Visualization of RecA Filaments and DNA by Fluorescence Microscopy

Nishinaka, Taro; Doi, Yuko; Hashimoto, Makiko; Hara, Reiko; Shibata, Takehiko; Harada, Yoshie; Kinosita, Kazuhiko; Noji, Hiroyuki; Yashima, Eiji

doi:10.1093/jb/mvm033

Cited by 9 publications

(7 citation statements)

References 39 publications

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“…Insights into the transition between the two conformations, and the roles of ATP hydrolysis and DNA tension in controlling this transition have recently been provided by single-molecule studies on Rad5144–46 and RecA 47. Crystallographic analyses of RecA filaments have also revealed how ATP binding at the protomer-protomer interface stabilizes the extended filament in the presence of ssDNA 9.…”

Section: Discussionmentioning

confidence: 99%

Crystal Structure of the Phage T4 Recombinase UvsX and Its Functional Interaction with the T4 SF2 Helicase UvsW

Gajewski

Webb

Galkin

et al. 2011

Journal of Molecular Biology

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Summary Bacteriophage T4 provides an important model system for studying the mechanism of homologous recombination. We have determined the crystal structure of the T4 UvsX recombinase, and the overall architecture and fold closely resembles that of RecA, including a highly conserved ATP binding site. Based on this new structure, we reanalyzed EM reconstructions of UvsX-DNA filaments and docked the UvsX crystal structure into two different filament forms, a compressed filament generated in the presence of ADP and an elongated filament generated in the presence of ATP and aluminum fluoride. In these reconstructions, the ATP binding site sits at the protomer interface, as in the RecA filament crystal structure. However, the environment of the ATP binding site is altered in the two filament reconstructions, suggesting that nucleotide cannot be as easily accommodated at the protomer interface of the compressed filament. Finally, we show that the phage helicase UvsW completes the UvsX-promoted strand-exchange reaction, allowing the generation of simple nicked circular product rather than complex networks of partially exchanged substrates.

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Section: Discussionmentioning

confidence: 99%

Crystal Structure of the Phage T4 Recombinase UvsX and Its Functional Interaction with the T4 SF2 Helicase UvsW

Gajewski

Webb

Galkin

et al. 2011

Journal of Molecular Biology

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“…In fact, the purified protein expressed activity equivalent to that of the wildtype. 30 To fix the RecA filament on a glass plate, M13mp18 circular ssDNA (7249 bases) was linearized by restriction enzyme, and a biotin molecule was attached at the 3′ terminus of the linear ssDNA via a PEG linker. A 4 μl (3 mm × 18 mm × 0.08 mm) solution exchange chamber was prepared by superposing two cover glasses, and streptavidin, which has four binding sites for biotin, was then immobilized on the glass surface via biotinylated bovine serum albumin (BSA).…”

Section: Contraction Of Reca Filamentsmentioning

confidence: 99%

“…We showed earlier that the major biochemical activities of RecA protein, ATPase and strand exchange activities, were not compromised by the labelling procedure. 30 The fluorescently labelled RecA filament was infused into the flow chamber, and allowed to become immobilized on the glass plate through the biotin-streptavidin binding (Figure 1(b)). Unbound RecA filaments were washed out with solution buffer containing 1 mM dATP and 0.53 μM wildtype RecA.…”

Section: Contraction Of Reca Filamentsmentioning

confidence: 99%

“…The prepared DNA substrate was referred to as M13-linker-biotin ssDNA. The 353C RecA derivative, where one cysteine residue was introduced to the C terminus of a wild-type RecA protein, was prepared and purified as described, 30 and further purified by anion-exchange column chromatography (UNOsphere Q, Bio-Rad). The wild-type RecA protein was purified as described above or was purchased from New England Biolabs (Ipswich, MA, USA).…”

Section: Substratesmentioning

confidence: 99%

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Elastic Behavior of RecA-DNA Helical Filaments

Nishinaka

Doi

Hara

et al. 2007

Journal of Molecular Biology

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“…The tube diameter was determined and was shown to decrease with increasing concentration. Further studies on actin filaments and DNA chains have been published in more recent years [21][22][23][24][25][26] . Also a study on the motion of synthetic single-walled carbon nano tubes in a gel, aimed at understanding the effect of flexibility on the diffusion of stiff filaments under confinement, has appeared 27 .…”

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confidence: 99%

Nanoscale Study of Polymer Dynamics

Keshavarz

Engelkamp

et al. 2015

ACS Nano

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The thermal motion of polymer chains in a crowded environment is anisotropic and highly confined. Whereas theoretical and experimental progress has been made, typically only indirect evidence of polymer dynamics is obtained either from scattering or mechanical response. Toward a complete understanding of the complicated polymer dynamics in crowded media such as biological cells, it is of great importance to unravel the role of heterogeneity and molecular individualism. In the present work, we investigate the dynamics of synthetic polymers and the tube-like motion of individual chains using time-resolved fluorescence microscopy. A single fluorescently labeled polymer molecule is observed in a sea of unlabeled polymers, giving access to not only the dynamics of the probe chain itself but also to that of the surrounding network. We demonstrate that it is possible to extract the characteristic time constants and length scales in one experiment, providing a detailed understanding of polymer dynamics at the single chain level. The quantitative agreement with bulk rheology measurements is promising for using local probes to study heterogeneity in complex, crowded systems.

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Visualization of RecA Filaments and DNA by Fluorescence Microscopy

Cited by 9 publications

References 39 publications

Crystal Structure of the Phage T4 Recombinase UvsX and Its Functional Interaction with the T4 SF2 Helicase UvsW

Crystal Structure of the Phage T4 Recombinase UvsX and Its Functional Interaction with the T4 SF2 Helicase UvsW

Elastic Behavior of RecA-DNA Helical Filaments

Nanoscale Study of Polymer Dynamics

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