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本文引用的文献

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Structure and functional reselection of the Mango-III fluorogenic RNA aptamer.芒果-III 荧光 RNA 适体的结构与功能重选。
Nat Chem Biol. 2019 May;15(5):472-479. doi: 10.1038/s41589-019-0267-9. Epub 2019 Apr 15.
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Spectral Tuning by a Single Nucleotide Controls the Fluorescence Properties of a Fluorogenic Aptamer.单核苷酸介导的光谱调谐控制荧光适体的荧光特性。
Biochemistry. 2019 Mar 26;58(12):1560-1564. doi: 10.1021/acs.biochem.9b00048. Epub 2019 Mar 11.
3
Broccoli Fluorets: Split Aptamers as a User-Friendly Fluorescent Toolkit for Dynamic RNA Nanotechnology.西兰花小花:分裂适体作为动态 RNA 纳米技术的用户友好型荧光工具包。
Molecules. 2018 Dec 2;23(12):3178. doi: 10.3390/molecules23123178.
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A Multicolor Large Stokes Shift Fluorogen-Activating RNA Aptamer with Cationic Chromophores.一种具有阳离子生色团的多色大斯托克斯位移荧光素激活 RNA 适体。
Chemistry. 2019 Feb 6;25(8):1931-1935. doi: 10.1002/chem.201805882. Epub 2019 Jan 11.
5
Structural basis for activation of fluorogenic dyes by an RNA aptamer lacking a G-quadruplex motif.缺乏 G-四链体结构的 RNA 适体激活荧光染料的结构基础。
Nat Commun. 2018 Oct 31;9(1):4542. doi: 10.1038/s41467-018-06942-3.
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De novo design of a fluorescence-activating β-barrel.从头设计一个荧光激活的β桶。
Nature. 2018 Sep;561(7724):485-491. doi: 10.1038/s41586-018-0509-0. Epub 2018 Sep 12.
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A multicolor riboswitch-based platform for imaging of RNA in live mammalian cells.基于多色核糖开关的活哺乳动物细胞内 RNA 成像平台。
Nat Chem Biol. 2018 Oct;14(10):964-971. doi: 10.1038/s41589-018-0103-7. Epub 2018 Jul 30.
8
Crystal Structures of the Mango-II RNA Aptamer Reveal Heterogeneous Fluorophore Binding and Guide Engineering of Variants with Improved Selectivity and Brightness.芒果-II RNA适配体的晶体结构揭示了异质荧光团结合,并指导了具有更高选择性和亮度的变体工程。
Biochemistry. 2018 Jul 3;57(26):3544-3548. doi: 10.1021/acs.biochem.8b00399. Epub 2018 May 24.
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Fluorogenic RNA Mango aptamers for imaging small non-coding RNAs in mammalian cells.用于在哺乳动物细胞中成像小非编码RNA的荧光RNA芒果适配体。
Nat Commun. 2018 Feb 13;9(1):656. doi: 10.1038/s41467-018-02993-8.
10
Development of a genetically encodable FRET system using fluorescent RNA aptamers.利用荧光RNA适配体开发一种基因编码的荧光共振能量转移(FRET)系统。
Nat Commun. 2018 Jan 2;9(1):18. doi: 10.1038/s41467-017-02435-x.

从荧光蛋白到荧光 RNA:用于细胞大分子成像的工具。

From fluorescent proteins to fluorogenic RNAs: Tools for imaging cellular macromolecules.

机构信息

Biochemistry and Biophysics Center, National Heart, Lung, and Blood Institute, Bethesda, Maryland, 20892-8012.

出版信息

Protein Sci. 2019 Aug;28(8):1374-1386. doi: 10.1002/pro.3632. Epub 2019 May 11.

DOI:10.1002/pro.3632
PMID:31017335
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6635776/
Abstract

The explosion in genome-wide sequencing has revealed that noncoding RNAs are ubiquitous and highly conserved in biology. New molecular tools are needed for their study in live cells. Fluorescent RNA-small molecule complexes have emerged as powerful counterparts to fluorescent proteins, which are well established, universal tools in the study of proteins in cell biology. No naturally fluorescent RNAs are known; all current fluorescent RNA tags are in vitro evolved or engineered molecules that bind a conditionally fluorescent small molecule and turn on its fluorescence by up to 5000-fold. Structural analyses of several such fluorescence turn-on aptamers show that these compact (30-100 nucleotides) RNAs have diverse molecular architectures that can restrain their photoexcited fluorophores in their maximally fluorescent states, typically by stacking between planar nucleotide arrangements, such as G-quadruplexes, base triples, or base pairs. The diversity of fluorogenic RNAs as well as fluorophores that are cell permeable and bind weakly to endogenous cellular macromolecules has already produced RNA-fluorophore complexes that span the visual spectrum and are useful for tagging and visualizing RNAs in cells. Because the ligand binding sites of fluorogenic RNAs are not constrained by the need to autocatalytically generate fluorophores as are fluorescent proteins, they may offer more flexibility in molecular engineering to generate photophysical properties that are tailored to experimental needs.

摘要

基因组测序的爆炸式增长揭示了非编码 RNA 在生物学中无处不在且高度保守。需要新的分子工具来研究活细胞中的非编码 RNA。荧光 RNA-小分子复合物已成为荧光蛋白的有力替代品,荧光蛋白是细胞生物学中研究蛋白质的成熟且通用的工具。目前还没有天然荧光 RNA;所有当前的荧光 RNA 标签都是体外进化或工程分子,它们与条件性荧光小分子结合,并将其荧光强度提高多达 5000 倍。对几种这种荧光开启适体的结构分析表明,这些紧凑的(30-100 个核苷酸)RNA 具有多种分子结构,可以将其光激发荧光团限制在其最大荧光状态,通常通过堆叠在平面核苷酸排列之间来实现,例如 G-四链体、碱基三链体或碱基对。荧光 RNA 和可穿透细胞并与内源性细胞大分子弱结合的荧光团的多样性已经产生了跨越可见光谱的 RNA-荧光团复合物,可用于标记和可视化细胞中的 RNA。由于荧光 RNA 的配体结合位点不受需要自动催化产生荧光团的限制,因此与荧光蛋白相比,它们在分子工程中可能具有更大的灵活性,以产生针对实验需求定制的光物理性质。