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Oriented Soft DNA Curtains for Single-Molecule Imaging

[Image: see text] Over the past 20 years, single-molecule methods have become extremely important for biophysical studies. These methods, in combination with new nanotechnological platforms, can significantly facilitate experimental design and enable faster data acquisition. A nanotechnological plat...

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Autores principales: Kopu̅stas, Aurimas, Ivanovaitė, Šaru̅nė, Rakickas, Tomas, Pocevičiu̅tė, Ernesta, Paksaitė, Justė, Karvelis, Tautvydas, Zaremba, Mindaugas, Manakova, Elena, Tutkus, Marijonas
Formato: Online Artículo Texto
Lenguaje:English
Publicado: American Chemical Society 2021
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8280724/
https://www.ncbi.nlm.nih.gov/pubmed/33689355
http://dx.doi.org/10.1021/acs.langmuir.1c00066
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author Kopu̅stas, Aurimas
Ivanovaitė, Šaru̅nė
Rakickas, Tomas
Pocevičiu̅tė, Ernesta
Paksaitė, Justė
Karvelis, Tautvydas
Zaremba, Mindaugas
Manakova, Elena
Tutkus, Marijonas
author_facet Kopu̅stas, Aurimas
Ivanovaitė, Šaru̅nė
Rakickas, Tomas
Pocevičiu̅tė, Ernesta
Paksaitė, Justė
Karvelis, Tautvydas
Zaremba, Mindaugas
Manakova, Elena
Tutkus, Marijonas
author_sort Kopu̅stas, Aurimas
collection PubMed
description [Image: see text] Over the past 20 years, single-molecule methods have become extremely important for biophysical studies. These methods, in combination with new nanotechnological platforms, can significantly facilitate experimental design and enable faster data acquisition. A nanotechnological platform, which utilizes a flow-stretch of immobilized DNA molecules, called DNA Curtains, is one of the best examples of such combinations. Here, we employed new strategies to fabricate a flow-stretch assay of stably immobilized and oriented DNA molecules using a protein template-directed assembly. In our assay, a protein template patterned on a glass coverslip served for directional assembly of biotinylated DNA molecules. In these arrays, DNA molecules were oriented to one another and maintained extended by either single- or both-end immobilization to the protein templates. For oriented both-end DNA immobilization, we employed heterologous DNA labeling and protein template coverage with the antidigoxigenin antibody. In contrast to single-end immobilization, both-end immobilization does not require constant buffer flow for keeping DNAs in an extended configuration, allowing us to study protein–DNA interactions at more controllable reaction conditions. Additionally, we increased the immobilization stability of the biotinylated DNA molecules using protein templates fabricated from traptavidin. Finally, we demonstrated that double-tethered Soft DNA Curtains can be used in nucleic acid-interacting protein (e.g., CRISPR-Cas9) binding assay that monitors the binding location and position of individual fluorescently labeled proteins on DNA.
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spelling pubmed-82807242021-07-16 Oriented Soft DNA Curtains for Single-Molecule Imaging Kopu̅stas, Aurimas Ivanovaitė, Šaru̅nė Rakickas, Tomas Pocevičiu̅tė, Ernesta Paksaitė, Justė Karvelis, Tautvydas Zaremba, Mindaugas Manakova, Elena Tutkus, Marijonas Langmuir [Image: see text] Over the past 20 years, single-molecule methods have become extremely important for biophysical studies. These methods, in combination with new nanotechnological platforms, can significantly facilitate experimental design and enable faster data acquisition. A nanotechnological platform, which utilizes a flow-stretch of immobilized DNA molecules, called DNA Curtains, is one of the best examples of such combinations. Here, we employed new strategies to fabricate a flow-stretch assay of stably immobilized and oriented DNA molecules using a protein template-directed assembly. In our assay, a protein template patterned on a glass coverslip served for directional assembly of biotinylated DNA molecules. In these arrays, DNA molecules were oriented to one another and maintained extended by either single- or both-end immobilization to the protein templates. For oriented both-end DNA immobilization, we employed heterologous DNA labeling and protein template coverage with the antidigoxigenin antibody. In contrast to single-end immobilization, both-end immobilization does not require constant buffer flow for keeping DNAs in an extended configuration, allowing us to study protein–DNA interactions at more controllable reaction conditions. Additionally, we increased the immobilization stability of the biotinylated DNA molecules using protein templates fabricated from traptavidin. Finally, we demonstrated that double-tethered Soft DNA Curtains can be used in nucleic acid-interacting protein (e.g., CRISPR-Cas9) binding assay that monitors the binding location and position of individual fluorescently labeled proteins on DNA. American Chemical Society 2021-03-09 2021-03-23 /pmc/articles/PMC8280724/ /pubmed/33689355 http://dx.doi.org/10.1021/acs.langmuir.1c00066 Text en © 2021 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 Kopu̅stas, Aurimas
Ivanovaitė, Šaru̅nė
Rakickas, Tomas
Pocevičiu̅tė, Ernesta
Paksaitė, Justė
Karvelis, Tautvydas
Zaremba, Mindaugas
Manakova, Elena
Tutkus, Marijonas
Oriented Soft DNA Curtains for Single-Molecule Imaging
title Oriented Soft DNA Curtains for Single-Molecule Imaging
title_full Oriented Soft DNA Curtains for Single-Molecule Imaging
title_fullStr Oriented Soft DNA Curtains for Single-Molecule Imaging
title_full_unstemmed Oriented Soft DNA Curtains for Single-Molecule Imaging
title_short Oriented Soft DNA Curtains for Single-Molecule Imaging
title_sort oriented soft dna curtains for single-molecule imaging
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC8280724/
https://www.ncbi.nlm.nih.gov/pubmed/33689355
http://dx.doi.org/10.1021/acs.langmuir.1c00066
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