Your search keyword '"Reid C Johnson"' showing total 133 results

1. Multiple serine transposase dimers assemble the transposon-end synaptic complex during IS607-family transposition

Author

Wenyang Chen, Sridhar Mandali, Stephen P Hancock, Pramod Kumar, Michael Collazo, Duilio Cascio, and Reid C Johnson

Subjects

DNA transposition, serine recombinase, nucleoprotein complex, Helicobacter pylori, Mycobacteria tuberculosis, Sulfolobus islandicus, Medicine, Science, Biology (General), QH301-705.5

Abstract

IS607-family transposons are unusual because they do not have terminal inverted repeats or generate target site duplications. They encode two protein-coding genes, but only tnpA is required for transposition. Our X-ray structures confirm that TnpA is a member of the serine recombinase (SR) family, but the chemically-inactive quaternary structure of the dimer, along with the N-terminal location of the DNA binding domain, are different from other SRs. TnpA dimers from IS1535 cooperatively associate with multiple subterminal repeats, which together with additional nonspecific binding, form a nucleoprotein filament on one transposon end that efficiently captures a second unbound end to generate the paired-end complex (PEC). Formation of the PEC does not require a change in the dimeric structure of the catalytic domain, but remodeling of the C-terminal α-helical region is involved. We posit that the PEC recruits a chemically-active conformer of TnpA to the transposon end to initiate DNA chemistry.

Published

2018

2. DNA Sequence Determinants Controlling Affinity, Stability and Shape of DNA Complexes Bound by the Nucleoid Protein Fis.

Author

Stephen P Hancock, Stefano Stella, Duilio Cascio, and Reid C Johnson

Subjects

Medicine, Science

Abstract

The abundant Fis nucleoid protein selectively binds poorly related DNA sequences with high affinities to regulate diverse DNA reactions. Fis binds DNA primarily through DNA backbone contacts and selects target sites by reading conformational properties of DNA sequences, most prominently intrinsic minor groove widths. High-affinity binding requires Fis-stabilized DNA conformational changes that vary depending on DNA sequence. In order to better understand the molecular basis for high affinity site recognition, we analyzed the effects of DNA sequence within and flanking the core Fis binding site on binding affinity and DNA structure. X-ray crystal structures of Fis-DNA complexes containing variable sequences in the noncontacted center of the binding site or variations within the major groove interfaces show that the DNA can adapt to the Fis dimer surface asymmetrically. We show that the presence and position of pyrimidine-purine base steps within the major groove interfaces affect both local DNA bending and minor groove compression to modulate affinities and lifetimes of Fis-DNA complexes. Sequences flanking the core binding site also modulate complex affinities, lifetimes, and the degree of local and global Fis-induced DNA bending. In particular, a G immediately upstream of the 15 bp core sequence inhibits binding and bending, and A-tracts within the flanking base pairs increase both complex lifetimes and global DNA curvatures. Taken together, our observations support a revised DNA motif specifying high-affinity Fis binding and highlight the range of conformations that Fis-bound DNA can adopt. The affinities and DNA conformations of individual Fis-DNA complexes are likely to be tailored to their context-specific biological functions.

Published

2016

3. Multiple interfaces between a serine recombinase and an enhancer control site-specific DNA inversion

Author

Meghan M McLean, Yong Chang, Gautam Dhar, John K Heiss, and Reid C Johnson

Subjects

Salmonella enterica, site-specific DNA recombination, serine recombinase, recombinational enhancer, synaptic complex, DNA strand exchange, Medicine, Science, Biology (General), QH301-705.5

Abstract

Serine recombinases are often tightly controlled by elaborate, topologically-defined, nucleoprotein complexes. Hin is a member of the DNA invertase subclass of serine recombinases that are regulated by a remote recombinational enhancer element containing two binding sites for the protein Fis. Two Hin dimers bound to specific recombination sites associate with the Fis-bound enhancer by DNA looping where they are remodeled into a synaptic tetramer competent for DNA chemistry and exchange. Here we show that the flexible beta-hairpin arms of the Fis dimers contact the DNA binding domain of one subunit of each Hin dimer. These contacts sandwich the Hin dimers to promote remodeling into the tetramer. A basic region on the Hin catalytic domain then contacts enhancer DNA to complete assembly of the active Hin tetramer. Our results reveal how the enhancer generates the recombination complex that specifies DNA inversion and regulates DNA exchange by the subunit rotation mechanism.

Published

2013

4. Testing mechanisms of DNA sliding by architectural DNA-binding proteins: dynamics of single wild-type and mutant protein molecules in vitro and in vivo

Author

Yuji Itoh, Sridhar Mandali, Cheng Tan, Reid C. Johnson, Yining Wu, Shoji Takada, Eriko Mano, and Kiyoto Kamagata

Subjects

Saccharomyces cerevisiae Proteins, AcademicSubjects/SCI00010, Mutant, Saccharomyces cerevisiae, Biology, Molecular Dynamics Simulation, DNA-binding protein, Mitochondrial Proteins, chemistry.chemical_compound, Mutant protein, Information and Computing Sciences, Genetics, Nucleoid, Binding site, Circular bacterial chromosome, Gene regulation, Chromatin and Epigenetics, Bacterial nucleoid, DNA, Biological Sciences, Chromosomes, Bacterial, Single Molecule Imaging, DNA-Binding Proteins, chemistry, Biophysics, HMGN Proteins, Mutant Proteins, Environmental Sciences, Developmental Biology, Protein Binding

Abstract

Architectural DNA-binding proteins (ADBPs) are abundant constituents of eukaryotic or bacterial chromosomes that bind DNA promiscuously and function in diverse DNA reactions. They generate large conformational changes in DNA upon binding yet can slide along DNA when searching for functional binding sites. Here we investigate the mechanism by which ADBPs diffuse on DNA by single-molecule analyses of mutant proteins rationally chosen to distinguish between rotation-coupled diffusion and DNA surface sliding after transient unbinding from the groove(s). The properties of yeast Nhp6A mutant proteins, combined with molecular dynamics simulations, suggest Nhp6A switches between two binding modes: a static state, in which the HMGB domain is bound within the minor groove with the DNA highly bent, and a mobile state, where the protein is traveling along the DNA surface by means of its flexible N-terminal basic arm. The behaviors of Fis mutants, a bacterial nucleoid-associated helix-turn-helix dimer, are best explained by mobile proteins unbinding from the major groove and diffusing along the DNA surface. Nhp6A, Fis, and bacterial HU are all near exclusively associated with the chromosome, as packaged within the bacterial nucleoid, and can be modeled by three diffusion modes where HU exhibits the fastest and Fis the slowest diffusion.

Published

2021

5. The HMGB chromatin protein Nhp6A can bypass obstacles when traveling on DNA

Author

Satoshi Takahashi, Kana Ouchi, Yining Wu, Eriko Mano, Reid C. Johnson, Kiyoto Kamagata, Cheng Tan, Shoji Takada, and Sridhar Mandali

Subjects

Saccharomyces cerevisiae Proteins, AcademicSubjects/SCI00010, Saccharomyces cerevisiae, Molecular Dynamics Simulation, DNA-binding protein, Bacterial protein, Motion, 03 medical and health sciences, chemistry.chemical_compound, Molecular dynamics, Genetics, Fluorescence microscope, 030304 developmental biology, 0303 health sciences, biology, Gene regulation, Chromatin and Epigenetics, 030302 biochemistry & molecular biology, DNA, Chromatin protein, biology.organism_classification, Single Molecule Imaging, Chromatin, chemistry, Biophysics, HMGN Proteins, Protein Binding

Abstract

DNA binding proteins rapidly locate their specific DNA targets through a combination of 3D and 1D diffusion mechanisms, with the 1D search involving bidirectional sliding along DNA. However, even in nucleosome-free regions, chromosomes are highly decorated with associated proteins that may block sliding. Here we investigate the ability of the abundant chromatin-associated HMGB protein Nhp6A from Saccharomyces cerevisiae to travel along DNA in the presence of other architectural DNA binding proteins using single-molecule fluorescence microscopy. We observed that 1D diffusion by Nhp6A molecules is retarded by increasing densities of the bacterial proteins Fis and HU and by Nhp6A, indicating these structurally diverse proteins impede Nhp6A mobility on DNA. However, the average travel distances were larger than the average distances between neighboring proteins, implying Nhp6A is able to bypass each of these obstacles. Together with molecular dynamics simulations, our analyses suggest two binding modes: mobile molecules that can bypass barriers as they seek out DNA targets, and near stationary molecules that are associated with neighboring proteins or preferred DNA structures. The ability of mobile Nhp6A molecules to bypass different obstacles on DNA suggests they do not block 1D searches by other DNA binding proteins.

