Your search keyword '"R., Bianco"' showing total 71 results

1. SSB Facilitates Fork-Substrate Discrimination by the PriA DNA Helicase

Author

Hui Yin Tan and Piero R. Bianco

Subjects

Chemistry, QD1-999

Published

2021

2. Rep and UvrD Antagonize One Another at Stalled Replication Forks and This Is Exacerbated by SSB

Author

Xiaoyi Liu, Jiun Xiang Seet, Yi Shi, and Piero R. Bianco

Subjects

Chemistry, QD1-999

Published

2019

3. The mechanism of action of the <scp>SSB</scp> interactome reveals it is the first <scp>OB</scp> ‐fold family of genome guardians in prokaryotes

Author

Piero R. Bianco

Subjects

DNA, Bacterial, Models, Molecular, Protein Conformation, Amino Acid Motifs, Oligonucleotides, Reviews, DNA, Single-Stranded, Oligosaccharides, Computational biology, Binding, Competitive, Biochemistry, Interactome, Genome, DNA-binding protein, SH3 domain, 03 medical and health sciences, chemistry.chemical_compound, Bacterial Proteins, Protein Interaction Mapping, Escherichia coli, medicine, Gene Regulatory Networks, Molecular Biology, 030304 developmental biology, 0303 health sciences, Oligonucleotide, Chemistry, 030302 biochemistry & molecular biology, Gene Expression Regulation, Bacterial, DNA-Binding Proteins, Klebsiella pneumoniae, Mechanism of action, Protein Multimerization, medicine.symptom, Linker, Genome, Bacterial, DNA, Protein Binding

Abstract

The single-stranded DNA binding protein (SSB) is essential to all aspects of DNA metabolism in bacteria. This protein performs two distinct, but closely intertwined and indispensable functions in the cell. SSB binds to single-stranded DNA (ssDNA) and at least 20 partner proteins resulting in their regulation. These partners comprise a family of genome guardians known as the SSB interactome. Essential to interactome regulation is the linker/OB-fold network of interactions. This network of interactions forms when one or more PXXP motifs in the linker of SSB bind to an OB-fold in a partner, with interactome members involved in competitive binding between the linker and ssDNA to their OB-fold. Consequently, when linker-binding occurs to an OB-fold in an interactome partner, proteins are loaded onto the DNA. When linker/OB-fold interactions occur between SSB tetramers, cooperative ssDNA-binding results, producing a multi-tetrameric complex that rapidly protects the ssDNA. Within this SSB-ssDNA complex, there is an extensive and dynamic network of linker/OB-fold interactions that involves multiple tetramers bound contiguously along the ssDNA lattice. The dynamic behavior of these tetramers which includes binding mode changes, sliding as well as DNA wrapping/unwrapping events, are likely coupled to the formation and disruption of linker/OB-fold interactions. This behavior is essential to facilitating downstream DNA processing events. As OB-folds are critical to the essence of the linker/OB-fold network of interactions, and they are found in multiple interactome partners, the SSB interactome is classified as the first family of prokaryotic, oligosaccharide/oligonucleotide binding fold (OB-fold) genome guardians.

Published

2021

4. Single-molecule insight into stalled replication fork rescue in Escherichia coli

Author

Yue Lu and Piero R. Bianco

Subjects

DNA Replication, Exodeoxyribonuclease V, AcademicSubjects/SCI00010, Cell, Biology, medicine.disease_cause, chemistry.chemical_compound, RuvABC, Bacterial Proteins, Escherichia coli, Genetics, medicine, Survey and Summary, RecBCD, Endodeoxyribonucleases, Escherichia coli Proteins, DNA replication, Cell cycle, DNA Replication Fork, Single Molecule Imaging, Cell biology, DNA-Binding Proteins, medicine.anatomical_structure, chemistry, DNA

Abstract

DNA replication forks stall at least once per cell cycle in Escherichia coli. DNA replication must be restarted if the cell is to survive. Restart is a multi-step process requiring the sequential action of several proteins whose actions are dictated by the nature of the impediment to fork progression. When fork progress is impeded, the sequential actions of SSB, RecG and the RuvABC complex are required for rescue. In contrast, when a template discontinuity results in the forked DNA breaking apart, the actions of the RecBCD pathway enzymes are required to resurrect the fork so that replication can resume. In this review, we focus primarily on the significant insight gained from single-molecule studies of individual proteins, protein complexes, and also, partially reconstituted regression and RecBCD pathways. This insight is related to the bulk-phase biochemical data to provide a comprehensive review of each protein or protein complex as it relates to stalled DNA replication fork rescue.

Published

2021

5. Atomic force microscopy–based characterization of the interaction of PriA helicase with stalled DNA replication forks

Author

Zhiqiang Sun, Yaqing Wang, Yuri L. Lyubchenko, and Piero R. Bianco

Subjects

DNA Replication, 0301 basic medicine, Dna duplex, Substrate recognition, Microscopy, Atomic Force, Biochemistry, Substrate Specificity, 03 medical and health sciences, chemistry.chemical_compound, Protein–DNA interaction, Molecular Biology, dnaB helicase, 030102 biochemistry & molecular biology, biology, Chemistry, Atomic force microscopy, DNA Helicases, DNA replication, Helicase, DNA, Cell Biology, Cell biology, stomatognathic diseases, 030104 developmental biology, biology.protein, Molecular Biophysics

Abstract

In bacteria, the restart of stalled DNA replication forks requires the DNA helicase PriA. PriA can recognize and remodel abandoned DNA replication forks, unwind DNA in the 3′-to-5′ direction, and facilitate the loading of the helicase DnaB onto the DNA to restart replication. Single-stranded DNA–binding protein (SSB) is typically present at the abandoned forks, but it is unclear how SSB and PriA interact, although it has been shown that the two proteins interact both physically and functionally. Here, we used atomic force microscopy to visualize the interaction of PriA with DNA substrates with or without SSB. These experiments were done in the absence of ATP to delineate the substrate recognition pattern of PriA before its ATP-catalyzed DNA-unwinding reaction. These analyses revealed that in the absence of SSB, PriA binds preferentially to a fork substrate with a gap in the leading strand. Such a preference has not been observed for 5′- and 3′-tailed duplexes, suggesting that it is the fork structure that plays an essential role in PriA's selection of DNA substrates. Furthermore, we found that in the absence of SSB, PriA binds exclusively to the fork regions of the DNA substrates. In contrast, fork-bound SSB loads PriA onto the duplex DNA arms of forks, suggesting a remodeling of PriA by SSB. We also demonstrate that the remodeling of PriA requires a functional C-terminal domain of SSB. In summary, our atomic force microscopy analyses reveal key details in the interactions between PriA and stalled DNA replication forks with or without SSB.

Published

2020

6. The mechanism of<scp>Single strand binding protein–RecG</scp>binding: Implications for<scp>SSB</scp>interactome function

Author

Karin R. Hsieh, Hui Yin Tan, Wenfei Ding, Jia Xiang Zhang, Piero R. Bianco, Jeffrey A. Mulkin, and Luke A. Wilczek

Subjects

Models, Molecular, musculoskeletal diseases, Oligonucleotides, Oligosaccharides, Computational biology, Biochemistry, DNA-binding protein, Interactome, SH3 domain, Single-stranded binding protein, 03 medical and health sciences, chemistry.chemical_compound, stomatognathic system, Point Mutation, skin and connective tissue diseases, Molecular Biology, 030304 developmental biology, 0303 health sciences, Binding Sites, biology, Chemistry, Escherichia coli Proteins, 030302 biochemistry & molecular biology, Helicase, Articles, eye diseases, DNA-Binding Proteins, stomatognathic diseases, PXXP Motif, biology.protein, DNA, Binding domain

Abstract

The Escherichia coli single‐strand DNA binding protein (SSB) is essential to viability where it functions to regulate SSB interactome function. Here it binds to single‐stranded DNA and to target proteins that comprise the interactome. The region of SSB that links these two essential protein functions is the intrinsically disordered linker. Key to linker function is the presence of three, conserved PXXP motifs that mediate binding to oligosaccharide‐oligonucleotide binding folds (OB‐fold) present in SSB and its interactome partners. Not surprisingly, partner OB‐fold deletions eliminate SSB binding. Furthermore, single point mutations in either the PXXP motifs or, in the RecG OB‐fold, obliterate SSB binding. The data also demonstrate that, and in contrast to the view currently held in the field, the C‐terminal acidic tip of SSB is not required for interactome partner binding. Instead, we propose the tip has two roles. First, and consistent with the proposal of Dixon, to regulate the structure of the C‐terminal domain in a biologically active conformation that prevents linkers from binding to SSB OB‐folds until this interaction is required. Second, as a secondary binding domain. Finally, as OB‐folds are present in SSB and many of its partners, we present the SSB interactome as the first family of OB‐fold genome guardians identified in prokaryotes.

Published

2020

7. Nanoscale interaction of RecG with mobile fork DNA

Author

Zhiqiang Sun, Yuri L. Lyubchenko, Yaqing Wang, and Piero R. Bianco

Subjects

0303 health sciences, biology, Atomic force microscopy, 030302 biochemistry & molecular biology, General Engineering, Helicase, Bioengineering, General Chemistry, Bacterial genome size, DNA Replication Fork, DNA-binding protein, Article, Atomic and Molecular Physics, and Optics, stomatognathic diseases, 03 medical and health sciences, chemistry.chemical_compound, chemistry, Duplex (building), Fork (system call), biology.protein, Biophysics, General Materials Science, DNA, 030304 developmental biology

Abstract

The RecG DNA helicase is a guardian of the bacterial genome where it dominates stalled DNA replication fork rescue. The single-stranded DNA binding protein (SSB) is involved in this process and promotes the binding of RecG to stalled replication forks. Atomic force microscopy (AFM) was used to investigate the interaction of RecG and SSB on a mobile fork substrate capable of being regressed. In the absence of proteins, the fork undergoes spontaneous dynamics between two states defined by the length of the DNA complementarity at the fork. Binding of SSB does not affect these dynamics as it binds to single-stranded regions as expected. In contrast, RecG interacts with the two states quite differently. We demonstrate that RecG has two modes of interaction with fork DNA in the presence of SSB and ATP. In the first mode, RecG translocates over the duplex region and this activity is defined by SSB-mediated remodeling of the helicase. In the second mode, RecG utilizes its helicase activity to regress the fork, in an ATP-dependent manner, displacing SSB on the ssDNA. Overall, our results highlight two functions of RecG that can be employed in the regulation of stalled DNA replication fork rescue.

