Your search keyword '"Shubeena Chib"' showing total 8 results

1. DEAD-box RNA helicases Dbp2, Ded1 and Mss116 bind to G-quadruplex nucleic acids and destabilize G-quadruplex RNA

Author

Samuel G. Mackintosh, Shubeena Chib, John C. Marecki, Zachary J Waldrip, Andrea D Edwards, Andrea Putnam, Alicia K. Byrd, Michael J. Guderyon, Kevin D. Raney, Boris Zybailov, Zhaofeng Gao, Kirk West, Jun Gao, and Eckhard Jankowsky

Subjects

Saccharomyces cerevisiae Proteins, Saccharomyces cerevisiae, Plasma protein binding, 010402 general chemistry, G-quadruplex, 01 natural sciences, DNA-binding protein, Article, Catalysis, DEAD-box RNA Helicases, Adenosine Triphosphate, Affinity chromatography, Tandem Mass Spectrometry, Materials Chemistry, heterocyclic compounds, Chromatography, High Pressure Liquid, biology, 010405 organic chemistry, Chemistry, Metals and Alloys, Helicase, RNA, General Chemistry, Recombinant Proteins, In vitro, 0104 chemical sciences, Surfaces, Coatings and Films, Electronic, Optical and Magnetic Materials, G-Quadruplexes, Kinetics, Biochemistry, Ceramics and Composites, biology.protein, Nucleic acid, Protein Binding

Abstract

We identified 29 G-quadruplex binding proteins by affinity purification and quantitative LC-MS/MS. We demonstrated that the DEAD-box RNA helicases Dbp2, Ded1 and Mss116 preferentially bind to G-quadruplex nucleic acids in vitro and destabilize RNA quadruplexes, suggesting new potential roles for these helicases in disruption of quadruplex structures in RNA.

Published

2019

2. A biochemical and biophysical model of G-quadruplex DNA recognition by positive coactivator of transcription 4

Author

Kevin D. Raney, Wezley C. Griffin, Alicia K. Byrd, Shubeena Chib, and Jun Gao

Subjects

Models, Molecular, 0301 basic medicine, DNA, Single-Stranded, DNA footprinting, DNA and Chromosomes, Biology, Biochemistry, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Coactivator, Humans, Protein–DNA interaction, A-DNA, Molecular Biology, Replication protein A, Genetics, Cell Biology, DNA-Binding Proteins, G-Quadruplexes, DNA binding site, 030104 developmental biology, chemistry, Transcription Coactivator, Biophysics, 030217 neurology & neurosurgery, DNA, Protein Binding, Transcription Factors

Abstract

DNA sequences that are guanine-rich have received considerable attention because of their potential to fold into a secondary, four-stranded DNA structure termed G-quadruplex (G4), which has been implicated in genomic instability and some human diseases. We have previously identified positive coactivator of transcription (PC4), a single-stranded DNA (ssDNA)-binding protein, as a novel G4 interactor. Here, to expand on these previous observations, we biochemically and biophysically characterized the interaction between PC4 and G4DNA. PC4 can bind alternative G4DNA topologies with a low nanomolar Kd value of ∼2 nm, similar to that observed for ssDNA. In consideration of the different structural features between G4DNA and ssDNA, these binding data indicated that PC4 can interact with G4DNA in a manner distinct from ssDNA. The stoichiometry of the PC4-G4 complex was 1:1 for PC4 dimer:G4 substrate. PC4 did not enhance the rate of folding of G4DNA, and formation of the PC4-G4DNA complex did not result in unfolding of the G4DNA structure. We assembled a G4DNA structure flanked by duplex DNA. We find that PC4 can interact with this G4DNA, as well as the complementary C-rich strand. Molecular docking simulations and DNA footprinting experiments suggest a model where a PC4 dimer accommodates the DNA with one monomer on the G4 strand and the second monomer bound to the C-rich strand. Collectively, these data provide a novel mode of PC4 binding to a DNA secondary structure that remains within the framework of the model for binding to ssDNA. Additionally, consideration of the PC4-G4DNA interaction could provide insight into the biological functions of PC4, which remain incompletely understood.

Published

2017

3. Evidence That G-quadruplex DNA Accumulates in the Cytoplasm and Participates in Stress Granule Assembly in Response to Oxidative Stress

Author

Mihir Jaiswal, Samuel G. Mackintosh, Shubeena Chib, Wezley C. Griffin, Megan R. Reed, Matthew R. Bell, Boris Zybailov, Kevin D. Raney, Leena Maddukuri, Angus M. MacNicol, Giulia Baldini, John C. Marecki, Alicia K. Byrd, Robert L. Eoff, and Jun Gao

