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Double-stemmed and split structural variants of fluorescent RNA Mango aptamers

Aptamers with fluorogenic ligands are emerging as useful tools to quantify and track RNA molecules. The RNA Mango family of aptamers have a useful combination of tight ligand binding, bright fluorescence, and small size. However, the simple structure of these aptamers, with a single base-paired stem...

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Autores principales: Herrera-Gutierrez, Jeremy, Burden, Steven J., Kobernat, Sarah E., Shults, Nicholas H., Smith, Mark, Fologea, Daniel, Hayden, Eric J.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Cold Spring Harbor Laboratory Press 2023
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10573287/
https://www.ncbi.nlm.nih.gov/pubmed/37268327
http://dx.doi.org/10.1261/rna.079651.123
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author Herrera-Gutierrez, Jeremy
Burden, Steven J.
Kobernat, Sarah E.
Shults, Nicholas H.
Smith, Mark
Fologea, Daniel
Hayden, Eric J.
author_facet Herrera-Gutierrez, Jeremy
Burden, Steven J.
Kobernat, Sarah E.
Shults, Nicholas H.
Smith, Mark
Fologea, Daniel
Hayden, Eric J.
author_sort Herrera-Gutierrez, Jeremy
collection PubMed
description Aptamers with fluorogenic ligands are emerging as useful tools to quantify and track RNA molecules. The RNA Mango family of aptamers have a useful combination of tight ligand binding, bright fluorescence, and small size. However, the simple structure of these aptamers, with a single base-paired stem capped by a G-quadruplex, can limit the sequence and structural modifications needed for many use-inspired designs. Here we report new structural variants of RNA Mango that have two base-paired stems attached to the quadruplex. Fluorescence saturation analysis of one of the double-stemmed constructs showed a maximum fluorescence that is ∼75% brighter than the original single-stemmed Mango I. A small number of mutations to nucleotides in the tetraloop-like linker of the second stem were subsequently analyzed. The effect of these mutations on the affinity and fluorescence suggested that the nucleobases of the second linker do not directly interact with the fluorogenic ligand (TO1-biotin), but may instead induce higher fluorescence by indirectly altering the ligand properties in the bound state. The effects of the mutations in this second tetraloop-like linker indicate the potential of this second stem for rational design and reselection experiments. Additionally, we demonstrated that a bimolecular mango designed by splitting the double-stemmed Mango can function when two RNA molecules are cotranscribed from different DNA templates in a single in vitro transcription. This bimolecular Mango has potential application in detecting RNA–RNA interactions. Together, these constructs expand the designability of the Mango aptamers to facilitate future applications of RNA imaging.
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spelling pubmed-105732872023-10-14 Double-stemmed and split structural variants of fluorescent RNA Mango aptamers Herrera-Gutierrez, Jeremy Burden, Steven J. Kobernat, Sarah E. Shults, Nicholas H. Smith, Mark Fologea, Daniel Hayden, Eric J. RNA Articles Aptamers with fluorogenic ligands are emerging as useful tools to quantify and track RNA molecules. The RNA Mango family of aptamers have a useful combination of tight ligand binding, bright fluorescence, and small size. However, the simple structure of these aptamers, with a single base-paired stem capped by a G-quadruplex, can limit the sequence and structural modifications needed for many use-inspired designs. Here we report new structural variants of RNA Mango that have two base-paired stems attached to the quadruplex. Fluorescence saturation analysis of one of the double-stemmed constructs showed a maximum fluorescence that is ∼75% brighter than the original single-stemmed Mango I. A small number of mutations to nucleotides in the tetraloop-like linker of the second stem were subsequently analyzed. The effect of these mutations on the affinity and fluorescence suggested that the nucleobases of the second linker do not directly interact with the fluorogenic ligand (TO1-biotin), but may instead induce higher fluorescence by indirectly altering the ligand properties in the bound state. The effects of the mutations in this second tetraloop-like linker indicate the potential of this second stem for rational design and reselection experiments. Additionally, we demonstrated that a bimolecular mango designed by splitting the double-stemmed Mango can function when two RNA molecules are cotranscribed from different DNA templates in a single in vitro transcription. This bimolecular Mango has potential application in detecting RNA–RNA interactions. Together, these constructs expand the designability of the Mango aptamers to facilitate future applications of RNA imaging. Cold Spring Harbor Laboratory Press 2023-09 /pmc/articles/PMC10573287/ /pubmed/37268327 http://dx.doi.org/10.1261/rna.079651.123 Text en © 2023 Herrera-Gutierrez et al.; Published by Cold Spring Harbor Laboratory Press for the RNA Society https://creativecommons.org/licenses/by/4.0/This article, published in RNA, is available under a Creative Commons License (Attribution 4.0 International), as described at http://creativecommons.org/licenses/by/4.0/ (https://creativecommons.org/licenses/by/4.0/) .
spellingShingle Articles
Herrera-Gutierrez, Jeremy
Burden, Steven J.
Kobernat, Sarah E.
Shults, Nicholas H.
Smith, Mark
Fologea, Daniel
Hayden, Eric J.
Double-stemmed and split structural variants of fluorescent RNA Mango aptamers
title Double-stemmed and split structural variants of fluorescent RNA Mango aptamers
title_full Double-stemmed and split structural variants of fluorescent RNA Mango aptamers
title_fullStr Double-stemmed and split structural variants of fluorescent RNA Mango aptamers
title_full_unstemmed Double-stemmed and split structural variants of fluorescent RNA Mango aptamers
title_short Double-stemmed and split structural variants of fluorescent RNA Mango aptamers
title_sort double-stemmed and split structural variants of fluorescent rna mango aptamers
topic Articles
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10573287/
https://www.ncbi.nlm.nih.gov/pubmed/37268327
http://dx.doi.org/10.1261/rna.079651.123
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