Published

2020

8. Dynamics of the PriA Helicase at Stalled DNA Replication Forks

Author

Piero R. Bianco, Yuri L. Lyubchenko, Yaqing Wang, and Zhiqiang Sun

Subjects

DNA Replication, Dna duplex, DNA, Single-Stranded, 010402 general chemistry, 01 natural sciences, Primosome, Article, chemistry.chemical_compound, 0103 physical sciences, Materials Chemistry, Physical and Theoretical Chemistry, Helicase activity, 010304 chemical physics, biology, Chemistry, Atomic force microscopy, Escherichia coli Proteins, DNA replication, DNA Helicases, Helicase, DNA, 0104 chemical sciences, Surfaces, Coatings and Films, Cell biology, DNA-Binding Proteins, biology.protein

Abstract

The DNA helicase PriA is a key protein for restarting stalled DNA replication forks in bacteria. With 3′ to 5′ helicase activity, PriA is important in primosome assembly. We used atomic force microscopy (AFM) and specifically employed time-lapse AFM to visualize the interaction of PriA with two DNA substrates. The results show that most of the PriA molecules are observed bound at the fork. However, PriA is capable of translocating over distances of about 400 bp. There is a preference for the long-range translocation of PriA depending on the fork type. For a fork with the nascent leading strand as single-stranded DNA (ssDNA; F4 substrate), PriA translocates preferentially on the parental arm of the fork. For the substrate F14, which contains an additional ssDNA segment between the parental and lagging arms (5 nt gap), PriA translocates on both the parental and lagging strand arms. These data suggest that transient formation of the single-stranded regions during the DNA replication can change the selection of the DNA duplex by PriA. Translocation of the helicase was directly visualized by time-lapse AFM imaging, which revealed that PriA can switch strands during translocation. These novel features of PriA shed new light on the mechanisms of PriA interaction with stalled replication forks. [Image: see text]

Published

2021

9. Restriction of RecG translocation by DNA mispairing

Author

Mohtadin Hashemi, Yuri L. Lyubchenko, Zhiqiang Sun, Piero R. Bianco, and Yaqing Wang

Subjects

chemistry.chemical_compound, chemistry, Base pair, Atomic force microscopy, DNA replication, biology.protein, Helicase, Chromosomal translocation, Bacterial genome size, Biology, DNA-binding protein, DNA, Cell biology

Abstract

The RecG DNA helicase plays a crucial role in stalled replication fork rescue as the guardian of the bacterial genome. We have recently demonstrated that single-strand DNA binding protein (SSB) promotes binding of RecG to the stalled replication fork by remodeling RecG, enabling the helicase to translocate ahead of the fork. We also hypothesized that mispairing of DNA could limit such translocation of RecG, which plays the role of roadblocks for the fork movement. Here, we used atomic force microscopy (AFM) to directly test this hypothesis and investigate how sensitive RecG translocation is to different types of mispairing. We found that a C-C mismatch at a distance of 30 bp away from the fork position prevents translocation of RecG over this mispairing. A G-bulge placed at the same distance also has a similar roadblock efficiency. However, a C-C mismatch 10 bp away from the fork does not prevent RecG translocation, as 10 bp from fork is within the distance of footprint of RecG on fork DNA. Our findings suggest that retardation of RecG translocation ahead of the replication fork can be a mechanism for the base pairing control for DNA replication machinery.

Published

2021

10. In Vivo Binding of Single-Stranded DNA-Binding Protein to Stalled Replication Fork Helicases

Author

Piero R. Bianco and Cong Yu

Subjects

DNA Replication, DNA, Bacterial, Cell, DNA, Single-Stranded, medicine.disease_cause, Article, law.invention, Single-stranded binding protein, 03 medical and health sciences, In vivo, law, Single-stranded DNA binding, Escherichia coli, medicine, Protein complex formation, 030304 developmental biology, 0303 health sciences, Binding Sites, biology, Chemistry, Escherichia coli Proteins, 030302 biochemistry & molecular biology, DNA Helicases, Helicase, Recombinant Proteins, Cell biology, DNA-Binding Proteins, medicine.anatomical_structure, biology.protein, Recombinant DNA, Electrophoresis, Polyacrylamide Gel, Plasmids, Protein Binding

Abstract

Understanding protein-protein interactions is key to unraveling protein function in vivo. Here we describe a dual/triple-plasmid system that enables co-expression of two, or three, recombinant proteins harboring different affinity tags in the same Escherichia coli cell. This novel protein expression system provides a platform to understand protein-protein interactions and enables researchers to study protein complex formation and in vivo localization.

Published

2021

11. Characterize the Interaction of the DNA Helicase PriA with the Stalled DNA Replication Fork Using Atomic Force Microscopy

Author

Zhiqiang Sun, Yaqing Wang, Yuri L. Lyubchenko, and Piero R. Bianco

Subjects

biology, Chemistry, Atomic force microscopy, Strategy and Management, Mechanical Engineering, Metals and Alloys, DNA replication, Helicase, DNA Replication Fork, Industrial and Manufacturing Engineering, chemistry.chemical_compound, Förster resonance energy transfer, Methods Article, biology.protein, Biophysics, Surface plasmon resonance, dnaB helicase, DNA

Abstract

In bacteria, the restart of stalled DNA replication forks requires the DNA helicase PriA. PriA can recognize and remodel abandoned DNA replication forks, unwind DNA in the 3'-to-5' direction, and facilitate the loading of the helicase DnaB onto the DNA to restart replication. ssDNA-binding protein (SSB) is typically present at the abandoned forks, protecting the ssDNA from nucleases. Research that is based on the assays for junction dissociation, surface plasmon resonance, single-molecule FRET, and x-ray crystal structure has revealed the helicase activity of PriA, the SSB-PriA interaction, and structural information of PriA helicase. Here, we used Atomic Force Microscopy (AFM) to visualize the interaction between PriA and DNA substrates with or without SSB in the absence of ATP to delineate the substrate recognition pattern of PriA before its ATP-catalyzed DNA-unwinding reaction. The protocol describes the steps to obtain high-resolution AFM images and the details of data analysis and presentation.

Published

2021

12. SSB facilitates fork substrate discrimination by PriA

Author

Hui Yin Tan and Piero R. Bianco

Subjects

Bacteriophage, biology, Chemistry, DNA replication, biology.protein, Atpase activity, Substrate (chemistry), Helicase, Fork (file system), biology.organism_classification, Gene, Primosome, Cell biology

Abstract

PriA is a member of the SuperFamily 2 helicase family. Its rolein vivois to reload the primosome onto stalled replication forks resulting in the restart of the previously stalled DNA replication process. SSB is known to play key roles in mediating activities at replication forks and it is known to bind to PriA. To gain mechanistic insight into the PriA-SSB interaction, a coupled spectrophotometric assay was utilized to characterize the ATPase activity of PriAin vitroin the presence of fork substrates. The results demonstrate that SSB enhances the ability of PriA to discriminate between fork substrates 140-fold. This is due to a significant increase in the catalytic efficiency of the helicase induced by DNA-bound SSB. This interaction is species-specific as bacteriophage gene 32 protein cannot substitute for theE.coliprotein. SSB, while enhancing the activity of PriA on its preferred fork, both decreases the affinity of the helicase for other forks and decreases catalytic efficiency. Central to the stimulation afforded by SSB is the unique ability of PriA to bind with high affinity to the 3’-OH placed at the end of the nascent leading strand at the fork. When both the 3’-OH and SSB are present, the maximum effect is observed. This ensures that PriA will only load onto the correct fork, in the right orientation, thereby ensuring that replication restart is directed to only the template lagging strand.

Published

2020

13. High-yield purification of exceptional-quality, single-molecule DNA substrates

Author

Yue Lu and Piero R. Bianco

Subjects

oligonucleotide, column chromatography, Oligonucleotide, DNA substrate, Substrate (chemistry), Combinatorial chemistry, Article, chemistry.chemical_compound, Column chromatography, chemistry, Yield (chemistry), TSKgel DNA-stat, Nucleic acid, General Earth and Planetary Sciences, Molecule, single-molecule, Ion-exchange resin, DNA, General Environmental Science

Abstract

Single-molecule studies involving DNA or RNA, require homogeneous preparations of nucleic acid substrates of exceptional quality. Over the past several years, a variety of methods have been published describing different purification methods but these are frustratingly inconsistent with variable yields even in the hands of experienced bench scientists. To address these issues, we present an optimized and straightforward, column-based approach that is reproducible and produces high yields of substrates or substrate components of exceptional quality. Central to the success of the method presented is the use of a non-porous anion exchange resin. In addition to the use of this resin, we encourage the optimization of each step in the construction of substrates. The fully optimized method produces high yields of a hairpin DNA substrate of exceptional quality. While this substrate is suitable for single-molecule, magnetic tweezer experiments, the described method is readily adaptable to the production of DNA substrates for the majority of single-molecule studies involving nucleic acids ranging in size from 70–15000 bp.

Published

2020

14. DNA Helicase-SSB Interactions Critical to the Regression and Restart of Stalled DNA Replication Forks in Escherichia coli

Author

Piero R. Bianco

Subjects

0301 basic medicine, lcsh:QH426-470, DNA repair, DNA replication, 03 medical and health sciences, chemistry.chemical_compound, Genetics, Holliday junction, RecG, biochemistry, Genetics (clinical), dnaB helicase, 030102 biochemistry & molecular biology, biology, Chemistry, Helicase, Cell cycle, Cell biology, helicase, lcsh:Genetics, single-strand binding protein (SSB), 030104 developmental biology, Stalled DNA replication fork, biology.protein, Replisome, DNA

Abstract

In Escherichia coli, DNA replication forks stall on average once per cell cycle. When this occurs, replisome components disengage from the DNA, exposing an intact, or nearly intact fork. Consequently, the fork structure must be regressed away from the initial impediment so that repair can occur. Regression is catalyzed by the powerful, monomeric DNA helicase, RecG. During this reaction, the enzyme couples unwinding of fork arms to rewinding of duplex DNA resulting in the formation of a Holliday junction. RecG works against large opposing forces enabling it to clear the fork of bound proteins. Following subsequent processing of the extruded junction, the PriA helicase mediates reloading of the replicative helicase DnaB leading to the resumption of DNA replication. The single-strand binding protein (SSB) plays a key role in mediating PriA and RecG functions at forks. It binds to each enzyme via linker/OB-fold interactions and controls helicase-fork loading sites in a substrate-dependent manner that involves helicase remodeling. Finally, it is displaced by RecG during fork regression. The intimate and dynamic SSB-helicase interactions play key roles in ensuring fork regression and DNA replication restart.

