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Probing the Hydrogen-Bonding Environment of Individual Bases in DNA Duplexes with Isotope-Edited Infrared Spectroscopy

[Image: see text] Measuring the strength of the hydrogen bonds between DNA base pairs is of vital importance for understanding how our genetic code is physically accessed and recognized in cells, particularly during replication and transcription. Therefore, it is important to develop probes for thes...

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Autores principales: Fick, Robert J., Liu, Amy Y., Nussbaumer, Felix, Kreutz, Christoph, Rangadurai, Atul, Xu, Yu, Sommer, Roger D., Shi, Honglue, Scheiner, Steve, Stelling, Allison L.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: American Chemical Society 2021
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8311644/
https://www.ncbi.nlm.nih.gov/pubmed/34236202
http://dx.doi.org/10.1021/acs.jpcb.1c01351
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author Fick, Robert J.
Liu, Amy Y.
Nussbaumer, Felix
Kreutz, Christoph
Rangadurai, Atul
Xu, Yu
Sommer, Roger D.
Shi, Honglue
Scheiner, Steve
Stelling, Allison L.
author_facet Fick, Robert J.
Liu, Amy Y.
Nussbaumer, Felix
Kreutz, Christoph
Rangadurai, Atul
Xu, Yu
Sommer, Roger D.
Shi, Honglue
Scheiner, Steve
Stelling, Allison L.
author_sort Fick, Robert J.
collection PubMed
description [Image: see text] Measuring the strength of the hydrogen bonds between DNA base pairs is of vital importance for understanding how our genetic code is physically accessed and recognized in cells, particularly during replication and transcription. Therefore, it is important to develop probes for these key hydrogen bonds (H-bonds) that dictate events critical to cellular function, such as the localized melting of DNA. The vibrations of carbonyl bonds are well-known probes of their H-bonding environment, and their signals can be observed with infrared (IR) spectroscopy. Yet, pinpointing a single bond of interest in the complex IR spectrum of DNA is challenging due to the large number of carbonyl signals that overlap with each other. Here, we develop a method using isotope editing and infrared (IR) spectroscopy to isolate IR signals from the thymine (T) C2=O carbonyl. We use solvatochromatic studies to show that the TC2=O signal’s position in the IR spectrum is sensitive to the H-bonding capacity of the solvent. Our results indicate that C2=O of a single T base within DNA duplexes experiences weak H-bonding interactions. This finding is consistent with the existence of a third, noncanonical CH···O H-bond between adenine and thymine in both Watson–Crick and Hoogsteen base pairs in DNA.
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spelling pubmed-83116442021-07-27 Probing the Hydrogen-Bonding Environment of Individual Bases in DNA Duplexes with Isotope-Edited Infrared Spectroscopy Fick, Robert J. Liu, Amy Y. Nussbaumer, Felix Kreutz, Christoph Rangadurai, Atul Xu, Yu Sommer, Roger D. Shi, Honglue Scheiner, Steve Stelling, Allison L. J Phys Chem B [Image: see text] Measuring the strength of the hydrogen bonds between DNA base pairs is of vital importance for understanding how our genetic code is physically accessed and recognized in cells, particularly during replication and transcription. Therefore, it is important to develop probes for these key hydrogen bonds (H-bonds) that dictate events critical to cellular function, such as the localized melting of DNA. The vibrations of carbonyl bonds are well-known probes of their H-bonding environment, and their signals can be observed with infrared (IR) spectroscopy. Yet, pinpointing a single bond of interest in the complex IR spectrum of DNA is challenging due to the large number of carbonyl signals that overlap with each other. Here, we develop a method using isotope editing and infrared (IR) spectroscopy to isolate IR signals from the thymine (T) C2=O carbonyl. We use solvatochromatic studies to show that the TC2=O signal’s position in the IR spectrum is sensitive to the H-bonding capacity of the solvent. Our results indicate that C2=O of a single T base within DNA duplexes experiences weak H-bonding interactions. This finding is consistent with the existence of a third, noncanonical CH···O H-bond between adenine and thymine in both Watson–Crick and Hoogsteen base pairs in DNA. American Chemical Society 2021-07-08 2021-07-22 /pmc/articles/PMC8311644/ /pubmed/34236202 http://dx.doi.org/10.1021/acs.jpcb.1c01351 Text en © 2021 The Authors. Published by American Chemical Society Permits the broadest form of re-use including for commercial purposes, provided that author attribution and integrity are maintained (https://creativecommons.org/licenses/by/4.0/).
spellingShingle Fick, Robert J.
Liu, Amy Y.
Nussbaumer, Felix
Kreutz, Christoph
Rangadurai, Atul
Xu, Yu
Sommer, Roger D.
Shi, Honglue
Scheiner, Steve
Stelling, Allison L.
Probing the Hydrogen-Bonding Environment of Individual Bases in DNA Duplexes with Isotope-Edited Infrared Spectroscopy
title Probing the Hydrogen-Bonding Environment of Individual Bases in DNA Duplexes with Isotope-Edited Infrared Spectroscopy
title_full Probing the Hydrogen-Bonding Environment of Individual Bases in DNA Duplexes with Isotope-Edited Infrared Spectroscopy
title_fullStr Probing the Hydrogen-Bonding Environment of Individual Bases in DNA Duplexes with Isotope-Edited Infrared Spectroscopy
title_full_unstemmed Probing the Hydrogen-Bonding Environment of Individual Bases in DNA Duplexes with Isotope-Edited Infrared Spectroscopy
title_short Probing the Hydrogen-Bonding Environment of Individual Bases in DNA Duplexes with Isotope-Edited Infrared Spectroscopy
title_sort probing the hydrogen-bonding environment of individual bases in dna duplexes with isotope-edited infrared spectroscopy
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8311644/
https://www.ncbi.nlm.nih.gov/pubmed/34236202
http://dx.doi.org/10.1021/acs.jpcb.1c01351
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