Published

2020

6. Control of the Serine Integrase Reaction: Roles of the Coiled-Coil and Helix E Regions in DNA Site Synapsis and Recombination

Author

Reid C. Johnson and Sridhar Mandali

Subjects

Prophages, Virus Integration, 1.1 Normal biological development and functioning, Mutant, Amino Acid Motifs, Medical and Health Sciences, Microbiology, synaptic complex, 03 medical and health sciences, chemistry.chemical_compound, Viral Proteins, Genetic, Protein Domains, Underpinning research, Recombinase, Genetics, Directionality, site-specific DNA recombination, Bacteriophages, Attachment Sites, Molecular Biology, 030304 developmental biology, Recombination, Genetic, Coiled coil, 0303 health sciences, phage A118, biology, Integrases, Agricultural and Veterinary Sciences, 030306 microbiology, Synapsis, Biological Sciences, Microbiological, Listeria monocytogenes, Recombination, Integrase, Cell biology, Chromosome Pairing, chemistry, serine recombinase, Attachment Sites, Microbiological, biology.protein, Generic health relevance, DNA, Research Article, Biotechnology

Abstract

Bacteriophage serine integrases catalyze highly specific recombination reactions between defined DNA segments called att sites. These reactions are reversible depending upon the presence of a second phage-encoded directionality factor. The bipartite C-terminal DNA binding region of integrases includes a recombinase domain (RD) connected to a zinc-binding domain (ZD), which contains a long flexible coiled-coil (CC) motif that extends away from the bound DNA. We directly show that the identities of the phage A118 integrase att sites are specified by the DNA spacing between the RD and ZD DNA recognition determinants, which in turn, directs the relative trajectories of the CC motifs on each subunit of the att -bound integrase dimer. Recombination between compatible dimer-bound att sites requires minimal length CC motifs and 14 residues surrounding the tip where pairing of CC motifs between synapsing dimers occurs. Our alanine-scanning data suggests that molecular interactions between CC motif tips may differ in integrative ( attP x attB ) and excisive ( attL x attR ) recombination reactions. We identify mutations in 5 residues within the integrase oligomerization helix that control the remodeling of dimers into tetramers during synaptic complex formation. Whereas most of these gain-of-function mutants still require the CC motifs for synapsis, one mutant efficiently, but indiscriminantly, forms synaptic complexes without the CC motifs. However, the CC motifs are still required for recombination, suggesting a function for the CC motifs after initial assembly of the integrase synaptic tetramer. Importance The robust and exquisitely-regulated site-specific recombination reactions promoted by serine integrases are integral to the life cycle of temperate bacteriophage, and in the case of the A118 prophage, are an important virulence factor by Listeria monocytogenes . The properties of these recombinases have led to their repurposing into tools for genetic engineering and synthetic biology. In this report, we identify determinants regulating synaptic complex formation between correct DNA sites, including the DNA architecture responsible for specifying the identity of recombination sites, features of the unique coiled-coil structure on the integrase that are required to initiate synapsis, and amino acid residues on the integrase oligomerization helix that control the remodeling of synapsing dimers into a tetramer active for DNA strand exchange.

Published

2021

7. Cooperative DNA binding by proteins through DNA shape complementarity

Author

Reid C. Johnson, Duilio Cascio, and Stephen P. Hancock

Subjects

DNA, Bacterial, Models, Molecular, Protein Conformation, alpha-Helical, Allosteric regulation, Genetic Vectors, Gene Expression, Cooperativity, Plasma protein binding, Biology, Crystallography, X-Ray, law.invention, 03 medical and health sciences, chemistry.chemical_compound, Viral Proteins, 0302 clinical medicine, law, Mutant protein, Factor For Inversion Stimulation Protein, Genetics, Escherichia coli, Protein Interaction Domains and Motifs, Cloning, Molecular, Molecular Biology, 030304 developmental biology, 0303 health sciences, Binding Sites, Base Sequence, Escherichia coli Proteins, Chromosome, Recombinational DNA Repair, Chromosomes, Bacterial, Bacteriophage lambda, Recombinant Proteins, Kinetics, chemistry, DNA Nucleotidyltransferases, Recombinant DNA, Biophysics, Nucleic Acid Conformation, Thermodynamics, Protein Conformation, beta-Strand, Sequence Alignment, 030217 neurology & neurosurgery, Recombination, DNA, Allosteric Site, Protein Binding

Abstract

Localized arrays of proteins cooperatively assemble onto chromosomes to control DNA activity in many contexts. Binding cooperativity is often mediated by specific protein–protein interactions, but cooperativity through DNA structure is becoming increasingly recognized as an additional mechanism. During the site-specific DNA recombination reaction that excises phage λ from the chromosome, the bacterial DNA architectural protein Fis recruits multiple λ-encoded Xis proteins to the attR recombination site. Here, we report X-ray crystal structures of DNA complexes containing Fis + Xis, which show little, if any, contacts between the two proteins. Comparisons with structures of DNA complexes containing only Fis or Xis, together with mutant protein and DNA binding studies, support a mechanism for cooperative protein binding solely by DNA allostery. Fis binding both molds the minor groove to potentiate insertion of the Xis β-hairpin wing motif and bends the DNA to facilitate Xis-DNA contacts within the major groove. The Fis-structured minor groove shape that is optimized for Xis binding requires a precisely positioned pyrimidine-purine base-pair step, whose location has been shown to modulate minor groove widths in Fis-bound complexes to different DNA targets.

Published

2019

8. Author response: Multiple serine transposase dimers assemble the transposon-end synaptic complex during IS607-family transposition

Author

Sridhar Mandali, Reid C. Johnson, Wenyang Chen, Pramod Kumar, Michael Collazo, Duilio Cascio, and Stephen P. Hancock

Subjects

Transposition (music), Serine, Genetics, Transposable element, Biology, Transposase

Published

2018

9. High Free-Energy Barrier of 1D Diffusion Along DNA by Architectural DNA-Binding Proteins

Author

Eriko Mano, Kiyoto Kamagata, Reid C. Johnson, Saori Kanbayashi, and Kana Ouchi

Subjects

Models, Molecular, 0301 basic medicine, Fluorescence-lifetime imaging microscopy, HMGB chromatin protein, Biochemistry & Molecular Biology, single-molecule fluorescence microscopy, Diffusion, Entropy, bacterial nucleoid protein, DNA-binding protein, Microbiology, Article, 03 medical and health sciences, chemistry.chemical_compound, Medicinal and Biomolecular Chemistry, Bacterial Proteins, Structural Biology, Models, HMGB Proteins, Molecule, Molecular Biology, Chemistry, Molecular, DNA, DNA-Binding Proteins, 030104 developmental biology, protein–DNA sliding dynamics, Biophysics, protein-DNA sliding dynamics, Nucleic Acid Conformation, Biochemistry and Cell Biology, DNA conformational change, Function (biology), Protein Binding

Abstract

Architectural DNA-binding proteins function to regulate diverse DNA reactions and have the defining property of significantly changing DNA conformation. Although the 1D movement along DNA by other types of DNA-binding proteins has been visualized, the mobility of architectural DNA-binding proteins on DNA remains unknown. Here, we applied single-molecule fluorescence imaging on arrays of extended DNA molecules to probe the binding dynamics of three structurally distinct architectural DNA-binding proteins: Nhp6A, HU, and Fis. Each of these proteins was observed to move along DNA, and the salt concentration independence of the 1D diffusion implies sliding with continuous contact to DNA. Nhp6A and HU exhibit a single sliding mode, whereas Fis exhibits two sliding modes. Based on comparison of the diffusion coefficients and sizes of many DNA binding proteins, the architectural proteins are categorized into a new group distinguished by an unusually high free-energy barrier for 1D diffusion. The higher free-energy barrier for 1D diffusion by architectural proteins can be attributed to the large DNA conformational changes that accompany binding and impede rotation-coupled movement along the DNA grooves.

Published

2018

10. Control of Recombination Directionality by the Listeria Phage A118 Protein Gp44 and the Coiled-Coil Motif of Its Serine Integrase

Author

Kushol Gupta, Anthony R. Dawson, Reid C. Johnson, Gregory D. Van Duyne, Sridhar Mandali, and Henkin, Tina M

Subjects

0301 basic medicine, Gene Expression Regulation, Viral, Listeria, FLP-FRT recombination, Virus Integration, Amino Acid Motifs, Biology, Medical and Health Sciences, Microbiology, Bacteriophage, 03 medical and health sciences, Viral Proteins, Genetic, Protein Domains, Serine, Genetics, site-specific DNA recombination, Bacteriophages, Site-specific recombination, Viral, Molecular Biology, Recombination, Genetic, Integrases, Agricultural and Veterinary Sciences, DNA-binding domain, Biological Sciences, biology.organism_classification, Listeria monocytogenes, Recombination, Integrase, Temperateness, 030104 developmental biology, Gene Expression Regulation, biology.protein, serine integrase, Cre-Lox recombination, recombination directionality factor, Research Article, Biotechnology

Abstract

The serine integrase of phage A118 catalyzes integrative recombination between attP on the phage and a specific attB locus on the chromosome of Listeria monocytogenes , but it is unable to promote excisive recombination between the hybrid attL and attR sites found on the integrated prophage without assistance by a recombination directionality factor (RDF). We have identified and characterized the phage-encoded RDF Gp44, which activates the A118 integrase for excision and inhibits integration. Gp44 binds to the C-terminal DNA binding domain of integrase, and we have localized the primary binding site to be within the mobile coiled-coil (CC) motif but distinct from the distal tip of the CC that is required for recombination. This interaction is sufficient to inhibit integration, but a second interaction involving the N-terminal end of Gp44 is also required to activate excision. We provide evidence that these two contacts modulate the trajectory of the CC motifs as they extend out from the integrase core in a manner dependent upon the identities of the four att sites. Our results support a model whereby Gp44 shapes the Int-bound complexes to control which att sites can synapse and recombine. IMPORTANCE Serine integrases mediate directional recombination between bacteriophage and bacterial chromosomes. These highly regulated site-specific recombination reactions are integral to the life cycle of temperate phage and, in the case of Listeria monocytogenes lysogenized by A118 family phage, are an essential virulence determinant. Serine integrases are also utilized as tools for genetic engineering and synthetic biology because of their exquisite unidirectional control of the DNA exchange reaction. Here, we identify and characterize the recombination directionality factor (RDF) that activates excision and inhibits integration reactions by the phage A118 integrase. We provide evidence that the A118 RDF binds to and modulates the trajectory of the long coiled-coil motif that extends from the large carboxyl-terminal DNA binding domain and is postulated to control the early steps of recombination site synapsis.