Published

2020

15. AFM characterization of the interaction of PriA helicase with stalled DNA replication forks

Author

Yaqing Wang, Zhiqiang Sun, Yuri L. Lyubchenko, and Piero R. Bianco

Subjects

0303 health sciences, Dna duplex, biology, Chemistry, Atomic force microscopy, 030302 biochemistry & molecular biology, DNA replication, Helicase, Cell biology, stomatognathic diseases, 03 medical and health sciences, chemistry.chemical_compound, Single-stranded DNA binding, biology.protein, DNA unwinding, dnaB helicase, DNA, 030304 developmental biology

Abstract

In bacteria, the restart of stalled DNA replication forks requires the PriA DNA helicase. PriA recognizes and remodels abandoned DNA replication forks performing the DNA unwinding in 3’ to 5’-direction and facilitates loading of the DnaB helicase onto the DNA to restart replication. The single stranded DNA binding protein (SSB) is typically present at the abandoned forks, but there is gap in the knowledge on the interaction between SSB and PriA protein. Here, we used atomic force microscopy (AFM) to visualize the interaction of PriA with DNA substrates in the absence or presence of SSB. Results show that in the absence of SSB, PriA binds preferentially to a fork substrate with a gap in the leading strand. Preferential binding occurs only on forked DNA structures as 5’- and 3’-tailed duplexes were bound equally well. Furthermore, in the absence of SSB, PriA bound exclusively to the fork regions of substrates. In contrast, fork bound SSB loads PriA onto the duplex DNA arms of forks. When the fork has a gap in the leading strand, PriA localizes to both the parental and lagging strand arms. When the gap is present in the lagging strand, PriA is loaded preferentially onto the leading strand arm of the fork. Remodeling of PriA requires a functional C-terminal domain of SSB.

Published

2020

16. Editorial: Single-molecule studies of DNA–protein interactions collection 2021

Author

Rodrigo Reyes-Lamothe, Julian E. Sale, and Piero R. Bianco

Subjects

AcademicSubjects/SCI00010, Protein dna, DNA, Computational biology, Biology, Single Molecule Imaging, DNA-Binding Proteins, DNA metabolism, chemistry.chemical_compound, Editorial, chemistry, Genetics, Molecule, Introductory Journal Article

Published

2021

17. The tale of SSB

Author

Piero R. Bianco

Subjects

0301 basic medicine, chemistry.chemical_classification, Genetics, Escherichia coli Proteins, Biophysics, DNA, Single-Stranded, Biology, Models, Biological, Interactome, Article, SH3 domain, Cell biology, DNA-Binding Proteins, 03 medical and health sciences, chemistry.chemical_compound, 030104 developmental biology, Enzyme, chemistry, Tetramer, Single-stranded DNA binding, Nucleic acid, Humans, Molecular Biology, Linker, DNA

Abstract

The E. coli single stranded DNA binding protein (SSB) is essential to all aspects of DNA metabolism. Here, it has two seemingly disparate but equally important roles: it binds rapidly and cooperatively to single stranded DNA (ssDNA) and it binds to partner proteins that constitute the SSB interactome. These two roles are not disparate but are instead, intimately linked. A model is presented wherein the intrinsically disordered linker (IDL) is directly responsible for mediating protein-protein interactions. It does this by binding, via PXXP motifs, to the OB-fold (aka SH3 domain) of a nearby protein. When the nearby protein is another SSB tetramer, this leads to a highly efficient ssDNA binding reaction that rapidly and cooperatively covers and protects the exposed nucleic acid from degradation. Alternatively, when the nearby protein is a member of the SSB interactome, loading of the enzyme onto the DNA takes places.

Published

2017

18. Super-resolution imaging reveals changes inEscherichia coliSSB localization in response to DNA damage

Author

Tianyu Zhao, Juliane Nguyen, Zilin Wang, Yan Liu, Ming Lei, Jia Xiang Zhang, Michael B. Deci, Rongyan He, Feng Xu, and Piero R. Bianco

Subjects

DNA repair, DNA damage, Green Fluorescent Proteins, Biology, medicine.disease_cause, Interactome, Article, 03 medical and health sciences, chemistry.chemical_compound, Genetics, Escherichia coli, medicine, Inner membrane, Single-strand DNA-binding protein, 030304 developmental biology, 0303 health sciences, 030306 microbiology, Escherichia coli Proteins, Cell Membrane, DNA replication, Cell Biology, Recombinant Proteins, DnaA, Cell biology, DNA-Binding Proteins, Cytosol, stomatognathic diseases, Protein Transport, chemistry, Protein Multimerization, Single-Cell Analysis, DNA, DNA Damage

Abstract

TheE. colisingle stranded DNA binding protein (SSB) is essential to viability. It plays key roles in DNA metabolism where it binds to nascent single strands of DNA and to target proteins known as the SSB interactome. There are >2,000 tetramers of SSB per cell with perhaps 100-150 associated with genome at any one time, either at DNA replication forks or at sites of DNA repair. The remaining 1,900 tetramers could constantly diffuse throughout the cytosol or be associated with the inner membrane as observed for other DNA metabolic enzymes such as DnaA and RecA. To visualize SSB directly and to ascertain spatiotemporal changes in tetramer localization in response to DNA damage, SSB-GFP chimeras were visualized using a novel, super-resolution microscope optimized for visualization of prokaryotic cells. Results show that in the absence of DNA damage, SSB localizes to a small number of foci and the excess protein is observed associated with the inner membrane where it binds to the major phospholipids. Within five minutes following DNA damage, the vast majority of SSB disengages from the membrane and is found almost exclusively in the cell interior. Here, it is observed in a large number of foci, in discreet structures or, in diffuse form spread over the genome, thereby enabling repair events. In the process, it may also deliver interactome partners such as RecG or PriA to sites where their repair functions are required.

Published

2019

19. Rep and UvrD Antagonize One Another at Stalled Replication Forks and This Is Exacerbated by SSB

Author

Yi Shi, Xiaoyi Liu, Jiun Xiang Seet, and Piero R. Bianco

Subjects

chemistry.chemical_classification, 0303 health sciences, biology, General Chemical Engineering, ATPase, 030302 biochemistry & molecular biology, DNA replication, Helicase, General Chemistry, Article, Cell biology, lcsh:Chemistry, 03 medical and health sciences, chemistry.chemical_compound, Enzyme, lcsh:QD1-999, chemistry, RNA polymerase, biology.protein, Holliday junction, DNA, 030304 developmental biology

Abstract

The Rep and UvrD DNA helicases are proposed to act at stalled DNA replication forks to facilitate replication restart when RNA polymerase stalls forks. To clarify the role of these DNA helicases in fork rescue, we used a coupled spectrophotometric ATPase assay to determine how they act on model fork substrates. For both enzymes, activity is low on regressed fork structures, suggesting that they act prior to the regression step that generates a Holliday junction. In fact, the preferred cofactors for both enzymes are forks with a gap in the nascent leading strand, consistent with the 3′–5′ direction of translocation. Surprisingly, for Rep, this specificity is altered in the presence of stoichiometric amounts of a single-strand DNA-binding protein (SSB) relative to a fork with a gap in the nascent lagging strand. Even though Rep and UvrD are similar in structure, elevated concentrations of SSB inhibit Rep, but they have little to no effect on UvrD. Furthermore, Rep and UvrD antagonize one another at a fork. This is surprising given that these helicases have been shown to form a heterodimer and are proposed to act together to rescue an RNA polymerase-stalled fork. Consequently, the results herein indicate that although Rep and UvrD can act on similar fork substrates, they cannot function on the same fork simultaneously.

Published

2018

20. Dynamics of the interaction of RecG protein with stalled replication forks

Author

Zhiqiang Sun, Yuri L. Lyubchenko, Piero R. Bianco, Mohtadin Hashemi, and Galina Warren

Subjects

0301 basic medicine, DNA Replication, DNA, Bacterial, Models, Molecular, Dna duplex, Base pair, Bacterial genome size, medicine.disease_cause, Microscopy, Atomic Force, Biochemistry, Article, 03 medical and health sciences, chemistry.chemical_compound, medicine, Escherichia coli, 030102 biochemistry & molecular biology, biology, Chemistry, Escherichia coli Proteins, DNA replication, Helicase, Replication (computing), Cell biology, DNA-Binding Proteins, 030104 developmental biology, Multiprotein Complexes, biology.protein, DNA

Abstract

As a guardian of the bacterial genome, the RecG DNA helicase repairs DNA replication and rescues stalled replication. We applied atomic force microscopy (AFM) to directly visualize dynamics of RecG upon the interaction with replication fork substrates in the presence and absence of SSB using high-speed AFM. We directly visualized that RecG moves back and forth over dozens of base pairs in the presence of SSB. There is no RecG translocation in the absence of SSB. Computational modeling was performed to build models of Escherichia coli RecG in a free state and in complex with the fork. The simulations revealed the formation of complexes of RecG with the fork and identified conformational transitions that may be responsible for RecG remodeling that can facilitate RecG translocation along the DNA duplex. Such complexes do not form with the DNA duplex, which is in line with experimental data. Overall, our results provide mechanistic insights into the modes of interaction of RecG with the replication fork, suggesting a novel role of RecG in the repair of stalled DNA replication forks.

