Single-molecule sorting of DNA helicases

Bain, Fletcher E; Wu, Colin G.; Spies, Maria

doi:10.1016/j.ymeth.2016.05.009

Cited by 19 publications

(27 citation statements)

References 33 publications

(31 reference statements)

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“…Our TIRF-FRET setup uses Cy3 as a donor fluorophore (excited by a 532 nm, DPSS Laser, Coherent Inc.) and Cy5 as an acceptor fluorophore. An evanescent wave generated by total internal reflection of the laser source, specifically illuminates molecules that are tethered to the surface of the observation flowcell (<100nm) (Axelrod, 2008, Bain et al, 2016). The scattered light is removed using a Cy3/Cy5 dual band-pass filter (Semrock, FF01-577/690) in the emission optical path.…”

Section: Observing Rad51 Nucleation On Ssdna Using Total Internal mentioning

confidence: 99%

“…Images are chromatically separated into Cy3 image (using a Chroma ET605/70m filter) and Cy5 image (using a Chroma ET700/75m filter) using a 630-nm dichroic mirror inside the dual-view system (DV2; Photometrics) (Figure 2A). An evanescent wave generated by total internal reflection of the laser source, specifically illuminates molecules that are tethered to the surface of the slide (<100nm) (Axelrod, 2008, Bain et al, 2016) (Figure 2B). …”

Section: Observing Rad51 Nucleation On Ssdna Using Total Internal mentioning

confidence: 99%

“…Before use, the tubes are equilibrated to room temperature for about 20 minutes in a dark chamber to prevent condensation onto the treated surface. The passivated and functionalized quartz slides and borosilicate glass coverslips are then assembled in the observation flowcells using double-sided tape and epoxy (detailed procedures for cleaning, passivating, functionalizing, and assembling the flowcells can be found in (Joo and Ha, 2012a, Bain et al, 2016)) and depicted later in (Figure 4). This procedure reduces the non-specific binding of proteins and nanoscopic impurities in buffers that might auto-fluoresce.…”

Section: Observing Rad51 Nucleation On Ssdna Using Total Internal mentioning

confidence: 99%

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Observation and Analysis of RAD51 Nucleation Dynamics at Single-Monomer Resolution

Subramanyam

Kinz-Thompson

Gonzalez

et al. 2018

Methods in Enzymology

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Human RAD51 promotes accurate DNA repair by homologous recombination and is involved in protection and repair of damaged DNA replication forks. The active species of RAD51 and related recombinases in all organisms is a nucleoprotein filament assembled on single-stranded DNA (ssDNA). The formation of a nucleoprotein filament competent for the recombination reaction, or for DNA replication support, is a delicate and strictly regulated process, which occurs through filament nucleation followed by filament extension. The rates of these two phases of filament formation define the capacity of RAD51 to compete with the ssDNA-binding protein RPA, as well as the lengths of the resulting filament segments. Single-molecule approaches can provide a wealth of quantitative information on the kinetics of RAD51 nucleoprotein filament assembly, internal dynamics, and disassembly. In this chapter, we describe how to setup a single-molecule total internal reflection fluorescence microscopy (TIRFM) experiment to monitor the initial steps of RAD51 nucleoprotein filament formation in real time and at single-monomer resolution. This approach is based on the unique, stretched-ssDNA conformation within the recombinase nucleoprotein filament and follows the efficiency of Förster resonance energy transfer (EFRET) between two DNA-conjugated fluorophores. We will discuss the practical aspects of the experimental setup, extraction of the FRET trajectories, and how to analyze and interpret the data to obtain information on RAD51 nucleation kinetics, the mechanism of nucleation, and the oligomeric species involved in filament formation.

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Section: Observing Rad51 Nucleation On Ssdna Using Total Internal mentioning

confidence: 99%

Section: Observing Rad51 Nucleation On Ssdna Using Total Internal mentioning

confidence: 99%

Section: Observing Rad51 Nucleation On Ssdna Using Total Internal mentioning

confidence: 99%

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Observation and Analysis of RAD51 Nucleation Dynamics at Single-Monomer Resolution

Subramanyam

Kinz-Thompson

Gonzalez

et al. 2018

Methods in Enzymology

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“…The construction of the system is described in detail in (Ghoneim and Spies, 2014, Bain et al, 2016). Briefly, this system was built on an Olympus IX-71 frame (Olympus America Inc).…”

Section: Observing Macromolecular Interactions Using Single-molecumentioning

confidence: 99%

“…For bacterially expressed proteins, BAP and the presence of 100 μM biotin in the growth media is sufficient for the efficient biotinylation of the target proteins. For proteins expressed in human, baculovirus or yeast cells, the expression system must also contain a vector for the expression of BirA ligase (see (Bain et al, 2016) for a protocol for the expression of biotinylated proteins in human cells, (Honda et al, 2014) for the baculovirus expression, and (Boehm et al, 2016) for the yeast expression).…”

Section: Observing Macromolecular Interactions Using Single-molecumentioning

confidence: 99%

Quantifying the Assembly of Multicomponent Molecular Machines by Single-Molecule Total Internal Reflection Fluorescence Microscopy

Boehm

Subramanyam

Ghoneim

et al. 2016

Methods in Enzymology

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Large, dynamic macromolecular complexes play essential roles in many cellular processes. Knowing how the components of these complexes associate with one another and undergo structural rearrangements is critical to understanding how they function. Single-molecule total internal reflection fluorescence (TIRF) microscopy is a powerful approach for addressing these fundamental issues. In this article, we first discuss single-molecule TIRF microscopes and strategies to immobilize and fluorescently label macromolecules. We then review the use of single-molecule TIRF microscopy to study the formation of binary macromolecular complexes using one-color imaging and inhibitors. We conclude with a discussion of the use of TIRF microscopy to examine the formation of higher-order (i.e., ternary, quaternary, etc.) complexes using multi-color setups. The focus throughout this article is on experimental design, controls, data acquisition, and data analysis. We hope that single-molecule TIRF microscopy, which has largely been the province of specialists, will soon become as common in the tool box of biophysicists and biochemists as structural approaches has become today.

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