Published

2017

11. Facilitated Dissociation of Transcription Factors from Single DNA Binding Sites

Author

Reid C. Johnson, Rebecca D. Giuntoli, Monica Olvera de la Cruz, John F. Marko, Ramsey I. Kamar, Edward J. Banigan, and Aykut Erbas

Subjects

0301 basic medicine, Saccharomyces cerevisiae Proteins, Cooperativity, Plasma protein binding, Saccharomyces cerevisiae, 010402 general chemistry, DNA-protein interactions, 01 natural sciences, Dissociation (chemistry), Mitochondrial Proteins, 03 medical and health sciences, chemistry.chemical_compound, chemical kinetics, Genetics, Binding site, DNA, Fungal, Transcription factor, transcription factor, 030304 developmental biology, 0303 health sciences, Multidisciplinary, Binding Sites, 030102 biochemistry & molecular biology, facilitated dissociation, DNA, Bacterial nucleoid, Receptor–ligand kinetics, 0104 chemical sciences, DNA binding site, Kinetics, Fungal, 030104 developmental biology, PNAS Plus, chemistry, Biochemistry, biomolecule binding, Biophysics, HMGN Proteins, Generic health relevance, DNA–protein interactions, Protein Binding, Transcription Factors

Abstract

The binding of transcription factors (TFs) to DNA controls most aspects of cellular function, making the understanding of their binding kinetics imperative. The standard description of bimolecular interactions posits TF off-rates are independent of TF concentration in solution. However, recent observations have revealed that proteins in solution can accelerate the dissociation of DNA-bound proteins. To study the molecular basis of facilitated dissociation (FD), we have used single-molecule imaging to measure dissociation kinetics of Fis, a key E. coli TF and major bacterial nucleoid protein, from single dsDNA binding sites. We observe a strong FD effect characterized by an exchange rate ∽1 × 104 M-1s-1, establishing that FD of Fis occurs at the single-binding-site level, and we find that the off-rate saturates at large Fis concentrations in solution. While spontaneous (i.e., competitor-free) dissociation shows a strong salt dependence, we find that facilitated dissociation depends only weakly on salt. These results are quantitatively explained by a model in which partially dissociated bound proteins are susceptible to invasion by competitor proteins in solution. We also report FD of NHP6A, a yeast TF whose structure differs significantly from Fis. We further perform molecular dynamics simulations, which indicate that FD can occur for molecules that interact far more weakly than those we have studied. Taken together, our results indicate that FD is a general mechanism assisting in the local removal of TFs from their binding sites and does not necessarily require cooperativity, clustering, or binding site overlap.SIGNIFICANCE STATEMENTTranscription factors (TFs) control biological processes by binding and unbinding to DNA. Therefore it is crucial to understand the mechanisms that affect TF binding kinetics. Recent studies challenge the standard picture of TF binding kinetics by demonstrating cases of proteins in solution accelerating TF dissociation rates through a facilitated dissociation (FD) process. Our study shows that FD can occur at the level of single binding sites, without the action of large protein clusters or long DNA segments. Our results quantitatively support a model of FD in which competitor proteins invade partially dissociated states of DNA-bound TFs. FD is expected to be a general mechanism for modulating gene expression by altering the occupancy of TFs on the genome.Author ContributionsRamsey I. Kamardesigned research, performed research, contributed new reagents/analytic tools, analyzed data, wrote the paperEdward J. Banigandesigned research, performed research, contributed new reagents/analytic tools, analyzed data, wrote the paperAykut Erbasdesigned research, performed research, contributed new reagents/analytic tools, analyzed data, wrote the paperRebecca D. Giuntolidesigned research, performed research, contributed new reagents/analytic tools, analyzed data, wrote the paperMonica Olvera de la Cruzdesigned research, performed research, wrote the paperReid C. Johnsondesigned research, performed research, contributed new reagents/analytic tools, analyzed data, wrote the paperJohn F. Markodesigned research, performed research, contributed new reagents/analytic tools, analyzed data, wrote the paper

Published

2017

12. Facilitated Dissociation of a Nucleoid Protein from the Bacterial Chromosome

Author

Nastaran Hadizadeh, John F. Marko, Reid C. Johnson, and Gourse, RL

Subjects

0301 basic medicine, 1.1 Normal biological development and functioning, Plasma protein binding, Biology, medicine.disease_cause, Medical and Health Sciences, Microbiology, Chromosomes, Green fluorescent protein, 03 medical and health sciences, chemistry.chemical_compound, Underpinning research, Factor For Inversion Stimulation Protein, medicine, Escherichia coli, Genetics, Nucleoid, Molecular Biology, Transcription factor, 030102 biochemistry & molecular biology, Agricultural and Veterinary Sciences, Circular bacterial chromosome, Escherichia coli Proteins, Bacterial, Articles, Chromosomes, Bacterial, Biological Sciences, Kinetics, 030104 developmental biology, Biochemistry, chemistry, Biophysics, Generic health relevance, DNA, Transcription Factors, Protein Binding

Abstract

Off-rates of proteins from the DNA double helix are widely considered to be dependent only on the interactions inside the initially bound protein-DNA complex and not on the concentration of nearby molecules. However, a number of recent single-DNA experiments have shown off-rates that depend on solution protein concentration, or “facilitated dissociation.” Here, we demonstrate that this effect occurs for the major Escherichia coli nucleoid protein Fis on isolated bacterial chromosomes. We isolated E. coli nucleoids and showed that dissociation of green fluorescent protein (GFP)-Fis is controlled by solution Fis concentration and exhibits an “exchange” rate constant ( k exch ) of ≈10 4 M −1 s −1 , comparable to the rate observed in single-DNA experiments. We also show that this effect is strongly salt dependent. Our results establish that facilitated dissociation can be observed in vitro on chromosomes assembled in vivo . IMPORTANCE Bacteria are important model systems for the study of gene regulation and chromosome dynamics, both of which fundamentally depend on the kinetics of binding and unbinding of proteins to DNA. In experiments on isolated E. coli chromosomes, this study showed that the prolific transcription factor and chromosome packaging protein Fis displays a strong dependence of its off-rate from the bacterial chromosome on Fis concentration, similar to that observed in in vitro experiments. Therefore, the free cellular DNA-binding protein concentration can strongly affect lifetimes of proteins bound to the chromosome and must be taken into account in quantitative considerations of gene regulation. These results have particularly profound implications for transcription factors where DNA binding lifetimes can be a critical determinant of regulatory function.

Published

2016

13. Controlled rotation mechanism of DNA strand exchange by the Hin serine recombinase

Author

Xianbin Lei, Meghan M. McLean, Botao Xiao, John F. Marko, and Reid C. Johnson

Subjects

0301 basic medicine, Models, Molecular, Rotation, Protein Conformation, Chemical, Biology, Article, law.invention, Serine, 03 medical and health sciences, chemistry.chemical_compound, Bacterial Proteins, Genetic, law, Salmonella, Models, Factor For Inversion Stimulation Protein, Genetics, Recombinase, Point Mutation, Site-specific recombination, DNA Nucleotidyltransferases, chemistry.chemical_classification, Recombination, Genetic, DNA ligase, Multidisciplinary, Models, Genetic, DNA, Superhelical, Molecular, DNA, Recombinant Proteins, Recombination, DNA-Binding Proteins, Protein Subunits, 030104 developmental biology, chemistry, Biochemistry, Models, Chemical, Recombinant DNA, Biophysics, Nucleic Acid Conformation, Superhelical, Plasmids

Abstract

DNA strand exchange by serine recombinases has been proposed to occur by a large-scale rotation of halves of the recombinase tetramer. Here we provide the first direct physical evidence for the subunit rotation mechanism for the Hin serine invertase. Single-DNA looping assays using an activated mutant (Hin-H107Y) reveal specific synapses between two hix sites. Two-DNA “braiding” experiments, where separate DNA molecules carrying a single hix are interwound, show that Hin-H107Y cleaves both hix sites and mediates multi-step rotational relaxation of the interwinding. The variable numbers of rotations in the DNA braid experiments are in accord with data from bulk experiments that follow DNA topological changes accompanying recombination by the hyperactive enzyme. The relatively slow Hin rotation rates, combined with pauses, indicate considerable rotary friction between synapsed subunit pairs. A rotational pausing mechanism intrinsic to serine recombinases is likely to be crucial for DNA ligation and for preventing deleterious DNA rearrangements.