Published

2018

21. SSB binds to the RecG and PriA helicasesin vivoin the absence of DNA

Author

Hui Yin Tan, Cong Yu, Meerim Choi, Christopher S. Cohan, Adam J. Stanenas, Piero R. Bianco, Alicia K. Byrd, and Kevin D. Raney

Subjects

DNA Replication, DNA, Bacterial, 0301 basic medicine, DNA damage, DNA, Single-Stranded, Plasma protein binding, Article, 03 medical and health sciences, chemistry.chemical_compound, stomatognathic system, In vivo, Escherichia coli, Genetics, Inner membrane, 030102 biochemistry & molecular biology, biology, Extramural, Escherichia coli Proteins, Cell Membrane, DNA Helicases, DNA replication, Helicase, Cell Biology, Cell biology, DNA-Binding Proteins, stomatognathic diseases, 030104 developmental biology, Microscopy, Fluorescence, chemistry, biology.protein, DNA, Protein Binding

Abstract

The E. coli single-stranded DNA-binding protein (SSB) binds to the fork DNA helicases RecG and PriA in vitro. Typically for binding to occur, 1.3 M ammonium sulfate must be present, bringing into question the validity of these data as these are non-physiological conditions. To determine whether SSB can bind to these helicases, we examined binding in vivo. First, using fluorescence microscopy, we show that SSB localizes PriA and RecG to the vicinity of the inner membrane in the absence of DNA damage. Localization requires that SSB be in excess over the DNA helicases and the SSB C-terminus and both PriA and RecG be present. Second, using purification of tagged complexes, our results demonstrate that SSB binds to PriA and RecG in vivo, in the absence of DNA. We propose that this may be the “storage form” of RecG and PriA. We further propose that when forks stall, RecG and PriA are targeted to the fork by SSB which, by virtue of its high affinity for single stranded DNA, allows these helicases to out compete other proteins. This ensures their actions in the early stages of the rescue of stalled replication forks.

Published

2016

22. I came to a fork in the DNA and there was RecG

Author

Piero R. Bianco

Subjects

DNA Replication, Models, Molecular, DNA Repair, Protein Conformation, Biophysics, Biology, Article, Fork (software development), chemistry.chemical_compound, ATP hydrolysis, Inner membrane, Molecular Biology, dnaB helicase, chemistry.chemical_classification, Genetics, Escherichia coli Proteins, Helicase, Forkhead Transcription Factors, DNA, Enzyme, Models, Chemical, chemistry, Duplex (building), biology.protein, DNA Damage, Protein Binding

Abstract

RecG is a potent, atypical, monomeric DNA helicase. It simultaneously couples ATP hydrolysis to duplex unwinding and rewinding, and to the displacement of proteins bound to the DNA. A model is presented for the localization of the enzyme to the inner membrane via its binding to SSB. Upon fork stalling, SSB targets the enzyme to the fork where it can act. RecG displays a strong preference for processing the fork in the regression direction, that is, away from the site of damage that initially led to fork arrest. Regression is mediated by strong binding of the wedge domain to the fork arms as well as to parental duplex DNA by the helicase domains. Once RecG has regressed the fork, it will dissociate leaving the now relaxed, Holliday junction-like DNA, available for further processing by enzymes such as RuvAB.

Published

2015

23. Direct AFM Visualization of RecG Translocation after Remodeling by SSB Protein

Author

Yuri L. Lyubchenko, Zhiqiang Sun, Mohtadin Hashemil, and Piero R. Bianco

Subjects

biology, Chemistry, Atomic force microscopy, Biophysics, biology.protein, Chromosomal translocation, Single-stranded binding protein, Visualization

Published

2018

24. PcrA-mediated disruption of RecA nucleoprotein filaments—essential role of the ATPase activity of RecA

Author

Karen R. Thickman, Sanford H. Leuba, Grant D. Schauer, Saleem A. Khan, Matt V. Fagerburg, Syam P. Anand, and Piero R. Bianco

Subjects

ATPase, Mutant, DNA, Single-Stranded, Genome Integrity, Repair and Replication, Biology, Geobacillus stearothermophilus, 03 medical and health sciences, chemistry.chemical_compound, Adenosine Triphosphate, 0302 clinical medicine, Bacterial Proteins, Genetics, Recombinase, Nucleotide, 030304 developmental biology, Adenosine Triphosphatases, chemistry.chemical_classification, 0303 health sciences, DNA Helicases, Helicase, biochemical phenomena, metabolism, and nutrition, PcrA, Nucleoprotein, Cell biology, Adenosine Diphosphate, Protein Transport, Rec A Recombinases, chemistry, Biochemistry, biology.protein, bacteria, 030217 neurology & neurosurgery, DNA

Abstract

The essential DNA helicase, PcrA, regulates recombination by displacing the recombinase RecA from the DNA. The nucleotide-bound state of RecA determines the stability of its nucleoprotein filaments. Using single-molecule fluorescence approaches, we demonstrate that RecA displacement by a translocating PcrA requires the ATPase activity of the recombinase. We also show that in a 'head-on collision' between a polymerizing RecA filament and a translocating PcrA, the RecA K72R ATPase mutant, but not wild-type RecA, arrests helicase translocation. Our findings demonstrate that translocation of PcrA is not sufficient to displace RecA from the DNA and assigns an essential role for the ATPase activity of RecA in helicase-mediated disruption of its filaments.

Published

2012

25. Novel, fluorescent, SSB protein chimeras with broad utility

Author

Christopher S. Cohan, Adam G. Stanenas, Piero R. Bianco, Kevin D. Raney, Meerim Choi, Juan Liu, and Alicia K. Byrd

Subjects

HMG-box, DNA repair, Recombinant Fusion Proteins, DNA, Single-Stranded, Biology, Biochemistry, Article, law.invention, Single-stranded binding protein, chemistry.chemical_compound, law, Escherichia coli, Cloning, Molecular, Molecular Biology, RecBCD, Escherichia coli Proteins, DNA replication, Molecular biology, DNA-Binding Proteins, Luminescent Proteins, stomatognathic diseases, Microscopy, Fluorescence, chemistry, Recombinant DNA, biology.protein, DNA, In vitro recombination, Protein Binding

Abstract

The Escherichia coli single-stranded DNA binding protein (SSB) is a central player in DNA metabolism where it organizes genome maintenance complexes and stabilizes single-stranded DNA (ssDNA) intermediates generated during DNA processing. Due to the importance of SSB and to facilitate real-time studies, we developed a dual plasmid expression system to produce novel, chimeric SSB proteins. These chimeras, which contain mixtures of histidine-tagged and fluorescent protein(FP)-fusion subunits, are easily purified in milligram quantities and used without further modification, a significant enhancement over previous methods to produce fluorescent SSB. Chimeras retain the functionality of wild type in all assays, demonstrating that SSB function is unaffected by the FPs. We demonstrate the power and utility of these chimeras in single molecule studies providing a great level of insight into the biochemical mechanism of RecBCD. We also utilized the chimeras to show for the first time that RecG and SSB interact in vivo. Consequently, we anticipate that the chimeras described herein will facilitate in vivo, in vitro and single DNA molecule studies using proteins that do not require further modification prior to use.

Published

2011

26. Hop2-Mnd1 Condenses DNA to Stimulate the Synapsis Phase of DNA Strand Exchange

Author

Piero R. Bianco, R. Daniel Camerini-Otero, and Roberto J. Pezza

Subjects

Models, Molecular, chemistry.chemical_classification, DNA ligase, DNA clamp, HMG-box, Cations, Divalent, Protein, Biophysics, Cell Cycle Proteins, DNA, Biology, DNA condensation, Molecular biology, Branch migration, DNA-Binding Proteins, Chromosome Pairing, Mice, chemistry, Animals, Humans, Nucleic Acid Conformation, DNA supercoil, Strand invasion, Transcription bubble

Abstract

Hop2-Mnd1 is a meiotic recombination mediator that stimulates DNA strand invasion by both Dmc1 and Rad51. To understand the biochemical mechanism of this stimulation, we directly visualized the heterodimer acting on single molecules of duplex DNA using optical tweezers and video fluorescence microscopy. The results show that the Hop2-Mnd1 heterodimer efficiently condenses double-stranded DNA via formation of a bright spot or DNA condensate. The condensation of DNA is Hop2-Mnd1 concentration-dependent, reversible, and specific to the heterodimer, as neither Hop2 nor Mnd1 acting alone can facilitate this reaction. The results also show that the rate-limiting nucleation step of DNA condensation is overcome in the presence of divalent metal ions, with the following order of preference: Mn2+>Mg2+>Ca2+. Hop2-Mnd1/Dmc1/single-stranded DNA nucleoprotein filaments also condense double-stranded DNA in a heterodimer concentration-dependent manner. Of importance, the concentration dependence parallels that seen in DNA strand exchange. We propose that rapid DNA condensation is a key factor in stimulating synapsis, whereas decondensation may facilitate the invasion step and/or the ensuing branch migration process.

Published

2010

27. RecG interacts directly with SSB: implications for stalled replication fork regression

Author

Yuji Kimura, Jackson Buss, and Piero R. Bianco

Subjects

DNA Replication, DNA, Single-Stranded, Biology, DNA-binding protein, Single-stranded binding protein, chemistry.chemical_compound, Tetramer, Bacterial Proteins, Genetics, Binding site, chemistry.chemical_classification, Adenosine Triphosphatases, Binding Sites, Nucleic Acid Enzymes, Escherichia coli Proteins, DNA replication, DNA Helicases, DNA Replication Fork, Molecular biology, Cell biology, DNA-Binding Proteins, Enzyme, chemistry, biology.protein, DNA, Circular, DNA

Abstract

RecG and RuvAB are proposed to act at stalled DNA replication forks to facilitate replication restart. To define the roles of these proteins in fork regression, we used a combination of assays to determine whether RecG, RuvAB or both are capable of acting at a stalled fork. The results show that RecG binds to the C-terminus of single-stranded DNA binding protein (SSB) forming a stoichiometric complex of 2 RecG monomers per SSB tetramer. This binding occurs in solution and to SSB protein bound to single stranded DNA (ssDNA). The result of this binding is stabilization of the interaction of RecG with ssDNA. In contrast, RuvAB does not bind to SSB. Side-by-side analysis of the catalytic efficiency of the ATPase activity of each enzyme revealed that (-)scDNA and ssDNA are potent stimulators of the ATPase activity of RecG but not for RuvAB, whereas relaxed circular DNA is a poor cofactor for RecG but an excellent one for RuvAB. Collectively, these data suggest that the timing of repair protein access to the DNA at stalled forks is determined by the nature of the DNA available at the fork. We propose that RecG acts first, with RuvAB acting either after RecG or in a separate pathway following protein-independent fork regression.

