Smart Hairpins@MnO2 Nanosystem Enables Target-Triggered Enzyme-Free Exponential Amplification for Ultrasensitive Imaging of Intracellular MicroRNAs in Living Cells

Sensitive and specific imaging of microRNA (miRNA) in living cells is of great value for disease diagnosis and monitoring. Hybridization chain reaction (HCR) and DNAzyme-based methods have been considered as powerful tools for miRNA detection, with low efficient intracellular delivery and limited am...

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Veröffentlicht in:Analytical chemistry (Washington) 2022-06, Vol.94 (22), p.8014-8023
Hauptverfasser: Yang, Zizhong, Liu, Birong, Huang, Ting, Xie, Bao-Ping, Duan, Wen-Jun, Li, Min-Min, Chen, Jin-Xiang, Chen, Jun, Dai, Zong
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container_end_page 8023
container_issue 22
container_start_page 8014
container_title Analytical chemistry (Washington)
container_volume 94
creator Yang, Zizhong
Liu, Birong
Huang, Ting
Xie, Bao-Ping
Duan, Wen-Jun
Li, Min-Min
Chen, Jin-Xiang
Chen, Jun
Dai, Zong
description Sensitive and specific imaging of microRNA (miRNA) in living cells is of great value for disease diagnosis and monitoring. Hybridization chain reaction (HCR) and DNAzyme-based methods have been considered as powerful tools for miRNA detection, with low efficient intracellular delivery and limited amplification efficiency. Herein, we propose a Hairpins@MnO2 nanosystem for intracellular enzyme-free exponential amplification for miRNA imaging. The enzyme-free exponential amplification is based on the synergistic cross-activation between HCR and DNAzymes. The MnO2 nanosheets were employed as the carrier of three kinds of hairpin DNA probes and further provided appropriate Mn2+ as DNAzyme cofactors in the living cell. Upon entering cells and in the presence of highly expressed glutathione (GSH) in tumors, MnO2 is reduced to release Mn2+ and the three kinds of hairpin DNA probes. In the presence of target miRNA, the released hairpin DNA H1 and H2 probes self-assemble via HCR into the wire-shaped active Mn2+-based DNAzymes which further catalyze the cleavage of H3 to generate numerous new triggers to reversely stimulate HCR amplifiers, thus offering tremendously amplified Förster resonance energy transfer readout. The method has a detection limit of 33 fM, which is 2.4 × 104 times lower than that of the traditional HCR system. The developed method also has a high specificity; even miRNAs with a single base difference can be distinguished. Live cell imaging experiments confirmed that this Hairpins@MnO2 nanosystem allows accurate differentiation of miRNA expression of cancer cells and normal cells. The method holds great potential in biological research of nucleic acids.
doi_str_mv 10.1021/acs.analchem.2c01211
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Chem</addtitle><date>2022-06-07</date><risdate>2022</risdate><volume>94</volume><issue>22</issue><spage>8014</spage><epage>8023</epage><pages>8014-8023</pages><issn>0003-2700</issn><eissn>1520-6882</eissn><abstract>Sensitive and specific imaging of microRNA (miRNA) in living cells is of great value for disease diagnosis and monitoring. Hybridization chain reaction (HCR) and DNAzyme-based methods have been considered as powerful tools for miRNA detection, with low efficient intracellular delivery and limited amplification efficiency. Herein, we propose a Hairpins@MnO2 nanosystem for intracellular enzyme-free exponential amplification for miRNA imaging. The enzyme-free exponential amplification is based on the synergistic cross-activation between HCR and DNAzymes. The MnO2 nanosheets were employed as the carrier of three kinds of hairpin DNA probes and further provided appropriate Mn2+ as DNAzyme cofactors in the living cell. Upon entering cells and in the presence of highly expressed glutathione (GSH) in tumors, MnO2 is reduced to release Mn2+ and the three kinds of hairpin DNA probes. In the presence of target miRNA, the released hairpin DNA H1 and H2 probes self-assemble via HCR into the wire-shaped active Mn2+-based DNAzymes which further catalyze the cleavage of H3 to generate numerous new triggers to reversely stimulate HCR amplifiers, thus offering tremendously amplified Förster resonance energy transfer readout. The method has a detection limit of 33 fM, which is 2.4 × 104 times lower than that of the traditional HCR system. The developed method also has a high specificity; even miRNAs with a single base difference can be distinguished. Live cell imaging experiments confirmed that this Hairpins@MnO2 nanosystem allows accurate differentiation of miRNA expression of cancer cells and normal cells. The method holds great potential in biological research of nucleic acids.</abstract><cop>Washington</cop><pub>American Chemical Society</pub><doi>10.1021/acs.analchem.2c01211</doi><tpages>10</tpages><orcidid>https://orcid.org/0000-0002-9117-7447</orcidid><orcidid>https://orcid.org/0000-0002-3646-7396</orcidid></addata></record>
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source ACS Publications
subjects Amplification
Biological research
Cells (biology)
Chemistry
Cofactors
Deoxyribonucleic acid
DNA
DNA probes
Energy transfer
Enzymes
Glutathione
Hybridization
Intracellular
Manganese dioxide
Medical imaging
MicroRNAs
miRNA
Nucleic acids
Probes
Ribonucleic acid
RNA
Tumors
title Smart Hairpins@MnO2 Nanosystem Enables Target-Triggered Enzyme-Free Exponential Amplification for Ultrasensitive Imaging of Intracellular MicroRNAs in Living Cells
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