Published

2016

14. DNA Sequence Determinants Controlling Affinity, Stability and Shape of DNA Complexes Bound by the Nucleoid Protein Fis

Author

Reid C. Johnson, Stephen P. Hancock, Stefano Stella, Duilio Cascio, and Leng, Fenfei

Subjects

0301 basic medicine, Molecular biology, lcsh:Medicine, Crystallography, X-Ray, Biochemistry, Fluorophotometry, Sequencing techniques, Spectrum Analysis Techniques, Factor For Inversion Stimulation Protein, Fluorescence Resonance Energy Transfer, lcsh:Science, Base Pairing, Genetics, Multidisciplinary, DNA clamp, Crystallography, Protein Stability, Physics, Sequence analysis, Condensed Matter Physics, Nucleic acids, Chemistry, Spectrophotometry, Physical Sciences, Crystal Structure, DNA supercoil, Chemical characterization, Research Article, Protein Binding, HMG-box, Base pair, General Science & Technology, Molecular Sequence Data, DNA binding assay, Biology, Research and Analysis Methods, Phosphates, 03 medical and health sciences, Sequence Motif Analysis, DNA-binding proteins, Binding analysis, Solid State Physics, Protein–DNA interaction, Molecular Biology Techniques, Replication protein A, DNA sequence analysis, Binding Sites, 030102 biochemistry & molecular biology, Biology and life sciences, Base Sequence, Circular bacterial chromosome, lcsh:R, Chemical Compounds, DNA structure, Proteins, Correction, DNA, DNA binding site, Macromolecular structure analysis, 030104 developmental biology, Biophysics, X-Ray, Nucleic Acid Conformation, lcsh:Q, Generic health relevance

Abstract

The abundant Fis nucleoid protein selectively binds poorly related DNA sequences with high affinities to regulate diverse DNA reactions. Fis binds DNA primarily through DNA backbone contacts and selects target sites by reading conformational properties of DNA sequences, most prominently intrinsic minor groove widths. High-affinity binding requires Fis-stabilized DNA conformational changes that vary depending on DNA sequence. In order to better understand the molecular basis for high affinity site recognition, we analyzed the effects of DNA sequence within and flanking the core Fis binding site on binding affinity and DNA structure. X-ray crystal structures of Fis-DNA complexes containing variable sequences in the noncontacted center of the binding site or variations within the major groove interfaces show that the DNA can adapt to the Fis dimer surface asymmetrically. We show that the presence and position of pyrimidine-purine base steps within the major groove interfaces affect both local DNA bending and minor groove compression to modulate affinities and lifetimes of Fis-DNA complexes. Sequences flanking the core binding site also modulate complex affinities, lifetimes, and the degree of local and global Fis-induced DNA bending. In particular, a G immediately upstream of the 15 bp core sequence inhibits binding and bending, and A-tracts within the flanking base pairs increase both complex lifetimes and global DNA curvatures. Taken together, our observations support a revised DNA motif specifying high-affinity Fis binding and highlight the range of conformations that Fis-bound DNA can adopt. The affinities and DNA conformations of individual Fis-DNA complexes are likely to be tailored to their context-specific biological functions.

Published

2016

15. Variation of the folding and dynamics of theEscherichia colichromosome with growth conditions

Author

Nastaran Hadizadeh Yazdi, John F. Marko, Călin C. Guet, and Reid C. Johnson

Subjects

Cell division, Cell, Chromosome, Biology, medicine.disease_cause, Microbiology, Photobleaching, Molecular biology, Nucleoprotein, Protein filament, medicine.anatomical_structure, medicine, Biophysics, Nucleoid, Molecular Biology, Escherichia coli

Abstract

Summary We examine whether the Escherichia coli chromosome is folded into a self-adherent nucleoprotein complex, or alternately is a confined but otherwise unconstrained self-avoiding polymer. We address this through in vivo visualization, using an inducible GFP fusion to the nucleoid-associated protein Fis to nonspecifically decorate the entire chromosome. For a range of different growth conditions, the chromosome is a compact structure that does not fill the volume of the cell, and which moves from the new pole to the cell centre.Duringrapidgrowth,chromosomesegregation occurs well before cell division, with daughter chromosomes coupled by a thin inter-daughter filament before complete segregation, whereas during slow growth chromosomes stay adjacent until cell division occurs. Image correlation analysis indicates that sub-nucleoid structure is stable on a 1 min timescale, comparable to the timescale for redistribution time measured for GFP‐Fis after photobleaching. Optical deconvolutionandwrithecalculationanalysisindicate that the nucleoid has a large-scale coiled organization rather than being an amorphous mass. Our observations are consistent with the chromosome having a self-adherent filament organization.

Published

2012

16. Counting proteins bound to a single DNA molecule

Author

John S. Graham, John F. Marko, and Reid C. Johnson

Subjects

Escherichia coli Proteins, Biophysics, DNA, Cell Biology, Computational biology, Biology, Factor For Inversion Stimulation Protein, Biochemistry, DNA-binding protein, Genome, Fluorescence, Article, Cell biology, DNA-Binding Proteins, Bimolecular fluorescence complementation, chemistry.chemical_compound, Microscopy, Fluorescence, chemistry, Fluorescence microscope, Transcriptional regulation, Molecular Biology

Abstract

Chromosomes contain DNA covered with proteins performing functions such as architectural organization and transcriptional regulation. The ability to count the number of proteins bound to various regions of the genome is essential for understanding both architectural and regulatory functions. We present a straightforward method of counting gfp-conjugated proteins bound to an individual duplex DNA molecule by calibrating to a commercially available fluorescence standard using wide-field fluorescence microscopy. We demonstrate our method using the E. coli nucleoid-associated protein Fis.

Published

2011

17. Intrasubunit and Intersubunit Interactions Controlling Assembly of Active Synaptic Complexes during Hin-Catalyzed DNA Recombination

Author

Erin R. Sanders, John K. Heiss, and Reid C. Johnson

Subjects

Protein Conformation, Molecular Sequence Data, Sigma Factor, Biology, medicine.disease_cause, Catalysis, Article, law.invention, chemistry.chemical_compound, Protein structure, Structural Biology, law, Factor For Inversion Stimulation Protein, medicine, Recombinase, Amino Acid Sequence, Molecular Biology, Heat-Shock Proteins, Recombination, Genetic, Mutation, Sequence Homology, Amino Acid, DNA, Superhelical, Escherichia coli Proteins, Mutagenesis, Protein Subunits, chemistry, Biochemistry, Chromosome Inversion, Synapses, Mutagenesis, Site-Directed, Biophysics, Recombinant DNA, DNA supercoil, DNA

Abstract

Serine recombinases, which generate double-strand breaks in DNA, must be carefully regulated to ensure that chemically active DNA complexes are assembled correctly. In the Hin-catalyzed site-specific DNA inversion reaction, two inversely oriented recombination sites on the same DNA molecule assemble into a synaptic complex that uniquely generates inversion products. The Fis-bound recombinational enhancer, together with topological constraints directed by DNA supercoiling, functions to regulate Hin synaptic complex formation and activity. We have isolated a collection of gain-of-function mutants in 22 positions within the catalytic and oligomerization domains of Hin using two genetic screens and by site-directed mutagenesis. One genetic screen measured recombination in the absence of Fis and the other assessed SOS induction as a readout of increased DNA cleavage. These mutations, together with molecular modeling, identify important sites of dynamic intrasubunit and intersubunit interactions that regulate assembly of the active tetrameric recombination complex. Of particular interest are interactions between the oligomerization helix (helix E) and the catalytic domain of the same subunit that function to hold the dimer in an inactive state in the absence of the Fis/enhancer system. Among these is a relay involving a triad of phenylalanines that are proposed to switch positions during the transition from dimers to the catalytically active tetramer. Novel Hin mutants that generate synaptic complexes that are blocked at steps prior to DNA cleavage are also described.

Published

2011

18. Concentration-dependent exchange accelerates turnover of proteins bound to double-stranded DNA

Author

John S. Graham, John F. Marko, and Reid C. Johnson

Subjects

Saccharomyces cerevisiae Proteins, Plasma protein binding, Biology, medicine.disease_cause, HMGN Proteins, DNA-binding protein, Fluorescence, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Factor For Inversion Stimulation Protein, Information and Computing Sciences, Genetics, medicine, Molecular Biology, Escherichia coli, 030304 developmental biology, Regulation of gene expression, Microscopy, 0303 health sciences, Escherichia coli Proteins, DNA, Biological Sciences, DNA-Binding Proteins, Kinetics, Microscopy, Fluorescence, Biochemistry, chemistry, Membrane protein, Biophysics, Environmental Sciences, 030217 neurology & neurosurgery, Protein Binding, Developmental Biology

Abstract

The multistep kinetics through which DNA-binding proteins bind their targets are heavily studied, but relatively little attention has been paid to proteins leaving the double helix. Using single-DNA stretching and fluorescence detection, we find that sequence-neutral DNA-binding proteins Fis, HU and NHP6A readily exchange with themselves and with each other. In experiments focused on the Escherichia coli nucleoid-associated protein Fis, only a small fraction of protein bound to DNA spontaneously dissociates into protein-free solution. However, if Fis is present in solution, we find that a concentration-dependent exchange reaction occurs which turns over the bound protein, with a rate of k(exch) = 6 × 10(4) M(-1)s(-1). The bacterial DNA-binding protein HU and the yeast HMGB protein NHP6A display the same phenomenon of protein in solution accelerating dissociation of previously bound labeled proteins as exchange occurs. Thus, solvated proteins can play a key role in facilitating removal and renewal of proteins bound to the double helix, an effect that likely plays a major role in promoting the turnover of proteins bound to DNA in vivo and, therefore, in controlling the dynamics of gene regulation.