Published

2008

28. De Novo Design of Protein Mimics of B-DNA

Author

Deniz Yüksel, Piero R. Bianco, and Krishna Kumar

Subjects

0301 basic medicine, Models, Molecular, Base pair, Molecular Sequence Data, Molecular Conformation, Peptide, Cleavage (embryo), Article, Bacteriophage, 03 medical and health sciences, chemistry.chemical_compound, Amino Acid Sequence, Molecular Biology, chemistry.chemical_classification, Genetics, biology, Chemistry, Molecular Mimicry, Deoxyribonucleases, Type I Site-Specific, Proteins, Translation (biology), biology.organism_classification, Cell biology, 030104 developmental biology, Enzyme, DNA, B-Form, Peptides, DNA, Biotechnology, Protein Binding

Abstract

Structural mimicry of DNA is utilized in nature as a strategy to evade molecular defences mounted by host organisms. One such example is the protein Ocr – the first translation product to be expressed as the bacteriophage T7 infects E. coli. The structure of Ocr reveals an intricate and deliberate arrangement of negative charges that endows it with the ability to mimic ∼24 base pair stretches of B-DNA. This uncanny resemblance to DNA enables Ocr to compete in binding the type I restriction modification (R/M) system, and neutralizes the threat of hydrolytic cleavage of viral genomic material. Here, we report the de novo design and biophysical characterization of DNA mimicking peptides, and describe the inhibitory action of the designed helical bundles on a type I R/M enzyme, EcoR124I. This work validates the use of charge patterning as a design principle for creation of protein mimics of DNA, and serves as a starting point for development of therapeutic peptide inhibitors against human pathogens that employ molecular camouflage as part of their invasion stratagem.

Published

2016

29. Rad54 Oligomers Translocate and Cross-bridge Double-stranded DNA to Stimulate Synapsis

Author

Lauren R. Castanza, Piero R. Bianco, Justin J. Bradfield, and Andrea N. Donnelly

Subjects

Base pair, Biology, Article, Adenosine Triphosphate, Biopolymers, Structural Biology, Humans, Protein–DNA interaction, Molecular Biology, Replication protein A, Glutathione Transferase, chemistry.chemical_classification, DNA ligase, DNA clamp, Hydrolysis, Circular bacterial chromosome, fungi, DNA Helicases, DNA replication, Nuclear Proteins, DNA, DNA-Binding Proteins, Chromosome Pairing, Protein Transport, Microscopy, Fluorescence, chemistry, Biochemistry, Biophysics, DNA supercoil

Abstract

Rad54 is a key component of the eukaryotic recombination machinery. Its presence in DNA strand-exchange reactions in vitro results in a significant stimulation of the overall reaction rate. Using untagged Rad54, we show that this stimulation can be attributed to enhancement of the formation of a key reaction intermediate known as DNA networks. Using a novel, single DNA molecule, dual-optical tweezers approach we show how Rad54 stimulates DNA network formation. We discovered that Rad54 oligomers possess a unique ability to cross-bridge or bind double-stranded DNA molecules positioned in close proximity. Further, Rad54 oligomers rapidly translocate double-stranded DNA while simultaneously inducing topological loops in the DNA at the locus of the oligomer. The combination of the cross-bridging and double-stranded DNA translocation activities of Rad54 stimulates the formation of DNA networks, leading to rapid and efficient DNA strand exchange by Rad51.

Published

2007

30. Novel, Monomeric Cyanine Dyes as Reporters for DNA Helicase Activity

Author

Sarah McClelland, D. V. Kryvorotenko, Cuiling Xu, Piero R. Bianco, Vladyslava B. Kovalska, Mykhaylo Yu. Losytskyy, and Sergiy M. Yarmoluk

Subjects

Magnetic Resonance Spectroscopy, Sociology and Political Science, Clinical Biochemistry, DNA, Single-Stranded, Binding, Competitive, Biochemistry, chemistry.chemical_compound, Magnesium, Cyanine, Spectroscopy, Fluorescent Dyes, RecBCD, Benzoxazoles, biology, Quinolinium Compounds, DNA Helicases, Helicase, DNA, Carbocyanines, Fluorescence, Kinetics, Thiazoles, Clinical Psychology, DNA helicase activity, Spectrometry, Fluorescence, chemistry, biology.protein, Biophysics, Ethidium homodimer assay, Law, YOYO-1, Social Sciences (miscellaneous)

Abstract

The dimeric cyanine dyes, YOYO-1 and TOTO-1, are widely used as DNA probes because of their excellent fluorescent properties. They have a higher fluorescence quantum yield than ethidium homodimer, DAPI and Hoechst dyes and bind to double-stranded DNA with high affinity. However, these dyes are limited by heterogeneous staining at high dye loading, photocleavage of DNA under extended illumination, nicking of DNA, and inhibition of the activity of DNA binding enzymes. To overcome these limitations, seven novel cyanine dyes (Cyan-2, DC-21, DM, DM-1, DMB-2OH, SH-0367, SH1015-OH) were synthesized and tested for fluorescence emission, resistance to displacement by Mg(2+), and the ability to function as reporters for DNA unwinding. Results show that Cyan-2, DM-1, SH-0367 and SH1015-OH formed highly fluorescent complexes with dsDNA. Of these, only Cyan-2 and DM-1 exhibited a large fluorescence enhancement in buffers, and were resistant to displacement by Mg(2+). The potential of these two dyes to function as reporter molecules was evaluated using continuous fluorescence, DNA helicase assays. The rate of DNA unwinding was not significantly affected by either of these two dyes. Therefore, Cyan-2 and DM-1 form the basis for the synthesis of novel cyanine dyes with the potential to overcome the limitations of YOYO-1 and TOTO-1.

Published

2007

31. DNA Helicase Activity of PcrA Is Not Required for the Displacement of RecA Protein from DNA or Inhibition of RecA-Mediated Strand Exchange

Author

Haocheng Zheng, Piero R. Bianco, Syam P. Anand, Sanford H. Leuba, and Saleem A. Khan

Subjects

DNA, Bacterial, Mutant, DNA, Single-Stranded, Gram-Positive Bacteria, medicine.disease_cause, Microbiology, law.invention, chemistry.chemical_compound, Bacterial Proteins, law, Fluorescence Resonance Energy Transfer, medicine, Translocase, Molecular Biology, Recombination, Genetic, Mutation, biology, DNA Helicases, Helicase, biochemical phenomena, metabolism, and nutrition, PcrA, Enzymes and Proteins, Molecular biology, Rec A Recombinases, DNA helicase activity, chemistry, Recombinant DNA, biology.protein, Biophysics, bacteria, DNA

Abstract

PcrA is a conserved DNA helicase present in all gram-positive bacteria. Bacteria lacking PcrA show high levels of recombination. Lethality induced by PcrA depletion can be overcome by suppressor mutations in the recombination genes recFOR . RecFOR proteins load RecA onto single-stranded DNA during recombination. Here we test whether an essential function of PcrA is to interfere with RecA-mediated DNA recombination in vitro. We demonstrate that PcrA can inhibit the RecA-mediated DNA strand exchange reaction in vitro. Furthermore, PcrA displaced RecA from RecA nucleoprotein filaments. Interestingly, helicase mutants of PcrA also displaced RecA from DNA and inhibited RecA-mediated DNA strand exchange. Employing a novel single-pair fluorescence resonance energy transfer-based assay, we demonstrate a lengthening of double-stranded DNA upon polymerization of RecA and show that PcrA and its helicase mutants can reverse this process. Our results show that the displacement of RecA from DNA by PcrA is not dependent on its translocase activity. Further, our results show that the helicase activity of PcrA, although not essential, might play a facilitatory role in the RecA displacement reaction.

Published

2007

32. Studies on New Synthetic Antiviral Drugs, Ketoaldehydic Derivatives of Biphenyl: Virological Aspects in Experimental and Clinical Fields

Author

F. Magrassi, F. Coraggio, Sapio U, A. R. Bianco, V. Villari, Gabriele Mazzacca, M. Coltorti, V. Pecori, Altucci P, A. Di Simone, and Lorenzutti G

Subjects

Biphenyl, chemistry.chemical_compound, Antiviral chemotherapy, chemistry, business.industry, Medicine, Pharmacology, business

Published

2015

33. Inhibition of RecBCD Enzyme by Antineoplastic DNA Alkylating Agents

Author

Terry A. Beerman, Barbara Dziegielewska, and Piero R. Bianco

Subjects

Models, Molecular, Exodeoxyribonuclease V, Indoles, Cyclohexanecarboxylic Acids, Anthraquinones, Catalysis, Fluorescence, Duocarmycins, chemistry.chemical_compound, Adenosine Triphosphate, Structural Biology, Cyclohexenes, Escherichia coli, A-DNA, Antineoplastic Agents, Alkylating, Molecular Biology, Benzofurans, Recombination, Genetic, RecBCD, chemistry.chemical_classification, Nuclease, biology, Hydrolysis, DNA Helicases, Helicase, DNA, DNA Alkylation, Enzyme, chemistry, Adozelesin, Biochemistry, biology.protein, Nucleic Acid Conformation, Allosteric Site

Abstract

To understand how bulky adducts might perturb DNA helicase function, three distinct DNA-binding agents were used to determine the effects of DNA alkylation on a DNA helicase. Adozelesin, ecteinascidin 743 (Et743) and hedamycin each possess unique structures and sequence selectivity. They bind to double-stranded DNA and alkylate one strand of the duplex in cis, adding adducts that alter the structure of DNA significantly. The results show that Et743 was the most potent inhibitor of DNA unwinding, followed by adozelesin and hedamycin. Et743 significantly inhibited unwinding, enhanced degradation of DNA, and completely eliminated the ability of the translocating RecBCD enzyme to recognize and respond to the recombination hotspot χ. Unwinding of adozelesin-modified DNA was accompanied by the appearance of unwinding intermediates, consistent with enzyme entrapment or stalling. Further, adozelesin also induced “apparent” χ fragment formation. The combination of enzyme sequestering and pseudo-χ modification of RecBCD, results in biphasic time-courses of DNA unwinding. Hedamycin also reduced RecBCD activity, albeit at increased concentrations of drug relative to either adozelesin or Et743. Remarkably, the hedamycin modification resulted in constitutive activation of the bottom-strand nuclease activity of the enzyme, while leaving the ability of the translocating enzyme to recognize and respond to χ largely intact. Finally, the results show that DNA alkylation does not significantly perturb the allosteric interaction that activates the enzyme for ATP hydrolysis, as the efficiency of ATP utilization for DNA unwinding is affected only marginally. These results taken together present a unique response of RecBCD enzyme to bulky DNA adducts. We correlate these effects with the recently determined crystal structure of the RecBCD holoenzyme bound to DNA.