Subjects

0301 basic medicine, Cytoplasm, DNA damage, DNA repair, DNA and Chromosomes, Cytoplasmic Granules, medicine.disease_cause, Biochemistry, 03 medical and health sciences, chemistry.chemical_compound, Stress granule, medicine, Humans, Stress granule assembly, RNA, Messenger, Molecular Biology, Cell Biology, Nuclear DNA, Cell biology, G-Quadruplexes, Oxidative Stress, 030104 developmental biology, chemistry, Protein Biosynthesis, DNA, Oxidative stress, DNA Damage, HeLa Cells

Abstract

Cells engage numerous signaling pathways in response to oxidative stress that together repair macromolecular damage or direct the cell toward apoptosis. As a result of DNA damage, mitochondrial DNA or nuclear DNA has been shown to enter the cytoplasm where it binds to "DNA sensors," which in turn initiate signaling cascades. Here we report data that support a novel signaling pathway in response to oxidative stress mediated by specific guanine-rich sequences that can fold into G-quadruplex DNA (G4DNA). In response to oxidative stress, we demonstrate that sequences capable of forming G4DNA appear at increasing levels in the cytoplasm and participate in assembly of stress granules. Identified proteins that bind to endogenous G4DNA in the cytoplasm are known to modulate mRNA translation and participate in stress granule formation. Consistent with these findings, stress granule formation is known to regulate mRNA translation during oxidative stress. We propose a signaling pathway whereby cells can rapidly respond to DNA damage caused by oxidative stress. Guanine-rich sequences that are excised from damaged genomic DNA are proposed to enter the cytoplasm where they can regulate translation through stress granule formation. This newly proposed role for G4DNA provides an additional molecular explanation for why such sequences are prevalent in the human genome.

Published

2016

4. Yeast Helicase Pif1 Unwinds RNA:DNA Hybrids with Higher Processivity than DNA:DNA Duplexes

Author

Alicia K. Byrd, Shubeena Chib, and Kevin D. Raney

Subjects

0301 basic medicine, Saccharomyces cerevisiae Proteins, DNA polymerase, Base pair, DNA polymerase II, Saccharomyces cerevisiae, Biochemistry, 03 medical and health sciences, DNA, Fungal, Molecular Biology, Adenosine Triphosphatases, DNA clamp, biology, Circular bacterial chromosome, DNA Helicases, Nucleic Acid Hybridization, RNA, Fungal, Cell Biology, Processivity, Kinetics, 030104 developmental biology, Enzymology, biology.protein, DNA supercoil, Primase

Abstract

Saccharomyces cerevisiae Pif1, an SF1B helicase, has been implicated in both mitochondrial and nuclear functions. Here we have characterized the preference of Pif1 for RNA:DNA heteroduplexes in vitro by investigating several kinetic parameters associated with unwinding. We show that the preferential unwinding of RNA:DNA hybrids is due to neither specific binding nor differences in the rate of strand separation. Instead, Pif1 is capable of unwinding RNA:DNA heteroduplexes with moderately greater processivity compared with its duplex DNA:DNA counterparts. This higher processivity of Pif1 is attributed to slower dissociation from RNA:DNA hybrids. Biologically, this preferential role of the helicase may contribute to its functions at both telomeric and nontelomeric sites.

Published

2016

5. Yeast Sub1 and human PC4 are G-quadruplex binding proteins that suppress genome instability at co-transcriptionally formed G4 DNA

Author

Nayun Kim, Christopher R. Lopez, Shashank Hambarde, Kevin D. Raney, Jun Gao, Wezley C. Griffin, Yang Yu, Shubeena Chib, Grzegorz Ira, and Shivani Singh

Subjects

0301 basic medicine, Genome instability, Saccharomyces cerevisiae Proteins, HMG-box, Transcription, Genetic, Base pair, Saccharomyces cerevisiae, Biology, Genome Integrity, Repair and Replication, Genomic Instability, 03 medical and health sciences, Gene Expression Regulation, Fungal, Genetics, Humans, Amino Acid Sequence, DNA, Fungal, Replication protein A, DNA clamp, Binding Sites, Genome, 030102 biochemistry & molecular biology, Sequence Homology, Amino Acid, DNA Helicases, DNA binding site, DNA-Binding Proteins, G-Quadruplexes, 030104 developmental biology, DNA Topoisomerases, Type I, DNA supercoil, Sequence Alignment, In vitro recombination, Protein Binding, Transcription Factors

Abstract

G-quadruplex or G4 DNA is a non-B secondary DNA structure consisting of a stacked array of guanine-quartets that can disrupt critical cellular functions such as replication and transcription. When sequences that can adopt Non-B structures including G4 DNA are located within actively transcribed genes, the reshaping of DNA topology necessary for transcription process stimulates secondary structure-formation thereby amplifying the potential for genome instability. Using a reporter assay designed to study G4-induced recombination in the context of an actively transcribed locus in Saccharomyces cerevisiae, we tested whether co-transcriptional activator Sub1, recently identified as a G4-binding factor, contributes to genome maintenance at G4-forming sequences. Our data indicate that, upon Sub1-disruption, genome instability linked to co-transcriptionally formed G4 DNA in Top1-deficient cells is significantly augmented and that its highly conserved DNA binding domain or the human homolog PC4 is sufficient to suppress G4-associated genome instability. We also show that Sub1 interacts specifically with co-transcriptionally formed G4 DNA in vivo and that yeast cells become highly sensitivity to G4-stabilizing chemical ligands by the loss of Sub1. Finally, we demonstrate the physical and genetic interaction of Sub1 with the G4-resolving helicase Pif1, suggesting a possible mechanism by which Sub1 suppresses instability at G4 DNA.