Published

2010

19. Chromatin-dependent binding of the S. cerevisiae HMGB protein Nhp6A affects nucleosome dynamics and transcription

Author

Adam S. Sperling, Reid C. Johnson, Michael Mason, and Noah Dowell

Subjects

Binding Sites, Saccharomyces cerevisiae Proteins, Transcription, Genetic, HMG-box, High Mobility Group Proteins, Promoter, Saccharomyces cerevisiae, Biology, ChIP-on-chip, Molecular biology, Chromatin, Chromatin remodeling, Nucleosomes, ChIP-sequencing, Cell biology, DNA-Binding Proteins, DNA binding site, Genetics, HMGN Proteins, DNA, Fungal, Chromatin immunoprecipitation, Research Paper, Developmental Biology

Abstract

The Saccharomyces cerevisiae protein Nhp6A is a model for the abundant and multifunctional high-mobility group B (HMGB) family of chromatin-associated proteins. Nhp6A binds DNA in vitro without sequence specificity and bends DNA sharply, but its role in chromosome biology is poorly understood. We show by whole-genome chromatin immunoprecipitation (ChIP) and high-resolution whole-genome tiling arrays (ChIP–chip) that Nhp6A is localized to specific regions of chromosomes that include ∼23% of RNA polymerase II promoters. Nhp6A binding functions to stabilize nucleosomes, particularly at the transcription start site of these genes. Both genomic binding and transcript expression studies point to functionally related groups of genes that are bound specifically by Nhp6A and whose transcription is altered by the absence of Nhp6. Genomic analyses of Nhp6A mutants specifically defective in DNA bending reveal a critical role of DNA bending for stabilizing chromatin and coregulation of transcription but not for targeted binding by Nhp6A. We conclude that the chromatin environment, not DNA sequence recognition, localizes Nhp6A binding, and that Nhp6A stabilizes chromatin structure and coregulates transcription.

Published

2010

20. Modulation of HU–DNA interactions by salt concentration and applied force

Author

Reid C. Johnson, John F. Marko, and Botao Xiao

Subjects

Sodium, Kinetics, chemistry.chemical_element, Plasma protein binding, Biology, Buffers, Sodium Chloride, DNA condensation, Dissociation (chemistry), 03 medical and health sciences, chemistry.chemical_compound, Bacterial Proteins, Glutamates, Gene expression, Genetics, Molecular Biology, 030304 developmental biology, 0303 health sciences, Circular bacterial chromosome, 030302 biochemistry & molecular biology, DNA, DNA-Binding Proteins, chemistry, Biochemistry, Biophysics, Protein Binding

Abstract

HU is one of the most abundant proteins in bacterial chromosomes and participates in nucleoid compaction and gene regulation. We report experiments using DNA stretching that study the dependence of DNA condensation by HU on force, salt and HU concentration. Previous experiments at sub-physiological salt levels revealed that low concentrations of HU could compact DNA, whereas larger HU concentrations formed a DNA-stiffening complex. Here we report that this bimodal binding behavior depends sensitively on salt concentration. Only the compaction mode was observed for 150 mM and higher NaCl levels, i.e. for physiological salt concentrations. Similar results were obtained for the more physiological salt K-glutamate. Real-time studies of dissociation kinetics revealed that HU unbound slowly (minutes to hours under the conditions studied) but completely for salt concentrations at or above 100 mM NaCl; the lifetime of HU complexes was observed to increase with the HU concentration at which the complexes were formed, and to decrease with salt concentration. Higher salt levels of 300 mM NaCl completely eliminated observable HU binding to DNA. Finally, we observed that the dissociation kinetics depend on force applied to the DNA: increased applied force in the sub-piconewton range accelerates dissociation, suggesting a mechanism for DNA tension to regulate chromosome structure and gene expression.

Published

2010

21. The shape of the DNA minor groove directs binding by the DNA-bending protein Fis

Author

Stefano Stella, Reid C. Johnson, and Duilio Cascio

Subjects

DNA, Bacterial, Models, Molecular, Guanine, Materials science, In silico, Molecular Sequence Data, Sequence alignment, chemistry.chemical_compound, Protein structure, Factor For Inversion Stimulation Protein, Genetics, Protein Interaction Domains and Motifs, Groove (engineering), Base Sequence, Escherichia coli Proteins, Protein Structure, Tertiary, chemistry, Naked DNA, Biophysics, Crystallization, Sequence Alignment, DNA, Research Paper, Developmental Biology

Abstract

The bacterial nucleoid-associated protein Fis regulates diverse reactions by bending DNA and through DNA-dependent interactions with other control proteins and enzymes. In addition to dynamic nonspecific binding to DNA, Fis forms stable complexes with DNA segments that share little sequence conservation. Here we report the first crystal structures of Fis bound to high- and low-affinity 27-base-pair DNA sites. These 11 structures reveal that Fis selects targets primarily through indirect recognition mechanisms involving the shape of the minor groove and sequence-dependent induced fits over adjacent major groove interfaces. The DNA shows an overall curvature of approximately 65 degrees , and the unprecedented close spacing between helix-turn-helix motifs present in the apodimer is accommodated by severe compression of the central minor groove. In silico DNA structure models show that only the roll, twist, and slide parameters are sufficient to reproduce the changes in minor groove widths and recreate the curved Fis-bound DNA structure. Models based on naked DNA structures suggest that Fis initially selects DNA targets with intrinsically narrow minor grooves using the separation between helix-turn-helix motifs in the Fis dimer as a ruler. Then Fis further compresses the minor groove and bends the DNA to generate the bound structure.

Published

2010

22. Mechanical Constraints on Hin Subunit Rotation Imposed by the Fis/Enhancer System and DNA Supercoiling during Site-Specific Recombination

Author

John K. Heiss, Reid C. Johnson, and Gautam Dhar

Subjects

Biology, Article, chemistry.chemical_compound, Salmonella, Factor For Inversion Stimulation Protein, Recombinase, A-DNA, Site-specific recombination, Cysteine, Promoter Regions, Genetic, Molecular Biology, Invertasome, Recombination, Genetic, Binding Sites, Models, Genetic, DNA, Superhelical, Processivity, Cell Biology, Molecular biology, Protein Structure, Tertiary, Protein Subunits, Enhancer Elements, Genetic, chemistry, DNA Nucleotidyltransferases, Mutation, Biophysics, DNA supercoil, DNA

Abstract

Hin, a member of the serine family of site-specific recombinases, regulates gene expression by inverting a DNA segment. DNA inversion requires assembly of an invertasome complex in which a recombinational enhancer DNA segment bound by the Fis protein associates with the Hin synaptic complex at the base of a supercoiled DNA branch. Each of the four Hin subunits becomes covalently joined to the cleaved DNA ends, and DNA exchange occurs by translocation of a Hin subunit pair within the tetramer. We show here that, although the Hin tetramer forms a bidirectional molecular swivel, the Fis/enhancer system determines both the direction and number of subunit rotations. The chirality of supercoiling directs rotational direction, and the short DNA loop stabilized by Fis-Hin contacts limit rotational processivity, thereby ensuring that the DNA strands religate in the recombinant configuration. We identify multiple rotational conformers that are formed under different supercoiling and solution conditions.

Published

2009

23. Bacterial Site‐Specific DNA Inversion Systems

Author

Reid C. Johnson

Subjects

Regulation of gene expression, education.field_of_study, Mutant, Population, Synapsis, Biology, Cell biology, chemistry.chemical_compound, Biosynthesis, chemistry, Biochemistry, education, Gene, DNA, Recombination

Abstract

Specialized recombination reactions involving DNA inversions have evolved as a mechanism to generate genetic diversity within a population. They often function to preadapt a portion of a population to a sudden change in the environment or to allow a portion of a population to take advantage of a new situation. Site-specific DNA inversion reactions are characterized by recombination events which occur at defined sites and are usually catalyzed by an enzyme dedicated to that particular reaction. The low rate of inversion is believed to be primarily limited by the extremely low amounts of the Hin protein present in cells since overexpressing Hin coordinately increases inversion rates. In vivo studies have demonstrated that integration host factor (IHF) and leucine-responsive regulatory protein (LRP) participate in the fim inversion reaction. These two DNA bending proteins are believed to function together to help promote synapsis between IRL and IRR. FimB- and FimE-promoted inversion rates are also decreased in lrp mutants. LRP is a moderately abundant DNA binding and bending protein that functions as a global regulator of various genes involved in amino acid metabolism and fimbria biosynthesis. Recombination catalyzed by the Hin and Gin DNA invertases has been intensively studied in vitro, and the basic outline of the reaction is well understood. DNA inversion occurs in a simple buffered salt solution without the need for a high-energy cofactor other than the requirement for a negatively supercoiled substrate.