Published

2006

34. A Molecular Throttle

Author

Naofumi Handa, Maria Spies, Mark S. Dillingham, Ronald J. Baskin, Stephen C. Kowalczykowski, and Piero R. Bianco

Subjects

chemistry.chemical_classification, RecBCD, 0303 health sciences, Nuclease, Recombination hotspot, biology, Biochemistry, Genetics and Molecular Biology(all), Helicase, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Enzyme, chemistry, Biochemistry, Biophysics, biology.protein, bacteria, Translocase, Homologous recombination, 030217 neurology & neurosurgery, DNA, 030304 developmental biology

Abstract

RecBCD enzyme is a heterotrimeric helicase/nuclease that initiates homologous recombination at double-stranded DNA breaks. Several of its activities are regulated by the DNA sequence χ (5′-GCTGGTGG-3′), which is recognized in cis by the translocating enzyme. When RecBCD enzyme encounters χ, the intensity and polarity of its nuclease activity are changed, and the enzyme gains the ability to load RecA protein onto the χ-containing, unwound single-stranded DNA. Here, we show that interaction with χ also affects translocation by RecBCD enzyme. By observing translocation of individual enzymes along single molecules of DNA, we could see RecBCD enzyme pause precisely at χ. Furthermore, and more unexpectedly, after pausing at χ, the enzyme continues translocating but at approximately one-half the initial rate. We propose that interaction with χ results in an enzyme in which one of the two motor subunits, likely the RecD motor, is uncoupled from the holoenzyme to produce the slower translocase.

Published

2003

35. Remodeling of RecG Helicase at the DNA Replication Fork by SSB Protein

Author

Yuri L. Lyubchenko, Hui Yin Tan, Piero R. Bianco, and Zhiqiang Sun

Subjects

Genetics, DNA Replication, Multidisciplinary, Dna duplex, Binding Sites, biology, Escherichia coli Proteins, DNA replication, DNA Helicases, Helicase, DNA, Single-Stranded, DNA Replication Fork, DNA-binding protein, Article, Cell biology, Single-stranded binding protein, DNA-Binding Proteins, chemistry.chemical_compound, stomatognathic diseases, chemistry, biology.protein, Escherichia coli, Binding site, DNA

Abstract

The RecG DNA helicase a key player in stalled replication fork rescue. The single-stranded DNA binding protein (SSB) participates in this process, but its role in the interaction of RecG with the fork remains unclear. We used atomic force microscopy (AFM) to visualize the interaction of RecG with a fork DNA in the presence of SSB. We discovered that SSB enhances RecG loading efficiency onto the DNA fork by threefold. Additionally, SSB interacts with RecG leading to the RecG remodeling. As a result, RecG separates from the fork, but remains bound to the DNA duplex. Moreover, in this new binding mode RecG is capable of translocation along the parental duplex DNA. We propose a model of RecG interaction with the replication fork involving two RecG binding modes. SSB plays the role of a remodeling factor defining the mode of RecG binding to the fork mediated by the SSB C-terminus. In the translocating mode, RecG remains in the vicinity of the fork and is capable of initiating the fork regression. Our results afford novel mechanistic insights into RecG interaction with the replication fork and provide the basis for further structural studies.

Published

2014

36. Translocation step size and mechanism of the RecBC DNA helicase

Author

Piero R. Bianco and Stephen C. Kowalczykowski

Subjects

DNA, Bacterial, RecBCD, Exodeoxyribonuclease V, Multidisciplinary, DNA clamp, biology, Heparin, DNA polymerase, Base pair, Escherichia coli Proteins, Circular bacterial chromosome, DNA Helicases, DNA, Single-Stranded, Helicase, Substrate Specificity, chemistry.chemical_compound, Exodeoxyribonucleases, chemistry, Biochemistry, Escherichia coli, biology.protein, Biophysics, DNA polymerase I, DNA

Abstract

DNA helicases are ubiquitous enzymes that unwind double-stranded DNA. They are a diverse group of proteins that move in a linear fashion along a one-dimensional polymer lattice--DNA--by using a mechanism that couples nucleoside triphosphate hydrolysis to both translocation and double-stranded DNA unwinding to produce separate strands of DNA. The RecBC enzyme is a processive DNA helicase that functions in homologous recombination in Escherichia coli; it unwinds up to 6,250 base pairs per binding event and hydrolyses slightly more than one ATP molecule per base pair unwound. Here we show, by using a series of gapped oligonucleotide substrates, that this enzyme translocates along only one strand of duplex DNA in the 3'-->5' direction. The translocating enzyme will traverse, or 'step' across, single-stranded DNA gaps in defined steps that are 23 (+/-2) nucleotides in length. This step is much larger than the amount of double-stranded DNA that can be unwound using the free energy derived from hydrolysis of one molecule of ATP, implying that translocation and DNA unwinding are separate events. We propose that the RecBC enzyme both translocates and unwinds by a quantized, two-step, inchworm-like mechanism that may have parallels for translocation by other linear motor proteins.

Published

2000

37. ABRINDO A CAIXA DE PANDORA DOS NANOMEDICAMENTOS: HÁ REALMENTE MUITO MAIS ‘ESPAÇO LÁ EMBAIXO’

Author

Alexsandra Conceição Apolinário, Giovanna Cassone Salata, Arthur F. R. Bianco, Claudio Fukumori, and Luciana Biagini Lopes

Subjects

nanocarriers, nanomedicine, biological barriers, nanopharmacology, Chemistry, QD1-999

Abstract

Limitations of conventional treatment and dosage forms prompted the investigation of novel approaches that combine efficacy, selectivity and fewer adverse effects. These are the main promises of nanomedicine, generally defined as the application of nanotechnology to the biomedical field. Despite the considerable advances over the years and the large number of publications resulting from the growth of nanomedicine, there are still many hurdles and unknown factors limiting its successful translation from promise to reality. These factors range from the lack of standardization in the terminology and regulations, to the lack of understanding of interactions between nanocarriers and the biological system, and their influence on drug pharmacodynamics. In this manuscript, we aim at presenting and discussing concepts and terminologies used in the nanomedicine field and examining the main types of nanocarriers and their effects to modulate biological barriers and aid drug transport, bioavailability and targeting.

38. ATP binding and hydrolysis by Saccharomyces cerevisiae Msh2-Msh3 are differentially modulated by mismatch and double-strand break repair DNA substrates

Author

Jennifer A. Surtees, Piero R. Bianco, Gregory M. Williams, Bangchen Wang, Robin Eichmiller, and Charanya Kumar

Subjects

congenital, hereditary, and neonatal diseases and abnormalities, Saccharomyces cerevisiae Proteins, Saccharomyces cerevisiae, Biology, Biochemistry, DNA Mismatch Repair, Article, Substrate Specificity, chemistry.chemical_compound, Adenosine Triphosphate, ATP hydrolysis, Catalytic Domain, Nucleotide, DNA Breaks, Double-Stranded, DNA, Fungal, Molecular Biology, chemistry.chemical_classification, Hydrolysis, nutritional and metabolic diseases, Cell Biology, Double Strand Break Repair, digestive system diseases, DNA-Binding Proteins, Kinetics, MutS Homolog 2 Protein, Phenotype, chemistry, MSH3, MSH2, MutS Homolog 3 Protein, Mutation, DNA mismatch repair, Adenosine triphosphate, DNA

Abstract

In Saccharomyces cerevisiae, Msh2-Msh3-mediated mismatch repair (MMR) recognizes and targets insertion/deletion loops for repair. Msh2-Msh3 is also required for 3′ non-homologous tail removal (3′NHTR) in double-strand break repair. In both pathways, Msh2-Msh3 binds double-strand/single-strand junctions and initiates repair in an ATP-dependent manner. However, we recently demonstrated that the two pathways have distinct requirements with respect to Msh2-Msh3 activities. We identified a set of aromatic residues in the nucleotide binding pocket (FLY motif) of Msh3 that, when mutated, disrupted MMR, but left 3′ NHTR largely intact. One of these mutations, msh3Y942A, was predicted to disrupt the nucleotide sandwich and allow altered positioning of ATP within the pocket. To develop a mechanistic understanding of the differential requirements for ATP binding and/or hydrolysis in the two pathways, we characterized Msh2-Msh3 and Msh2-msh3Y942A ATP binding and hydrolysis activities in the presence of MMR and 3′ NHTR DNA substrates. We observed distinct, substrate-dependent ATP hydrolysis and nucleotide turnover by Msh2-Msh3, indicating that the MMR and 3′ NHTR DNA substrates differentially modify the ATP binding/hydrolysis activities of Msh2-Msh3. Msh2-msh3Y942A retained the ability to bind DNA and ATP but exhibited altered ATP hydrolysis and nucleotide turnover. We propose that both ATP and structure-specific repair substrates cooperate to direct Msh2-Msh3-mediated repair and suggest an explanation for the msh3Y942A separation-of-function phenotype.

