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Single Molecule Analysis

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Cover of 'Single Molecule Analysis'

Table of Contents

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    Book Overview
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    Chapter 1 Introduction to Optical Tweezers: Background, System Designs, and Applications
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    Chapter 2 Quantifying ATP-Independent Nucleosome Chaperone Activity with Single-Molecule Methods
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    Chapter 3 Protein Tethering for Single-Molecule Force Spectroscopy
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    Chapter 4 Insect Cell-Based Expression of Cytoskeletal Motor Proteins for Single-Molecule Studies
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    Chapter 5 Probing Mitotic Chromosome Mechanics Using Optical Tweezers
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    Chapter 6 A Brief Introduction to Single-Molecule Fluorescence Methods
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    Chapter 7 Single-Molecule Fluorescence Microscopy in Sensory Cilia of Living Caenorhabditis elegans
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    Chapter 8 Lattice Light-Sheet Motor-PAINT: A Method to Map the Orientations of Microtubules in Complex Three-Dimensional Arrays
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    Chapter 9 Fluorescence Microscopy of Nanochannel-Confined DNA
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    Chapter 10 Single-Molecule FRET X
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    Chapter 11 Single-Molecule Fluorescence Imaging of DNA Replication Stalling at Sites of Nucleoprotein Complexes
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    Chapter 12 Measuring Transcription Dynamics of Individual Genes Inside Living Cells
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    Chapter 13 Single-Molecule FRET-Resolved Protein Dynamics – from Plasmid to Data in Six Steps
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    Chapter 14 Atomic Force Microscopy: An Introduction
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    Chapter 15 Atomic Force Microscopy of Viruses: Stability, Disassembly, and Genome Release
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    Chapter 16 Unfolding and Refolding Proteins Using Single-Molecule AFM
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    Chapter 17 Visualizing Molecular Dynamics by High-Speed Atomic Force Microscopy
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    Chapter 18 An Introduction to Magnetic Tweezers
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    Chapter 19 Surface Functionalization, Nucleic Acid Tether Characterization, and Force Calibration for a Magnetic Tweezers Assay
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    Chapter 20 Correlated Single-Molecule Magnetic Tweezers and Fluorescence Measurements of DNA-Enzyme Interactions
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    Chapter 21 Detecting DNA Loops Using Tethered Particle Motion
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    Chapter 22 Single-Cell Measurements Using Acoustic Force Spectroscopy (AFS)
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    Chapter 23 DNA Origami-Based Single-Molecule Force Spectroscopy and Applications
Attention for Chapter 23: DNA Origami-Based Single-Molecule Force Spectroscopy and Applications
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Chapter title
DNA Origami-Based Single-Molecule Force Spectroscopy and Applications
Chapter number 23
Book title
Single Molecule Analysis
Published by
Humana, New York, NY, October 2023
DOI 10.1007/978-1-0716-3377-9_23
Pubmed ID
Book ISBNs
978-1-07-163376-2, 978-1-07-163377-9
Authors

Kevin Kramm, Tim Schröder, Andrés Manuel Vera, Lennart Grabenhorst, Philip Tinnefeld, Dina Grohmann

Abstract

Over the last years, single-molecule force spectroscopy provided insights into the intricate connection between mechanical stimuli and biochemical signaling. The underlying molecular mechanisms were uncovered and explored using techniques such as atomic force microscopy and force spectroscopy using optical or magnetic tweezers. These experimental approaches are limited by thermal noise resulting from a physical connection of the studied biological system to the macroscopic world. To overcome this limitation, we recently introduced the DNA origami force clamp (FC) which is a freely diffusing nanodevice that generates piconewton forces on a DNA sequence of interest. Binding of a protein to the DNA under tension can be detected employing fluorescence resonance energy transfer (FRET) as a sensitive readout.This protocol introduces the reader to the working principles of the FC and provides instructions to design and generate a DNA origami FC customized for a protein of interest. Molecular cloning techniques are employed to modify, produce, and purify a custom DNA scaffold. A fluorescently labeled DNA suitable to detect protein binding via FRET is generated via enzymatic ligation of commercial DNA oligonucleotides. After thermal annealing of all components, the DNA origami FC is purified using agarose gel electrophoresis. The final section covers the interrogation of the FC using confocal single-molecule FRET measurements and subsequent data analysis to quantify the binding of a DNA-binding protein to its cognate recognition site under a range of forces. Using this approach, force-dependent DNA-protein interactions can be studied on the single-molecule level on thousands of molecules in a parallelized fashion.

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Readers by professional status Count As %
Student > Ph. D. Student 1 100%
Student > Bachelor 1 100%
Readers by discipline Count As %
Agricultural and Biological Sciences 1 100%
Chemistry 1 100%