Published

2007

24. Fis Targets Assembly of the Xis Nucleoprotein Filament to Promote Excisive Recombination by Phage Lambda

Author

Daniel Yoo, Robert T. Clubb, Mohamad A. Abbani, Christie V. Papagiannis, Reid C. Johnson, Duilio Cascio, and My D. Sam

Subjects

Protein Conformation, Molecular Sequence Data, Plasma protein binding, Protomer, Crystallography, X-Ray, medicine.disease_cause, DNA-binding protein, Article, Viral Proteins, Protein structure, Bacterial Proteins, Structural Biology, Factor For Inversion Stimulation Protein, medicine, Binding site, Promoter Regions, Genetic, Molecular Biology, Recombination, Genetic, Genetics, Mutation, Binding Sites, Base Sequence, biology, Escherichia coli Proteins, Membrane Proteins, Lambda phage, biology.organism_classification, Bacteriophage lambda, Nucleoproteins, DNA Nucleotidyltransferases, Biophysics, Virus Activation, Dimerization, Protein Binding, Transcription Factors

Abstract

The phage-encoded Xis protein is the major determinant controlling the direction of recombination in phage lambda. Xis is a winged-helix DNA binding protein that cooperatively binds to the attR recombination site to generate a curved microfilament, which promotes assembly of the excisive intasome but inhibits formation of an integrative intasome. We find that lambda synthesizes surprisingly high levels of Xis immediately upon prophage induction when excision rates are maximal. However, because of its low sequence-specific binding activity, exemplified by a 1.9 Å co-crystal structure of a nonspecifically bound DNA complex, Xis is relatively ineffective at promoting excision in vivo in the absence of the host Fis protein. Fis binds to a segment in attR that almost entirely overlaps one of the Xis binding sites. Instead of sterically excluding Xis binding from this site, as has been previously believed, we show that Fis enhances binding of all three Xis protomers to generate the microfilament. A specific Fis-Xis interface is supported by the effects of mutations within each protein, and relaxed, but not completely sequence-neutral, binding by the central Xis protomer is supported by the effects of DNA mutations. We present a structural model for the 50 bp curved Fis-Xis cooperative complex that is assembled between the arm and Holliday junction Int binding sites whose trajectory places constraints on models for the excisive intasome structure.

Published

2007

25. Structure of the cooperative Xis–DNA complex reveals a micronucleoprotein filament that regulates phage lambda intasome assembly

Author

Duilio Cascio, Robert T. Clubb, Reid C. Johnson, Mohamad A. Abbani, Christie V. Papagiannis, and My D. Sam

Subjects

Virus Integration, Protomer, Regulatory Sequences, Nucleic Acid, Crystallography, X-Ray, law.invention, Viral Proteins, chemistry.chemical_compound, law, Escherichia coli, Directionality, Recombination, Genetic, Genetics, Binding Sites, Multidisciplinary, Base Sequence, Integrases, biology, Nucleic acid sequence, Cooperative binding, DNA, Biological Sciences, Chromosomes, Bacterial, Lambda phage, biology.organism_classification, Bacteriophage lambda, Integrase, Nucleoproteins, chemistry, Multiprotein Complexes, DNA Nucleotidyltransferases, Biophysics, biology.protein, Recombinant DNA, Nucleic Acid Conformation, Protein Binding

Abstract

The DNA architectural protein Xis regulates the construction of higher-order nucleoprotein intasomes that integrate and excise the genome of phage lambda from the Escherichia coli chromosome. Xis modulates the directionality of site-specific recombination by stimulating phage excision 10 6 -fold, while simultaneously inhibiting phage reintegration. Control is exerted by cooperatively assembling onto a ≈35-bp DNA regulatory element, which it distorts to preferentially stabilize an excisive intasome. Here, we report the 2.6-Å crystal structure of the complex between three cooperatively bound Xis proteins and a 33-bp DNA containing the regulatory element. Xis binds DNA in a head-to-tail orientation to generate a micronucleoprotein filament. Although each protomer is anchored to the duplex by a similar set of nonbase specific contacts, malleable protein–DNA interactions enable binding to sites that differ in nucleotide sequence. Proteins at the ends of the duplex sequence specifically recognize similar binding sites and participate in cooperative binding via protein–protein interactions with a bridging Xis protomer that is bound in a less specific manner. Formation of this polymer introduces ≈72° of curvature into the DNA with slight positive writhe, which functions to connect disparate segments of DNA bridged by integrase within the excisive intasome.

Published

2007

26. DNA-Segment-Facilitated Dissociation of Fis and NHP6A from DNA Detected via Single-Molecule Mechanical Response

Author

Nora B. Linzer, Reid C. Johnson, Monica Olvera de la Cruz, Edward J. Banigan, John S. Graham, Rebecca D. Giuntoli, Charles E. Sing, and John F. Marko

Subjects

Biochemistry & Molecular Biology, Saccharomyces cerevisiae Proteins, 1.1 Normal biological development and functioning, Kinetics, Saccharomyces cerevisiae, off-rate, medicine.disease_cause, Microbiology, Dissociation (chemistry), Article, chemistry.chemical_compound, Medicinal and Biomolecular Chemistry, Structural Biology, biomolecule interactions, Underpinning research, Factor For Inversion Stimulation Protein, medicine, Escherichia coli, binding kinetics, Genetics, Nucleoid, Molecule, Molecular Biology, Escherichia coli Proteins, DNA, unbinding, Receptor–ligand kinetics, Yeast, Crystallography, chemistry, Biophysics, HMGN Proteins, Salts, affinity, Generic health relevance, Biochemistry and Cell Biology, Protein Binding

Abstract

The rate of dissociation of a DNA-protein complex is often considered to be a property of that complex, without dependence on other nearby molecules in solution. We study the kinetics of dissociation of the abundant Escherichia coli nucleoid protein Fis from DNA, using a single-molecule mechanics assay. The rate of Fis dissociation from DNA is strongly dependent on the solution concentration of DNA. The off-rate (k(off)) of Fis from DNA shows an initially linear dependence on solution DNA concentration, characterized by an exchange rate of k(ex)≈9×10(-4) (ng/μl)(-1) s(-1) for 100 mM univalent salt buffer, with a very small off-rate at zero DNA concentration. The off-rate saturates at approximately k(off,max)≈8×10(-3) s(-1) for DNA concentrations above ≈20 ng/μl. This exchange reaction depends mainly on DNA concentration with little dependence on the length of the DNA molecules in solution or on binding affinity, but this does increase with increasing salt concentration. We also show data for the yeast HMGB protein NHP6A showing a similar DNA-concentration-dependent dissociation effect, with faster rates suggesting generally weaker DNA binding by NHP6A relative to Fis. Our results are well described by a model with an intermediate partially dissociated state where the protein is susceptible to being captured by a second DNA segment, in the manner of "direct transfer" reactions studied for other DNA-binding proteins. This type of dissociation pathway may be important to protein-DNA binding kinetics in vivo where DNA concentrations are large.

Published

2015

27. Controlling tetramer formation, subunit rotation and DNA ligation during Hin-catalyzed DNA inversion

Author

Yong Chang and Reid C. Johnson

Subjects

Models, Molecular, Rotation, Stereochemistry, Protein subunit, Dimer, Biology, Insert (molecular biology), chemistry.chemical_compound, Tetramer, Models, Catalytic Domain, Information and Computing Sciences, Genetics, Recombinase, chemistry.chemical_classification, DNA ligase, Recombinase activity, Nucleic Acid Enzymes, Molecular, DNA, Biological Sciences, Protein Subunits, chemistry, Biochemistry, Amino Acid Substitution, DNA Nucleotidyltransferases, Biocatalysis, Protein Multimerization, Hydrophobic and Hydrophilic Interactions, Environmental Sciences, Developmental Biology

Abstract

Two critical steps controlling serine recombinase activity are the remodeling of dimers into the chemically active synaptic tetramer and the regulation of subunit rotation during DNA exchange. We identify a set of hydrophobic residues within the oligomerization helix that controls these steps by the Hin DNA invertase. Phe105 and Met109 insert into hydrophobic pockets within the catalytic domain of the same subunit to stabilize the inactive dimer conformation. These rotate out of the catalytic domain in the dimer and into the subunit rotation interface of the tetramer. About half of residue 105 and 109 substitutions gain the ability to generate stable synaptic tetramers and/or promote DNA chemistry without activation by the Fis/enhancer element. Phe106 replaces Phe105 in the catalytic domain pocket to stabilize the tetramer conformation. Significantly, many of the residue 105 and 109 substitutions support subunit rotation but impair ligation, implying a defect in rotational pausing at the tetrameric conformer poised for ligation. We propose that a ratchet-like surface involving Phe105, Met109 and Leu112 within the rotation interface functions to gate the subunit rotation reaction. Hydrophobic residues are present in analogous positions in other serine recombinases and likely perform similar functions.

Published

2015

28. Site-specific DNA Inversion by Serine Recombinases

Author

Reid C. Johnson

Subjects

Microbiology (medical), DNA, Bacterial, Physiology, Protein subunit, Population, Biology, Article, Serine, chemistry.chemical_compound, Genetics, Recombinase, Bacteriophages, Site-specific recombination, education, Enhancer, Invertasome, Recombination, Genetic, education.field_of_study, General Immunology and Microbiology, Ecology, Bacteria, Cell Biology, Cell biology, Infectious Diseases, chemistry, DNA Nucleotidyltransferases, DNA

Abstract

Reversible site-specific DNA inversion reactions are widely distributed in bacteria and their viruses. They control a range of biological reactions that most often involve alterations of molecules on the surface of cells or phage. These programmed DNA rearrangements usually occur at a low frequency, thereby preadapting a small subset of the population to a change in environmental conditions, or in the case of phages, an expanded host range. A dedicated recombinase, sometimes with the aid of additional regulatory or DNA architectural proteins, catalyzes the inversion of DNA. RecA or other components of the general recombination-repair machinery are not involved. This chapter discusses site-specific DNA inversion reactions mediated by the serine recombinase family of enzymes and focuses on the extensively studied serine DNA invertases that are stringently controlled by the Fis-bound enhancer regulatory system. The first section summarizes biological features and general properties of inversion reactions by the Fis/enhancer-dependent serine invertases and the recently described serine DNA invertases in Bacteroides . Mechanistic studies of reactions catalyzed by the Hin and Gin invertases are then explored in more depth, particularly with regards to recent advances in our understanding of the function of the Fis/enhancer regulatory system. These include the steps leading to the formation of the active recombination complex (invertasome) containing the recombinase tetramer and Fis/enhancer element and the process of DNA strand exchange by rotation of synapsed subunit pairs within the invertasome. The role of DNA topological forces that function in concert with the Fis/enhancer controlling element in specifying the overwhelming bias for DNA inversion over deletion and intermolecular recombination is also discussed.

