of novel fluorogenic derivatives with infrared-shifted spectra. These chromophores can be fluorescently elicited by their specific interaction with G-quadruplex (G4), a unique noncanonical nucleic acid secondary structure, via inhibition of the chromophores' twisted-intramolecular charge transfer. This feature allows us to create, for the first time, FP mimics with tunable emission in the near-infrared (NIR) region (Em = 664-705 nm), namely, infrared G-quadruplex mimics of FPs (igMFP). Compared with their FP counterparts, igMFPs exhibit remarkably higher quantum yields, larger Stokes shift, and better photostability. In a proof-of-concept application using pathogen-related G4s as the target, we exploited igMFPs to directly visualize native hepatitis C virus (HCV) RNA genome in living cells via their in situ formation by the chromophore-bound viral G4 structure in the HCV core gene. Furthermore, igMFPs are capable of high contrast HCV RNA imaging in living mice bearing a HCV RNA-presenting mini-organ, providing the first application of FP mimics in whole-animal imaging.

摘要

绿色荧光蛋白(GFP)样荧光蛋白及其分子模拟物彻底改变了生物成像研究,但它们的发射光谱在很大程度上局限于可见光到远红光区域,这阻碍了其在完整动物体内的应用。在此,我们使用供体-受体-受体(D-A-A')分子构型对GFP样发色团进行结构调控,以发现一组具有红外光谱位移的新型荧光衍生物。这些发色团可以通过与G-四链体(G4)(一种独特的非经典核酸二级结构)的特异性相互作用而被荧光激发,通过抑制发色团的扭曲分子内电荷转移来实现。这一特性使我们首次创建了在近红外(NIR)区域(发射波长Em = 664 - 705 nm)具有可调发射的荧光蛋白模拟物,即荧光蛋白的红外G-四链体模拟物(igMFP)。与它们的荧光蛋白对应物相比,igMFP表现出显著更高的量子产率、更大的斯托克斯位移和更好的光稳定性。在一个以病原体相关G4为靶点的概念验证应用中,我们利用igMFP通过与HCV核心基因中发色团结合的病毒G4结构原位形成,直接在活细胞中可视化天然丙型肝炎病毒(HCV)RNA基因组。此外,igMFP能够在携带表达HCV RNA的微型器官的活体小鼠中进行高对比度的HCV RNA成像,这为荧光蛋白模拟物在全动物成像中的首次应用。

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