Activating Two-Photon Silica Nanoamplifier-Based CHA and FRET for Accurate Ratiometric Bioimaging of Intracellular MicroRNA.

Anal Chem

Zhejiang Engineering Research Center of Advanced Mass Spectrometry and Clinical Application, Institute of Mass Spectrometry, School of Materials Science and Chemical Engineering, Ningbo University, Ningbo, Zhejiang 315211, China.

Published: October 2024

AI Article Synopsis

  • The visualization of microRNA (miRNA) in cancer cells is crucial for understanding disease progression, and two-photon (TP) imaging offers distinct advantages over traditional methods due to its high resolution and deep tissue penetration.
  • This study introduces a two-photon silica nanoamplifier (TP-SNA) that combines TP dye-doped silica nanoparticles with a signal amplification strategy, enabling highly sensitive detection of endogenous miRNAs in tumor cells at various depths.
  • The TP-SNA successfully detected miR-203 with a detection limit of 33 pM and achieved a tissue penetration depth of 210 μm, showing potential for clinical diagnosis applications.

Article Abstract

In situ visualization of microRNA (miRNA) in cancer cells and diseased tissues is essential for advancing our comprehension of the onset and progression of associated diseases. Two-photon (TP) imaging, as an imaging technology with high spatiotemporal resolution, deep tissue penetration, and accurate target quantification, has distinctive advantages over single-photon imaging and has attracted increasing attention. Extensive research has been conducted on two-photon dye-doped silica nanoparticles, which exhibit a large two-photon absorption (TPA) cross-section, high fluorescence quantum yield, and excellent biocompatibility. However, the low abundance of RNA in tumor cells leads to insufficient signal output. Based on functional nucleic acid, a catalyzed hairpin self-assembly (CHA) signal amplification strategy, which has simplicity, robustness, and nonenzymatic characteristics, can achieve the amplification of DNA or RNA signals. Here, a two-photon silica nanoamplifier (TP-SNA) utilizing TP dye-doped silica nanoparticles (SiNPs) and functional nucleic acid was constructed, employing triggering catalyzed hairpin self-assembly and fluorescence resonance energy transfer (FRET) for highly sensitive detection and precise TP imaging of endogenous miRNAs in tumor cells and tissues at varying depths. The TP-SNA demonstrated the capability to detect miR-203 with a detection limit of 33 pM. The maximum two-photon tissue penetration depth of the two-photon nanoamplifier was 210 μm. The two-photon nanoamplifier developed in this study makes full use of the advantages of accurate TP ratiometric bioimaging and the CHA signal amplification strategy, which shows good application value for future transformation into clinical diagnosis.

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http://dx.doi.org/10.1021/acs.analchem.4c03630DOI Listing

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Article Synopsis
  • The visualization of microRNA (miRNA) in cancer cells is crucial for understanding disease progression, and two-photon (TP) imaging offers distinct advantages over traditional methods due to its high resolution and deep tissue penetration.
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  • The TP-SNA successfully detected miR-203 with a detection limit of 33 pM and achieved a tissue penetration depth of 210 μm, showing potential for clinical diagnosis applications.
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