Published

2017

6. When Helicase and Polymerases Collides and Unfolds G4-Quadruplex on their Track

Author

Jean-Baptiste Boulé, Shubeena Chib, Vincent Croquette, Samar Hodeib, and Kevin D. Raney

Subjects

Physics, biology, Track (disk drive), Biophysics, biology.protein, Helicase, Polymerase

Published

2018

7. Yeast transcription co-activator Sub1 and its human homolog PC4 preferentially bind to G-quadruplex DNA

Author

Jun Gao, Samuel G. Mackintosh, Shubeena Chib, Alan J. Tackett, Wezley C. Griffin, Kevin D. Raney, Alicia K. Byrd, and Boris Zybailov

Subjects

Saccharomyces cerevisiae Proteins, Response element, E-box, G-quadruplex, Catalysis, Article, Substrate Specificity, chemistry.chemical_compound, Transcription (biology), Materials Chemistry, Humans, heterocyclic compounds, General transcription factor, Base Sequence, Sequence Homology, Amino Acid, Binding protein, Metals and Alloys, General Chemistry, DNA, Molecular biology, Surfaces, Coatings and Films, Electronic, Optical and Magnetic Materials, Cell biology, DNA-Binding Proteins, G-Quadruplexes, chemistry, TAF2, Ceramics and Composites, Protein Binding, Transcription Factors

Abstract

Using a G-quadruplex bait, we identified the transcription co-activator Sub1 as a G-quadruplex binding protein by quantitative LC-MS/MS and demonstrated in vivo G-quadruplex binding by ChIP. In vitro, Sub1, and its human homolog PC4, bind preferentially to G-quadruplexes. This provides a possible mechanism by which G-quadruplexes can influence gene transcription.

Published

2015

8. Yeast Pif1 helicase exhibits a one-base-pair stepping mechanism for unwinding duplex DNA

Author

Smita S. Patel, Alicia K. Byrd, Manjula Pandey, Suja Aarattuthodiyil, Shubeena Chib, Kevin D. Raney, and Ramanagouda Ramanagoudr-Bhojappa

Subjects

chemistry.chemical_classification, Streptavidin, Saccharomyces cerevisiae Proteins, biology, Oligonucleotide, Base pair, DNA Helicases, Helicase, DNA, Single-Stranded, Cell Biology, Saccharomyces cerevisiae, DNA and Chromosomes, Biochemistry, chemistry.chemical_compound, Kinetics, Adenosine Triphosphate, chemistry, ATP hydrolysis, biology.protein, Nucleotide, Primase, DNA, Fungal, Molecular Biology, DNA

Abstract

Kinetic analysis of the DNA unwinding and translocation activities of helicases is necessary for characterization of the biochemical mechanism(s) for this class of enzymes. Saccharomyces cerevisiae Pif1 helicase was characterized using presteady state kinetics to determine rates of DNA unwinding, displacement of streptavidin from biotinylated DNA, translocation on single-stranded DNA (ssDNA), and ATP hydrolysis activities. Unwinding of substrates containing varying duplex lengths was fit globally to a model for stepwise unwinding and resulted in an unwinding rate of ∼75 bp/s and a kinetic step size of 1 base pair. Pif1 is capable of displacing streptavidin from biotinylated oligonucleotides with a linear increase in the rates as the length of the oligonucleotides increased. The rate of translocation on ssDNA was determined by measuring dissociation from varying lengths of ssDNA and is essentially the same as the rate of unwinding of dsDNA, making Pif1 an active helicase. The ATPase activity of Pif1 on ssDNA was determined using fluorescently labeled phosphate-binding protein to measure the rate of phosphate release. The quantity of phosphate released corresponds to a chemical efficiency of 0.84 ATP/nucleotides translocated. Hence, when all of the kinetic data are considered, Pif1 appears to move along DNA in single nucleotide or base pair steps, powered by hydrolysis of 1 molecule of ATP. Background: Pif1 helicase plays a variety of roles in both the nucleus and mitochondria. Results: The kinetic step size for Pif1 is one base pair, and translocation on ssDNA is coupled tightly with ATP hydrolysis. Conclusion: Hydrolysis of one ATP results in movement of Pif1 by a single nucleotide. Significance: Pif1 is an active helicase with a uniform stepping mechanism.

Published

2013