Structural and Biophysical Characterization of Murine Rif1 C Terminus Reveals High Specificity for DNA Cruciform Structures

Sukackaitė, Rasa; Jensen, Malene Ringkjøbing; Mas, Philippe J.; Blackledge, Martin; Buonomo, Sara B.C.; Hart, Darren J.

doi:10.1074/jbc.m114.557843

Cited by 33 publications

(35 citation statements)

References 41 publications

(35 reference statements)

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“…6b, lane 5). The DNAbinding domain of mammalian Rif1 has been reported to bind to structured DNAs including forked DNA, flap DNA and cruciform structures 31,32 . Therefore, we prepared various structured DNAs and used them in competition assays with the G 24 DNA, which is known to form a parallel-type G-quadruplex structure 33 .…”

Section: Purified Rif Protein Binds To G-quadruplex Structuresmentioning

confidence: 99%

“…Duplex DNA, Y-fork DNA, A-fork (5′) DNA (3′-flap DNA), A-fork (3′,5′) DNA (fork DNA) and cruciform DNA were generated by oligonucleotide annealing, as described in ref. 32. Various combinations of oligonucleotides were mixed in 10 mM Tris-HCl, pH 7.5, and 1 mM EDTA, heated at 98 °C for 4 min and cooled to room temperature.…”

Section: Competing Financial Interestsmentioning

confidence: 99%

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Rif1 binds to G quadruplexes and suppresses replication over long distances

Kanoh

Matsumoto

Fukatsu

et al. 2015

Nat Struct Mol Biol

146

169

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Rif1 regulates replication timing and repair of double-strand DNA breaks. Using a chromatin immunoprecipitation-sequencing method, we identified 35 high-affinity Rif1-binding sites in fission yeast chromosomes. Binding sites tended to be located near dormant origins and to contain at least two copies of a conserved motif, CNWWGTGGGGG. Base substitution within these motifs resulted in complete loss of Rif1 binding and in activation of late-firing or dormant origins located up to 50 kb away. We show that Rif1-binding sites adopt G quadruplex-like structures in vitro, in a manner dependent on the conserved sequence and on other G tracts, and that purified Rif1 preferentially binds to this structure. These results suggest that Rif1 recognizes and binds G quadruplex-like structures at selected intergenic regions, thus generating local chromatin structures that may exert long-range suppressive effects on origin firing.

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Section: Purified Rif Protein Binds To G-quadruplex Structuresmentioning

confidence: 99%

Section: Competing Financial Interestsmentioning

confidence: 99%

Rif1 binds to G quadruplexes and suppresses replication over long distances

Kanoh

Matsumoto

Fukatsu

et al. 2015

Nat Struct Mol Biol

146

169

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“…The Stokes radius ( R S ) of each TALE was estimated using the elution time with reference to a standard globular protein set (GE Healthcare)27. The experimental conditions used for the chromatography were the same as described in the sample preparation.…”

Section: Methodsmentioning

confidence: 99%

“…The HiLoad 26/600 Superdex 200 pg column was calibrated with a Gel Filtration Protein Calibration Kit (GE Healthcare) at a linear flow rate of 1 ml/min. The protein standards were as follows: Aprotinin ( M W : 6.5 kDa, R S : 13 Å), Ribonuclease A ( M W : 13.7 kDa, R S : 16 Å), Carbonic anhydrase ( M W : 29.0 kDa, R S : 20 Å), Ovalbumin ( M W : 44.0 kDa, R S : 30 Å), and Conalbumin ( M W : 75.0 kDa, R S : 36 Å)27. The gel-phase distribution coefficient, K av , for each protein was calculated using the equation K av = ( V e − V 0 )/( V c − V 0 ), where V e is the elution volume for the protein, V 0 is the column void volume determined using blue dextran 2000 (GE Healthcare) monitored at a wavelength of 280 nm, and V c is the geometric column volume (320 ml).…”

Section: Methodsmentioning

confidence: 99%

Non-RVD mutations that enhance the dynamics of the TAL repeat array along the superhelical axis improve TALEN genome editing efficacy

Tochio

Umehara

Uewaki

et al. 2016

Sci Rep

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Transcription activator-like effector (TALE) nuclease (TALEN) is widely used as a tool in genome editing. The DNA binding part of TALEN consists of a tandem array of TAL-repeats that form a right-handed superhelix. Each TAL-repeat recognises a specific base by the repeat variable diresidue (RVD) at positions 12 and 13. TALEN comprising the TAL-repeats with periodic mutations to residues at positions 4 and 32 (non-RVD sites) in each repeat (VT-TALE) exhibits increased efficacy in genome editing compared with a counterpart without the mutations (CT-TALE). The molecular basis for the elevated efficacy is unknown. In this report, comparison of the physicochemical properties between CT- and VT-TALEs revealed that VT-TALE has a larger amplitude motion along the superhelical axis (superhelical motion) compared with CT-TALE. The greater superhelical motion in VT-TALE enabled more TAL-repeats to engage in the target sequence recognition compared with CT-TALE. The extended sequence recognition by the TAL-repeats improves site specificity with limiting the spatial distribution of FokI domains to facilitate their dimerization at the desired site. Molecular dynamics simulations revealed that the non-RVD mutations alter inter-repeat hydrogen bonding to amplify the superhelical motion of VT-TALE. The TALEN activity is associated with the inter-repeat hydrogen bonding among the TAL repeats.

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“…Furthermore, they showed that CRII binds cruciform DNA with high selectivity and is therefore a DNA binding domain. 43 In a point of view article in Epigenetics, GonzalezRomero and Ausio discuss the unusual histone H1 variant in Drosophila, called dBigH1. 44 They state that, despite the presence of unusual acidic amino acid patches at the N-terminal end of dBigH1, in contrast to the arginine patches at the N-and C-terminal domains of other histone H1 proteins, the essential requirements of H1 proteins appears to be the presence of a lysine-and alanine-rich intrinsically disordered C-terminal domain.…”

Section: Analyzing Functions Of Idps and Idprsmentioning

confidence: 99%

Quarterly intrinsic disorder digest (April–May–June, 2014)

DeForte

Uversky

2017

Intrinsically Disordered Proteins

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This is the 6 th issue of the Digested Disorder series that continues to use only 2 criteria for inclusion of a paper to this digest: The publication date (a paper should be published within the covered time frame) and the topic (a paper should be dedicated to any aspect of protein intrinsic disorder). The current digest issue covers papers published during the second quarter of 2014; i.e., during the period of April, May, and June of 2014. Similar to previous issues, the papers are grouped hierarchically by topics they cover, and for each of the included papers a short description is given on its major findings.

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Structural and Biophysical Characterization of Murine Rif1 C Terminus Reveals High Specificity for DNA Cruciform Structures

Cited by 33 publications

References 41 publications

Rif1 binds to G quadruplexes and suppresses replication over long distances

Rif1 binds to G quadruplexes and suppresses replication over long distances

Non-RVD mutations that enhance the dynamics of the TAL repeat array along the superhelical axis improve TALEN genome editing efficacy

Quarterly intrinsic disorder digest (April–May–June, 2014)

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