Published

2013

39. Characterization of the ATPase activity of RecG and RuvAB proteins on model fork structures reveals insight into stalled DNA replication fork repair

Author

Syafiq Abd Wahab, Meerim Choi, and Piero R. Bianco

Subjects

DNA Replication, DNA Repair, DNA repair, DNA, Single-Stranded, DNA and Chromosomes, Biochemistry, DNA-binding protein, Substrate Specificity, chemistry.chemical_compound, Bacterial Proteins, Holliday junction, Escherichia coli, Protein–DNA interaction, Molecular Biology, Adenosine Triphosphatases, DNA, Cruciform, Binding Sites, biology, Escherichia coli Proteins, Hydrolysis, DNA replication, DNA Helicases, Helicase, Cell Biology, DNA Replication Fork, Molecular biology, Cell biology, chemistry, biology.protein, DNA, Bacteriophage M13, Protein Binding

Abstract

RecG and RuvAB are proposed to act at stalled DNA replication forks to facilitate replication restart. To clarify the roles of these proteins in fork regression, we used a coupled spectrophotometric ATPase assay to determine how these helicases act on two groups of model fork substrates: the first group mimics nascent stalled forks, whereas the second mimics regressed fork structures. The results show that RecG is active on the substrates in group 1, whereas these are poor substrates for RuvAB. In addition, in the presence of group 1 forks, the single-stranded DNA-binding protein (SSB) enhances the activity of RecG and enables it to compete with excess RuvA. In contrast, SSB inhibits the activity of RuvAB on these substrates. Results also show that the preferred regressed fork substrate for RuvAB is a Holliday junction, not a forked DNA. The active form of the enzyme on the Holliday junction contains a single RuvA tetramer. In contrast, although the enzyme is active on a regressed fork structure, RuvB loading by a single RuvA tetramer is impaired, and full activity requires the cooperative binding of two forked DNA substrate molecules. Collectively, the data support a model where RecG is responsible for stalled DNA replication fork regression. SSB ensures that if the nascent fork has single-stranded DNA character RuvAB is inhibited, whereas the activity of RecG is preferentially enhanced. Only once the fork has been regressed and the DNA is relaxed can RuvAB bind to a RecG-extruded Holliday junction. Background: DNA replication fork rescue requires the action of DNA helicases to regress the fork. Results: RecG is more active than RuvAB on substrates that mimic nascent stalled forks, whereas RuvAB is active on Holliday junctions. Conclusion: RecG in concert with SSB regresses stalled DNA replication forks, producing DNA substrates to which RuvAB can bind. Significance: RecG, not RuvAB, regresses stalled DNA replication forks.

Published

2013

40. Helicase Unwinding: Active or Merely Perfect?

Author

Piero R. Bianco and Martin R. Webb

Subjects

Base Composition, biology, Chemistry, DNA Helicases, Nucleic Acid Heteroduplexes, Oligonucleotides, Helicase, DNA, Single-Stranded, Computational biology, Article, Protein Transport, Viral Proteins, Structural Biology, biology.protein, DNA, Circular, Molecular Biology

Abstract

Helicases utilize the energy of ATP hydrolysis to unwind double-stranded DNA while translocating on the DNA. Mechanisms for melting the duplex have been characterized as active or passive, depending on whether the enzyme actively separates the base pairs or simply sequesters single-stranded DNA (ssDNA) that forms due to thermal fraying. Here, we show that Dda translocates unidirectionally on ssDNA at the same rate at which it unwinds double-stranded DNA in both ensemble and single-molecule experiments. Further, the unwinding rate is largely insensitive to the duplex stability and to the applied force. Thus, Dda transduces all of its translocase activity into DNA unwinding activity so that the rate of unwinding is limited by the rate of translocation and that the enzyme actively separates the duplex. Active and passive helicases have been characterized by dividing the velocity of DNA unwinding in base pairs per second (V(un)) by the velocity of translocation on ssDNA in nucleotides per second (V(trans)). If the resulting fraction is 0.25, then a helicase is considered to be at the lower end of the "active" range. In the case of Dda, the average DNA unwinding velocity was 257±42 bp/s, and the average translocation velocity was 267±15 nt/s. The V(un)/V(trans) value of 0.96 places Dda in a unique category of being an essentially "perfectly" active helicase.

Published

2012

41. Fluorescent Single-Stranded DNA-Binding Proteins Enable In Vitro and In Vivo Studies

Author

Juan Liu, Piero R. Bianco, Christopher S. Cohan, and Adam J. Stanenas

Subjects

DNA repair, Chemistry, Recombinant Fusion Proteins, DNA replication, Fluorescence, Chromatography, Affinity, Article, eye diseases, In vitro, DNA-Binding Proteins, Single-Stranded DNA Binding Proteins, stomatognathic diseases, Spectrometry, Fluorescence, Biochemistry, Tetramer, In vivo, Fluorescence microscope, Molecular Biology, Fluorescent Dyes

Abstract

Fluorescent single-stranded DNA-binding proteins (SSB) that have a defined number of fluorophores per tetramer are invaluable tools to understand biochemical mechanism and biological function. Here, we describe the purification of fluorescent SSB chimeras with a unique number of fluorescent subunits incorporated per tetramer. We describe the use of these tetramers to enable clear visualization of SSB in vivo. Purified chimeras also facilitate single molecule studies (Liu et al., Protein Sci 20:1005–1020, 2011).

Published

2012

42. RecG Interaction with the DNA Replication Fork. The Role of E. coli SSB Protein

Author

Piero R. Bianco, Yuri L. Lyubchenko, Hui Yin Tan, and Zhiqiang Sun

Subjects

biology, DNA repair, Mutant, Biophysics, DNA replication, Helicase, DNA Replication Fork, Molecular biology, eye diseases, Single-stranded binding protein, stomatognathic diseases, chemistry.chemical_compound, stomatognathic system, chemistry, biology.protein, skin and connective tissue diseases, DNA, Single-strand DNA-binding protein

Abstract

The RecG DNA helicase is a guardian of the bacterial genome. It binds to a variety of forked DNA structures thereby minimizing pathological DNA replication and facilitating stalled replication fork rescue. It is becomingly increasingly clear that SSB plays a critical role in the function of RecG, but the mechanisms of its interaction with SSB remain unclear. Here we use the atomic force microscope (AFM) to image the structure of RecG with a model fork substrate in the presence or absence of the single strand DNA binding protein (SSB). The DNA substrate has a 3′-end 69nt single stranded DNA (ssDNA) segment inserted between the two DNA duplexes. This design mimics a stalled fork with an ssDNA gap in the leading strand. The SSB proteins bind very specifically to the ssDNA segment with a yield of ∼90%. RecG protein also binds to the fork but the yield was ∼10%. However, the RecG loading on the same substrate increases three-fold in the presence of SSB suggesting that SSB facilitates RecG loading onto the fork. Moreover, in the presence of SSB, RecG becomes capable of translocating along the DNA duplex in an ATP hydrolysis-independent manner. No such mobility of RecG was observed in the absence of SSB. The preferable translocation direction is moving of RecG along parental arm which implies RecG could clear obstacles bound ahead of the fork. This novel activity of SSB requires the SSB C-terminus as a truncated SSB mutant does not substitute for wild type. SSB loading of RecG and subsequent translocation are unaffected by ATP, ADP or the non-hydrolyzable analog ATP-γ-S. Overall the results obtained reveal novel properties of RecG and highlight a new chaperone-type role of SSB in the DNA repair process.

Published

2015

43. Molecular reactivity in solution. Modelling of the effects of the solvent and of its stochastic fluctuation on an SN2 reaction

Author

R. Bianco, Maurizio Persico, Jacopo Tomasi, and S. Miertus

Subjects

Physics::Biological Physics, Quantitative Biology::Biomolecules, Reaction mechanism, Chemistry, General Physics and Astronomy, Thermodynamics, Polarizable continuum model, Condensed Matter::Soft Condensed Matter, Solvent, Reaction rate constant, Reaction dynamics, SN2 reaction, Physical chemistry, Physics::Chemical Physics, Physical and Theoretical Chemistry, Solvent effects, Chemical equilibrium

Abstract

The polarizable continuum model - used up to date to evaluate the effects of a solvent in equilibrium - has been modified to take into account the local fluctuations on the solvent. The elaborated modified model has been applied for the study of the S N 2 type reaction F − +CH 3 F→FCH 3 +F − . The reaction profiles and hypersurfaces have been calculated for this system being an equilibrium solvent as well as in solvent with various simulated fluctuations. It was found, that a fluctuation of the solvent occurring at the F − side can decrease the energy barrier up to 50% of its value in equilibrium solvent. The shape of the reaction hypersurface is also changed by solvent fluctuation - shifting the transition state towards reactants or products, according to the position at which the fluctuation occurs. The study was supplemented by the evaluation of trajectories for both cases, i.e. reaction in equilibrium as well as with a fluctuation in the solvent. The reaction dynamics is substantially altered by the presence of a fluctuation.

Published

1992

44. Type I restriction endonucleases are true catalytic enzymes

Author

Min Chi, Cuiling Xu, and Piero R. Bianco

Subjects

Restriction fragment, 03 medical and health sciences, chemistry.chemical_compound, Restriction map, Recognition sequence, Terminology as Topic, Enzyme Stability, Genetics, Flap endonuclease, 030304 developmental biology, 0303 health sciences, biology, Nucleic Acid Enzymes, 030302 biochemistry & molecular biology, Deoxyribonucleases, Type I Site-Specific, Nucleosides, DNA, DNA binding site, Restriction site, Restriction enzyme, Biochemistry, chemistry, biology.protein, Biocatalysis, Protein Multimerization, Holoenzymes, Protein Binding

Abstract

Type I restriction endonucleases are intriguing, multifunctional complexes that restrict DNA randomly, at sites distant from the target sequence. Restriction at distant sites is facilitated by ATP hydrolysis-dependent, translocation of double-stranded DNA towards the stationary enzyme bound at the recognition sequence. Following restriction, the enzymes are thought to remain associated with the DNA at the target site, hydrolyzing copious amounts of ATP. As a result, for the past 35 years type I restriction endonucleases could only be loosely classified as enzymes since they functioned stoichiometrically relative to DNA. To further understand enzyme mechanism, a detailed analysis of DNA cleavage by the EcoR124I holoenzyme was done. We demonstrate for the first time that type I restriction endonucleases are not stoichiometric but are instead catalytic with respect to DNA. Further, the mechanism involves formation of a dimer of holoenzymes, with each monomer bound to a target sequence and, following cleavage, each dissociates in an intact form to bind and restrict subsequent DNA molecules. Therefore, type I restriction endonucleases, like their type II counterparts, are true enzymes. The conclusion that type I restriction enzymes are catalytic relative to DNA has important implications for the in vivo function of these previously enigmatic enzymes.