Published

2015

29. Determinants of HMGB Proteins Required To Promote RAG1/2-Recombination Signal Sequence Complex Assembly and Catalysis during V(D)J Recombination

Author

Yi-Meng Yen, Jongbum Kwon, Ben Wong, Marjorie A. Oettinger, Reid C. Johnson, and Yan Dai

Subjects

Saccharomyces cerevisiae Proteins, HMG-box, Phenylalanine, Molecular Sequence Data, chemical and pharmacologic phenomena, Chromosome Structure and Dynamics, Biology, chemistry.chemical_compound, Animals, Nucleosome, Amino Acid Sequence, HMGB1 Protein, VDJ Recombinases, Molecular Biology, Sequence Deletion, Gene Rearrangement, Homeodomain Proteins, DNA clamp, V(D)J recombination, High Mobility Group Proteins, Nuclear Proteins, DNA, Cell Biology, DNA-binding domain, Molecular biology, Protein Structure, Tertiary, Rats, DNA-Binding Proteins, Repressor Proteins, DNA binding site, chemistry, Naked DNA, Biophysics, HMGN Proteins

Abstract

Efficient assembly of RAG1/2-recombination signal sequence (RSS) DNA complexes that are competent for V(D)J cleavage requires the presence of the nonspecific DNA binding and bending protein HMGB1 or HMGB2. We find that either of the two minimal DNA binding domains of HMGB1 is effective in assembling RAG1/2-RSS complexes on naked DNA and stimulating V(D)J cleavage but that both domains are required for efficient activity when the RSS is incorporated into a nucleosome. The single-domain HMGB protein from Saccharomyces cerevisiae, Nhp6A, efficiently assembles RAG1/2 complexes on naked DNA; however, these complexes are minimally competent for V(D)J cleavage. Nhp6A forms much more stable DNA complexes than HMGB1, and a variety of mutations that destabilize Nhp6A binding to bent microcircular DNA promote increased V(D)J cleavage. One of the two DNA bending wedges on Nhp6A and the analogous phenylalanine wedge at the DNA exit site of HMGB1 domain A were found to be essential for promoting RAG1/2-RSS complex formation. Because the phenylalanine wedge is required for specific recognition of DNA kinks, we propose that HMGB proteins facilitate RAG1/2-RSS interactions by recognizing a distorted DNA structure induced by RAG1/2 binding. The resulting complex must be sufficiently dynamic to enable the series of RAG1/2-mediated chemical reactions on the DNA.

Published

2005

30. Architecture of the Hin Synaptic Complex during Recombination

Author

Reid C. Johnson, Gautam Dhar, and Erin R. Sanders

Subjects

0303 health sciences, Conformational change, Biochemistry, Genetics and Molecular Biology(all), Protein subunit, Synapsis, Biology, General Biochemistry, Genetics and Molecular Biology, Serine, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Biochemistry, chemistry, Recombinase, Biophysics, Tyrosine, 030217 neurology & neurosurgery, Recombination, DNA, 030304 developmental biology

Abstract

Most site-specific recombinases can be grouped into two mechanistically distinct families. Whereas tyrosine recombinases exchange DNA strands through a Holliday intermediate, serine recombinases such as Hin generate double-strand breaks in each recombining partner. Here, site-directed protein crosslinking is used to elucidate the configuration of protein subunits and DNA within the Hin synaptic complex and to follow the movement of protein subunits during DNA strand exchange. Our results show that the protein interface mediating synapsis is localized to a region within the catalytic domains, thereby positioning the DNA strands on the outside of the Hin tetrameric complex. Unexpected crosslinks between residues within the dimerization helices provide evidence for a conformational change that accompanies DNA cleavage. We demonstrate that the Hin subunits, which are linked to the cleaved DNA ends by serine-phosphodiester bonds, translocate between synapsed dimers to exchange the DNA strands.

Published

2004

31. Stepwise Dissection of the Hin-catalyzed Recombination Reaction from Synapsis to Resolution

Author

Reid C. Johnson and Erin R. Sanders

Subjects

DNA, Bacterial, Models, Molecular, Base Pair Mismatch, Base pair, Stereochemistry, Biology, law.invention, Structure-Activity Relationship, chemistry.chemical_compound, Salmonella, Structural Biology, law, Factor For Inversion Stimulation Protein, Serine, Site-specific recombination, Base Pairing, Molecular Biology, Recombination, Genetic, Binding Sites, Base Sequence, DNA, Superhelical, Oligonucleotide, Chromosome Pairing, Kinetics, Amino Acid Substitution, chemistry, Biochemistry, DNA Nucleotidyltransferases, Recombinant DNA, DNA supercoil, Dimerization, DNA

Abstract

The Hin DNA invertase promotes a site-specific DNA recombination reaction in the Salmonella chromosome. The native Hin reaction exhibits overwhelming selectivity for promoting inversions between appropriately oriented recombination sites and requires the Fis regulatory protein, a recombinational enhancer, and a supercoiled DNA substrate. Here, we report a robust recombination reaction employing oligonucleotide substrates and a hyperactive mutant form of Hin. Synaptic complex intermediates purified by gel electrophoresis were found to contain four Hin protomers bound to two recombination sites. Each Hin protomer is associated covalently with a cleaved DNA end. The cleaved complexes can be ligated into both parental and recombinant orientations at equivalent frequencies, provided the core residues can base-pair, and are readily disassembled into separated DNA fragments bound by Hin dimers. Kinetic analyses reveal that synapsis occurs rapidly, followed by comparatively slow Hin-catalyzed DNA cleavage. Subsequent steps of the reaction, including DNA exchange and ligation, are fast. Thus, post-synaptic step(s) required for DNA cleavage limit the overall rate of the recombination reaction.

Published

2004

32. Activation of transcription initiation from a stable RNA promoter by a Fis protein-mediated DNA structural transmission mechanism

Author

G. Wesley Hatfield, Walter M. Holmes, Craig J. Benham, Reid C. Johnson, Michael L. Opel, and Kimberly A. Aeling

Subjects

biology, General transcription factor, Transcription (biology), biology.protein, RNA polymerase II, Promoter, Transcription factor II D, Molecular Biology, Microbiology, RNA polymerase II holoenzyme, Molecular biology, Abortive initiation, Transcription bubble

Abstract

Summary The leuV operon of Escherichia coli encodes three of the four genes for the tRNA1Leu isoacceptors. Transcription from this and other stable RNA promoters is known to be affected by a cis-acting UP element and by Fis protein interactions with the carboxyl-terminal domain of the α-subunits of RNA polymerase. In this report, we suggest that transcription from the leuV promoter also is activated by a Fis-mediated, DNA supercoiling-dependent mechanism similar to the IHF-mediated mechanism described previously for the ilvPG promoter (S. D. Sheridan et al., 1998, J Biol Chem 273: 21298–21308). We present evidence that Fis binding results in the translocation of superhelical energy from the promoter-distal portion of a supercoiling-induced DNA duplex destabilized (SIDD) region to the promoter-proximal portion of the leuV promoter that is unwound within the open complex. A mutant Fis protein, which is defective in contacting the carboxyl-terminal domain of the α-subunits of RNA polymerase, remains competent for stimulating open complex formation, suggesting that this DNA supercoiling-dependent component of Fis-mediated activation occurs in the absence of specific protein interactions between Fis and RNA polymerase. Fis-mediated translocation of superhelical energy from upstream binding sites to the promoter region may be a general feature of Fis-mediated activation of transcription at stable RNA promoters, which often contain A+T-rich upstream sequences.

Published

2004

33. Differential Affinity and Cooperativity Functions of the Amino-terminal 70 Residues of λ Integrase

Author

Arthur Landy, Hideki Aihara, Tom Ellenberger, Reid C. Johnson, Marco A. Azaro, Simone E. Nunes-Düby, Radhakrishna S. Tirumalai, Christie V. Papagiannis, and Dibyendu Sarkar

Subjects

DNA, Bacterial, Threonine, HMG-box, Stereochemistry, Oligonucleotides, Cooperativity, Biology, Viral Proteins, Structural Biology, Amino Acid Sequence, Site-specific recombination, Binding site, Molecular Biology, Recombination, Genetic, Binding Sites, Base Sequence, Integrases, Cooperative binding, Bacteriophage lambda, Molecular biology, Recombinant Proteins, Protein Structure, Tertiary, DNA-Binding Proteins, DNA binding site, A-site, DNA Nucleotidyltransferases, DNA, Viral, Protein Binding, Binding domain

Abstract

The site-specific recombinase (Int) of bacteriophage lambda is a heterobivalent DNA-binding protein that binds two different classes of DNA-binding sites within its recombination target sites. The several functions of Int are apportioned between a large carboxy-terminal domain that cleaves and ligates DNA at each of its four "core-type" DNA-binding sites and a small amino-terminal domain, whose primary function is binding to each of its five "arm-type" DNA sites, which are distant from the core region. Int bridges between the two classes of binding sites are facilitated by accessory DNA-bending proteins that along with Int comprise higher-order recombinogenic complexes. We show here that although the 64 amino-terminal residues of Int bind efficiently to a single arm site, this protein cannot form doubly bound complexes on adjacent arm sites. However, 1-70 Int does show the same cooperative binding to adjacent arm sites as the full length protein. We also found that 1-70 Int specifies cooperative interactions with the accessory protein Xis when the two are bound to their adjacent cognate sites P2 and X1, respectively. To complement the finding that these two amino-terminal domain functions (along with arm DNA binding) are all specified by residues 1-70, we determined that Thr75 is the first residue of the minimal carboxy-terminal domain, thereby identifying a specific interdomain linker region. We have measured the affinity constants for Int binding to each of the five arm sites and the cooperativity factors for Int binding to the two pairs of adjacent arm sites, and we have identified several DNA structural features that contribute to the observed patterns of Int binding to arm sites. Taken together, the results highlight several interesting features of arm DNA binding that invite speculation about additional levels of complexity in the regulation of lambda site-specific recombination.

