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Chemical Annealing Restructures RNA for Nanopore Detection.

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Peer-reviewed

Repository URI

https://www.repository.cam.ac.uk/handle/1810/368468

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Primary Published version (3.65 MB)
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Other

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Authors

Platnich, Casey M  ORCID logo  https://orcid.org/0000-0002-3634-4580

Abstract

RNA is a key biochemical marker, yet its chemical instability and complex secondary structure hamper its integration into DNA nanotechnology-based sensing platforms. Relying on the denaturation of the native RNA structure using urea, we show that restructured DNA/RNA hybrids can readily be prepared at room temperature. Using solid-state nanopore sensing, we demonstrate that the structures of our DNA/RNA hybrids conform to the design at the single-molecule level. Employing this chemical annealing procedure, we mitigate RNA self-cleavage, enabling the direct detection of restructured RNA molecules for biosensing applications.

Description

Publication status: Published

Keywords

RNA, Nanopores, DNA, Biosensing Techniques, Nucleic Acid Conformation, Nucleic Acid Hybridization, Nanotechnology, Urea

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Publisher

American Chemical Society (ACS)

Publisher DOI

https://doi.org/10.1021/jacs.4c03753

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Attribution 4.0 International
Except where otherwised noted, this item's license is described as Attribution 4.0 International
Sponsorship
European Commission Horizon 2020 (H2020) Future and Emerging Technologies (FET) (964995)
Herchel Smith Fellowship, European Union under the Horizon 2020 Program, FET- Open: DNA-FAIRYLIGHTS, Grant Agreement No. 964995, UK Research and Innovation (UKRI) under the UK government’s Horizon Europe funding guarantee EP/X023311/1.

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