A modular DNA scaffold to study protein–protein interactions at single-molecule resolution

被引:0
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作者
Dorota Kostrz
Hannah K. Wayment-Steele
Jing L. Wang
Maryne Follenfant
Vijay S. Pande
Terence R. Strick
Charlie Gosse
机构
[1] PSL Research University,Ecole Normale Supérieure, Institut de Biologie de l’Ecole Normale Supérieure (IBENS) CNRS, INSERM
[2] Laboratoire de Photonique et de Nanostructures,Department of Chemistry
[3] LPN-CNRS,Institut Jacques Monod, CNRS
[4] Stanford University,Department of Bioengineering
[5] Université Paris Diderot,undefined
[6] Université de Paris,undefined
[7] Stanford University,undefined
[8] Programme Equipe Labellisée,undefined
[9] Ligue Nationale Contre le Cancer,undefined
来源
Nature Nanotechnology | 2019年 / 14卷
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摘要
The residence time of a drug on its target has been suggested as a more pertinent metric of therapeutic efficacy than the traditionally used affinity constant. Here, we introduce junctured-DNA tweezers as a generic platform that enables real-time observation, at the single-molecule level, of biomolecular interactions. This tool corresponds to a double-strand DNA scaffold that can be nanomanipulated and on which proteins of interest can be engrafted thanks to widely used genetic tagging strategies. Thus, junctured-DNA tweezers allow a straightforward and robust access to single-molecule force spectroscopy in drug discovery, and more generally in biophysics. Proof-of-principle experiments are provided for the rapamycin-mediated association between FKBP12 and FRB, a system relevant in both medicine and chemical biology. Individual interactions were monitored under a range of applied forces and temperatures, yielding after analysis the characteristic features of the energy profile along the dissociation landscape.
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页码:988 / 993
页数:5
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