Published

2002

34. Regulation of Directionality in Bacteriophage λ Site-specific Recombination: Structure of the Xis Protein

Author

Jonathan M. Wojciak, Leah Corselli, James R. Lee, Christie V. Papagiannis, My D. Sam, Junji Iwahara, Robert T. Clubb, Martin L. Phillips, Kevin M. Connolly, and Reid C. Johnson

Subjects

Models, Molecular, Protein Conformation, Amino Acid Motifs, Protein Structure, Secondary, Bacteriophage, Structure-Activity Relationship, Viral Proteins, chemistry.chemical_compound, Lysogen, Structural Biology, Directionality, Site-specific recombination, Binding site, Nuclear Magnetic Resonance, Biomolecular, Molecular Biology, Recombination, Genetic, Genetics, Binding Sites, Base Sequence, Integrases, Models, Genetic, biology, Hydrogen Bonding, biology.organism_classification, Bacteriophage lambda, Recombinant Proteins, Protein Structure, Tertiary, Integrase, chemistry, Attachment Sites, Microbiological, DNA Nucleotidyltransferases, Mutagenesis, Site-Directed, Biophysics, biology.protein, Excisionase, DNA, Protein Binding

Abstract

Upon induction of a bacteriophage λ lysogen, a site-specific recombination reaction excises the phage genome from the chromosome of its bacterial host. A critical regulator of this process is the phage-encoded excisionase (Xis) protein, which functions both as a DNA architectural factor and by cooperatively recruiting integrase to an adjacent binding site specifically required for excision. Here we present the three-dimensional structure of Xis and the results of a structure-based mutagenesis study to define the molecular basis of its function. Xis adopts an unusual “winged”-helix motif that is modeled to interact with the major- and minor-grooves of its binding site through a single α-helix and loop structure (“wing”), respectively. The C-terminal tail of Xis, which is required for cooperative binding with integrase, is unstructured in the absence of DNA. We propose that asymmetric bending of DNA by Xis positions its unstructured C-terminal tail for direct contacts with the N-terminal DNA-binding domain of integrase and that an ensuing disordered to ordered transition of the tail may act to stabilize the formation of the tripartite integrase–Xis–DNA complex required for phage excision.

Published

2002

35. Identification of the tRNA-Dihydrouridine Synthase Family

Author

Paul Schimmel, Valérie de Crécy-Lagard, Reid C. Johnson, Anthony C. Bishop, and Jimin Xu

Subjects

Comparative genomics, Genetics, ATP synthase, biology, Cell Biology, medicine.disease_cause, Biochemistry, chemistry.chemical_compound, Plasmid, chemistry, Transfer RNA, Escherichia coli, biology.protein, medicine, Gene family, Dihydrouridine, Oxidoreductases, Molecular Biology, Gene, Genome, Bacterial, Plasmids

Abstract

5,6-Dihydrouridine (D) is a modified base found abundantly in the D-loops of tRNA from Archaea, Bacteria, and Eukarya. D is thought to be formed post-transcriptionally by the reduction of uridines in tRNA transcripts. Despite its abundance, no enzymes that catalyze D-formation have been identified. Using comparative genomics and computational methods we have identified members of the cluster of orthologous genes, COG0042, as putative dihydrouridine synthase encoding genes. Escherichia coli contains three COG0042 family members (yjbN, yhdG, and yohI). Strains were created where one, two, or all three of the COG0042 genes were deleted. Purified tRNA samples were investigated from the three single and the three double knockout strains, as well as from the triple deletion strain. The results showed that the COG0042 gene family is responsible for tRNA-dihydrouridine synthase activity in E. coli. They also suggest that the COG0042-encoded family members act site-specifically on the tRNA D-loop and contain non-redundant catalytic functions in vivo.

Published

2002

36. The DNA Architectural Protein HMGB1 Displays Two Distinct Modes of Action That Promote Enhanceosome Assembly

Author

Ben Wong, Katherine Mitsouras, Charina Arayata, Michael Carey, and Reid C. Johnson

Subjects

DNA Footprinting, DNA footprinting, chemical and pharmacologic phenomena, Biology, DNA-binding protein, Immediate early protein, Enhanceosome, Cell Line, Immediate-Early Proteins, Viral Proteins, Animals, HMGB1 Protein, Binding site, Enhancer, Molecular Biology, Transcriptional Regulation, Genetics, Binding Sites, Hydroxyl Radical, Protein footprinting, DNA, Cell Biology, Cell biology, DNA-Binding Proteins, DNA binding site, Enhancer Elements, Genetic, Mutation, Trans-Activators

Abstract

HMGB1 (also called HMG-1) is a DNA-bending protein that augments the affinity of diverse regulatory proteins for their DNA sites. Previous studies have argued for a specific interaction between HMGB1 and target proteins, which leads to cooperative binding of the complex to DNA. Here we propose a different model that emerged from studying how HMGB1 stimulates enhanceosome formation by the Epstein-Barr viral activator Rta on a target gene, BHLF-1. HMGB1 stimulates binding of individual Rta dimers to multiple sites in the enhancer. DNase I and hydroxyl radical footprinting, electrophoretic mobility shift assays, and immobilized template assays failed to reveal stable binding of HMGB1 within the complex. Furthermore, mutational analysis failed to identify a specific HMGB1 target sequence. The effect of HMGB1 on Rta could be reproduced by individual HMG domains, yeast HMO1, or bacterial HU. These results, combined with the effects of single-amino-acid substitutions within the DNA-binding surface of HMGB1 domain A, argue for a mechanism whereby DNA-binding and bending by HMGB1 stimulate Rta-DNA complex formation in the absence of direct interaction with Rta or a specific HMGB1 target sequence. The data contrast with our analysis of HMGB1 action on another BHLF-1 regulatory protein called ZEBRA. We discuss the two distinct modes of HMGB1 action on a single regulatory region and propose how HMGB1 can function in diverse contexts.

Published

2002

37. Subunit Exchange and the Role of Dimer Flexibility in DNA Binding by the Fis Protein

Author

Reid C. Johnson, Erin R. Sanders, José Luis Vázquez-Ibar, and Stacy K. Merickel

Subjects

chemistry.chemical_compound, Förster resonance energy transfer, Protein structure, HMG-box, chemistry, Bacterial DNA binding protein, Stereochemistry, Dimer, Protein subunit, Factor For Inversion Stimulation Protein, Biochemistry, DNA

Abstract

Fis is an abundant bacterial DNA binding protein that functions in many different reactions. We show here that Fis subunits rapidly exchange between dimers in solution by disulfide cross-linking mixtures of Fis mutants with different electrophoretic mobilities and by monitoring energy transfer between fluorescently labeled Fis subunits upon heterodimer formation. The effects of detergents and salt concentrations on subunit exchange imply that the dimer is predominantly stabilized by hydrophobic forces, consistent with the X-ray crystal structures. Specific and nonspecific DNA strongly inhibit Fis subunit exchange. In all crystal forms of Fis, the separation between the DNA recognition helices within the Fis dimer is too short to insert into adjacent major grooves on canonical B-DNA, implying that conformational changes within the Fis dimer and/or the DNA must occur upon binding. We therefore investigated the functional importance of dimer interface flexibility for Fis-DNA binding by studying the DNA binding properties of Fis mutants that were cross-linked at different positions in the dimer. Flexibility within the core dimer interface does not appear to be required for efficient DNA binding, Fis-DNA complex dissociation, or Fis-induced DNA bending. Moreover, FRET-based experiments provided no evidence for a change in the spatial relationship between the two helix-turn-helix motifs in the Fis dimer upon DNA binding. These results support a model in which the unusually short distance between DNA recognition helices on Fis is accommodated primarily through bending of the DNA.

Published

2002

38. Binding to Cisplatin-Modified DNA by the Saccharomyces cerevisiae HMGB Protein Nhp6A

Author

Ben, Wong, James E, Masse, Yi-Meng, Yen, Petros, Giannikopoulos, Juli, Feigon, Reid C, Johnson, and Petros, Giannikoupolous

Subjects

Saccharomyces cerevisiae Proteins, HMG-box, Base pair, DNA damage, Phenylalanine, Amino Acid Motifs, Molecular Sequence Data, Mutant, DNA Footprinting, DNA footprinting, Saccharomyces cerevisiae, Biology, Biochemistry, DNA-binding protein, DNA Adducts, chemistry.chemical_compound, Methionine, HMGB Proteins, medicine, