An intramolecular catalytic hairpin assembly on a DNA tetrahedron for mRNA imaging in living cells: improving reaction kinetics and signal stability

Enzyme-free amplification techniques based on dynamic DNA self-assembly (DDSA) have recently been developed for the in situ detection of mRNA in living cells. However, signal generation in traditional DDSA amplifiers is mainly dependent on the random diffusion of dissociative probes in a bulk soluti...

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Detalles Bibliográficos
Autores principales: Qing, Zhihe, Hu, Jinlei, Xu, Jingyuan, Zou, Zhen, Lei, Yanli, Qing, Taiping, Yang, Ronghua
Formato: Online Artículo Texto
Lenguaje:English
Publicado: The Royal Society of Chemistry 2019
Materias:
Chemistry
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8148388/
https://www.ncbi.nlm.nih.gov/pubmed/34123293
http://dx.doi.org/10.1039/c9sc04916a
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author Qing, Zhihe
Hu, Jinlei
Xu, Jingyuan
Zou, Zhen
Lei, Yanli
Qing, Taiping
Yang, Ronghua
author_facet Qing, Zhihe
Hu, Jinlei
Xu, Jingyuan
Zou, Zhen
Lei, Yanli
Qing, Taiping
Yang, Ronghua
author_sort Qing, Zhihe
collection PubMed
description Enzyme-free amplification techniques based on dynamic DNA self-assembly (DDSA) have recently been developed for the in situ detection of mRNA in living cells. However, signal generation in traditional DDSA amplifiers is mainly dependent on the random diffusion of dissociative probes in a bulk solution, which is generally accompanied by poor kinetics and interference from complex biological systems. In this work, a new amplifier based on the design of an intramolecular catalytic hairpin assembly (intra-CHA) is proposed for the FRET imaging of mRNA in living cells. Compared with that in the free catalytic hairpin assembly (free-CHA), probes H1 and H2 in intra-CHA were simultaneously fixed on a DNA tetrahedron. The distance between them was closer, the local concentration of H1 and H2 in intra-CHA was theoretically approximately 808-times higher than that in free-CHA, and the initial reaction rate was enhanced 15.6 fold. Due to the spatial confinement effect, the reaction kinetics for target-catalyzed signal generation were significantly improved. By virtue of the three-dimensional nanostructure, H1 and H2 in the intra-CHA amplifier entered cells without any transfection or nanocarrier, and the probes and their products were free from biological interference, providing much higher signal stability for the reliable imaging of mRNA in living cells.
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spelling pubmed-81483882021-06-11 An intramolecular catalytic hairpin assembly on a DNA tetrahedron for mRNA imaging in living cells: improving reaction kinetics and signal stability Qing, Zhihe Hu, Jinlei Xu, Jingyuan Zou, Zhen Lei, Yanli Qing, Taiping Yang, Ronghua Chem Sci Chemistry Enzyme-free amplification techniques based on dynamic DNA self-assembly (DDSA) have recently been developed for the in situ detection of mRNA in living cells. However, signal generation in traditional DDSA amplifiers is mainly dependent on the random diffusion of dissociative probes in a bulk solution, which is generally accompanied by poor kinetics and interference from complex biological systems. In this work, a new amplifier based on the design of an intramolecular catalytic hairpin assembly (intra-CHA) is proposed for the FRET imaging of mRNA in living cells. Compared with that in the free catalytic hairpin assembly (free-CHA), probes H1 and H2 in intra-CHA were simultaneously fixed on a DNA tetrahedron. The distance between them was closer, the local concentration of H1 and H2 in intra-CHA was theoretically approximately 808-times higher than that in free-CHA, and the initial reaction rate was enhanced 15.6 fold. Due to the spatial confinement effect, the reaction kinetics for target-catalyzed signal generation were significantly improved. By virtue of the three-dimensional nanostructure, H1 and H2 in the intra-CHA amplifier entered cells without any transfection or nanocarrier, and the probes and their products were free from biological interference, providing much higher signal stability for the reliable imaging of mRNA in living cells. The Royal Society of Chemistry 2019-12-18 /pmc/articles/PMC8148388/ /pubmed/34123293 http://dx.doi.org/10.1039/c9sc04916a Text en This journal is © The Royal Society of Chemistry https://creativecommons.org/licenses/by-nc/3.0/
spellingShingle Chemistry
Qing, Zhihe
Hu, Jinlei
Xu, Jingyuan
Zou, Zhen
Lei, Yanli
Qing, Taiping
Yang, Ronghua
An intramolecular catalytic hairpin assembly on a DNA tetrahedron for mRNA imaging in living cells: improving reaction kinetics and signal stability
title An intramolecular catalytic hairpin assembly on a DNA tetrahedron for mRNA imaging in living cells: improving reaction kinetics and signal stability
title_full An intramolecular catalytic hairpin assembly on a DNA tetrahedron for mRNA imaging in living cells: improving reaction kinetics and signal stability
title_fullStr An intramolecular catalytic hairpin assembly on a DNA tetrahedron for mRNA imaging in living cells: improving reaction kinetics and signal stability
title_full_unstemmed An intramolecular catalytic hairpin assembly on a DNA tetrahedron for mRNA imaging in living cells: improving reaction kinetics and signal stability
title_short An intramolecular catalytic hairpin assembly on a DNA tetrahedron for mRNA imaging in living cells: improving reaction kinetics and signal stability
title_sort intramolecular catalytic hairpin assembly on a dna tetrahedron for mrna imaging in living cells: improving reaction kinetics and signal stability
topic Chemistry
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8148388/
https://www.ncbi.nlm.nih.gov/pubmed/34123293
http://dx.doi.org/10.1039/c9sc04916a
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