4.8 Article

Framework Nucleic Acid-Based Spatial-Confinement Amplifier for miRNA Imaging in Living Cells

Journal

ANALYTICAL CHEMISTRY
Volume 94, Issue 6, Pages 2934-2941

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/acs.analchem.1c04866

Keywords

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Funding

  1. Basic Science Center Project for National Natural Science Foundation of China [72088101]
  2. National Natural Science Foundation of China [21904141, 22078369, 21878339]
  3. Hunan Provincial Natural Science Foundation of China [2019JJ50791]
  4. Key Research and Development Program of Hunan Province [2020SK2128]
  5. Hunan Provincial Key Laboratory of Food Safety Monitoring and Early Warning [2020KFJJ06]

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In this study, a framework nucleic acid (FNA)-based nonenzymatic spatial-confinement amplifier was developed for rapid and reliable intracellular miRNA imaging. By encapsulating the localized catalytic hairpin assembly (L-CHA) reactor in the inner cavity of the FNA and utilizing the spatial-confinement effect, the reaction rate was accelerated and the dynamic performance was improved.
Real-time in situ monitoring of miRNAs in living cells is often appealed to signal amplifiers to tackle their low abundance challenges. However, the poor kinetics of amplifiers and potential interferences from the complex intracellular environment hamper its widespread applications in vivo. Herein, we report a framework nucleic acid (FNA)-based nonenzymatic spatial-confinement amplifier for rapid and reliable intracellular miRNA imaging. The amplifier consists of a localized catalytic hairpin assembly (L-CHA) reactor encapsulated in the inner cavity of an FNA (a 20 bp cube). The L-CHA reactor is certainly confined to the internal frame by integrating two probes (H1 and H2) of the L-CHA within a DNA strand and harnessing it to the opposite angles of the cube. We find that the stability of the amplifier is remarkably improved due to the protection of the FNA. More importantly, the spatial-confinement effect of the FNA can endow the confined L-CHA amplifier with enhanced local concentrations of reagents (5000-fold), thereby accelerating the reaction rate and improving the dynamic performance (up to 14.34-fold). With these advantages, the proposed amplifier can enable accurate and effective monitoring of miRNA expression levels in living cells and poses great potential in medical diagnostics and biomedical research.

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