Published

2009

45. Laminar flow cells for single-molecule studies of DNA-protein interactions

Author

Laurence R. Brewer and Piero R. Bianco

Subjects

Materials science, Surface Properties, Microfluidics, Protein dna, Flow cell, Biosensing Techniques, Microscopy, Atomic Force, Biochemistry, Models, Biological, Article, chemistry.chemical_compound, Molecule, Molecular Biology, Nuclear Lamina, Proteins, Laminar flow, Cell Biology, DNA, Microfluidic Analytical Techniques, chemistry, Flow (mathematics), Microscopy, Fluorescence, Temporal resolution, Biophysics, Biotechnology, Protein Binding

Abstract

Microfluidic flow cells are used in single-molecule experiments, enabling measurements to be made with high spatial and temporal resolution. We discuss the fundamental processes affecting flow cell operation and describe the flow cells in use at present for studying the interaction of optically trapped or mechanically isolated, single DNA molecules with proteins. To assist the experimentalist in flow cell selection, we review the construction techniques and materials used to fabricate both single- and multiple-channel flow cells and the advantages of each design for different experiments.

Published

2008

46. Characterization of the ATPase activity of the Escherichia coli RecG protein reveals that the preferred cofactor is negatively supercoiled DNA

Author

Jackson Buss, Yuji Kimura, Stephen L. Slocum, and Piero R. Bianco

Subjects

Replication fork reversal, DNA, Bacterial, Poly T, DNA repair, DNA gyrase, Models, Biological, Article, Substrate Specificity, chemistry.chemical_compound, Adenosine Triphosphate, Structural Biology, Escherichia coli, Magnesium, Molecular Biology, Adenosine Triphosphatases, Binding Sites, biology, Base Sequence, DNA, Superhelical, Heparin, Topoisomerase, Escherichia coli Proteins, Hydrolysis, DNA Helicases, Helicase, Processivity, DNA-Binding Proteins, Kinetics, Biochemistry, chemistry, biology.protein, DNA supercoil, Nucleic Acid Conformation, DNA

Abstract

RecG is a member of the superfamily 2 helicase family. Its possible role in vivo is ATP hydrolysis driven regression of stalled replication forks. To gain mechanistic insight into how this is achieved, a coupled spectrophotometric assay was utilized to characterize the ATPase activity of RecG in vitro. The results demonstrate an overwhelming preference for negatively supercoiled DNA ((-)scDNA) as a cofactor for the hydrolysis of ATP. In the presence of (-)scDNA the catalytic efficiency of RecG and the processivity (as revealed through heparin trapping), were higher than on any other cofactor examined. The activity of RecG on (-)scDNA was not due to the presence of single-stranded regions functioning as loading sites for the enzyme as relaxed circular DNA treated with DNA gyrase, resulted in the highest levels of ATPase activity. Relaxation of (-)scDNA by a topoisomerase resulted in a 12-fold decrease in ATPase activity, comparable to that observed on both linear double-stranded (ds)DNA and (+)scDNA. In addition to the elevated activity in the presence of (-)scDNA, RecG also has high activity on model 4Y-substrates (i.e. chicken foot structures). This is due largely to the high apparent affinity of the enzyme for this DNA substrate, which is 46-fold higher than a 2Y-substrate (i.e. a three-way with two single-stranded (ss)DNA arms). Finally, the enzyme exhibited significant, but lower activity on ssDNA. This activity was enhanced by the Escherichia coli stranded DNA-binding protein (SSB) protein, which occurs through stabilizing of the binding of RecG to ssDNA. Stabilization is not afforded by the bacteriophage gene 32 protein, indicating a species specific, protein-protein interaction is involved. These results combine to provide significant insight into the manner and timing of the interaction of RecG with DNA at stalled replication forks.

Published

2007

47. Modulation of the Immune Response Using Dendritic Cell-Derived Exosomes

Author

Paul D. Robbins, Adrian E. Morelli, Seon Hee Kim, and Nicole R. Bianco

Subjects

medicine.diagnostic_test, Chemistry, Arthritis, Interleukin, Inflammation, Dendritic cell, medicine.disease, Microvesicles, Fas ligand, Cell biology, Flow cytometry, Immune system, medicine, medicine.symptom

Abstract

Initial studies in our laboratory were focused on the use of dendritic cells (DC) genetically modified to express Th2-derived cytokines (i.e., interleukin [IL]-4 and IL-10) or apoptotic proteins (i.e., Fas Ligand [FasL]) to reduce inflammation in a mouse model of experimentally induced arthritis. Exosomes are nano-sized vesicles (40-100 nm diameter) released by different cell types, including DC, that contain many of the proteins thought to be involved in regulating the immune response. We have demonstrated that exosomes derived from immature DC treated with immunomodulatory cytokines (i.e., IL-10, IL-4) are able to inhibit inflammation in a murine footpad model of delayed-type hypersensitivity (DTH) and reduce the severity of established collagen-induced arthritis (CIA). In fact, the exosomes were as therapeutic as the parental DC. Because purified DC-derived exosomes are very stable vesicles, they may be a better approach for future treatment of arthritis and other autoimmune disorders than the more unstable DC. In this chapter we detail a protocol for preparing the exosomes produced by murine bone marrow-derived DC. We also review methods to assess the purity and concentration of purified exosomes, by using electron microscopy, Western blot analysis, and flow cytometry. Finally, we describe methods to assess the function of exosomes in vitro, using the mixed leukocytes reaction, and in vivo by means of DTH and an experimental model of CIA.

Published

2007

48. Thermo-Structural Analysis of Ceramic Vanes for Gas Turbines

Author

Giuseppe Pasquero, L. De Lorenzis, Maurizio Fersini, Giovanni Paolo Zanon, R. Bianco, and Antonio Licciulli

Subjects

Materials science, Weibull modulus, Reaction bonded silicon carbide, Turbine, Thermal expansion, chemistry.chemical_compound, Thermal conductivity, chemistry, Silicon nitride, visual_art, Heat transfer, visual_art.visual_art_medium, Ceramic, Composite material

Abstract

Advanced structural ceramics such as Hot Pressed Silicon Nitride (HPSN) and Reaction Bonded Silicon Carbide (RBSC), thanks to their low density (3.1 ÷ 3.4 gr/cm3) and to their thermostructural properties, are interesting candidates for aerospace applications. This research investigates the feasibility of employing such monolithic advanced ceramics for the production of turbine vanes for aerospace applications, by means of a finite element analysis. A parametric study is performed to analyse the influence of the coefficient of thermal expansion, the specific heat, the thermal conductivity, and the Weibull modulus on structural stability, heat transfer properties and thermomechanical stresses under take-off and flying conditions. A nodal point that is evidenced is the high intensity of thermal stresses on the vane, both on steady state and in transient conditions. In order to reduce such stresses various simulations have been carried out varying geometrical parameters such as the wall thickness. Several open questions are evidenced and guidelines are drawn for the design and production of ceramic vanes for gas turbines.

Published

2006

49. The type I restriction endonuclease EcoR124I, couples ATP hydrolysis to bidirectional DNA translocation

Author

Piero R. Bianco and Elizabeth M. Hurley

Subjects

RecBCD, Adenosine Triphosphatases, DNA clamp, Exodeoxyribonuclease V, Models, Genetic, Circular bacterial chromosome, Escherichia coli Proteins, Deoxyribonucleases, Type I Site-Specific, Processivity, DNA, Biology, Restriction enzyme, chemistry.chemical_compound, Protein Subunits, Adenosine Triphosphate, Biochemistry, Recognition sequence, chemistry, Structural Biology, Biophysics, DNA supercoil, Magnesium, Molecular Biology

Abstract

Type I restriction endonuclease holoenzymes contain methylase (M), restriction (R) and specificity (S) subunits, present in an M2:R2:S1 stoichiometry. These enzymes bind to specific DNA sequences and translocate dsDNA in an ATP-dependent manner toward the holoenzyme anchored at the recognition sequence. Once translocation is impeded, DNA restriction, which functions to protect the host cell from invading DNA, takes place. Translocation and DNA cleavage are afforded by the two diametrically opposed R-subunits. To gain insight into the mechanism of translocation, a detailed characterization of the ATPase activity of EcoR124I was done. Results show that following recognition sequence binding, ATP hydrolysis-coupled, bidirectional DNA translocation by EcoR124I ensues, with the R-subunits transiently disengaging, on average, every 515 bp. Macroscopic processivity of 2031(+/-184)bp is maintained, as the R-subunits remain in close proximity to the DNA through association with the methyltransferase. Transient uncoupling of ATP hydrolysis from translocation results in 3.1(+/-0.4) ATP molecules being hydrolyzed per base-pair translocated per R-subunit. This is the first clear demonstration of the coupling of ATP hydrolysis to dsDNA translocation, albeit inefficient. Once translocation is impeded on supercoiled DNA, the DNA is cleaved. DNA cleavage inactivates the EcoR124I holoenzyme partially and reversibly, which explains the stoichiometric behaviour of type I restriction enzymes. Inactivated holoenzyme remains bound to the DNA at the recognition sequence and immediately releases the nascent ends. The release of nascent ends was demonstrated using a novel, fluorescence-based, real-time assay that takes advantage of the ability of the Escherichia coli RecBCD enzyme to unwind restricted dsDNA. The resulting unwinding of EcoR124I-restricted DNA by RecBCD reveals coordination between the restriction-modification and recombination systems that functions to destroy invading DNA efficiently. In addition, we demonstrate the displacement of EcoR124I following DNA cleavage by the translocating RecBCD enzyme, resulting in the restoration of catalytic function to EcoR124I.

Published

2005

50. Hepatitis C NS3 helicase unwinds RNA in leaps and bounds

Author

Piero R. Bianco

Subjects

Chemistry, RNA, General Medicine, Hepatitis C, Hepacivirus, Viral Nonstructural Proteins, Ns3 helicase, medicine.disease, Virology, medicine, RNA, Viral, LEAPS, RNA Helicases, RNA, Double-Stranded

Published

2004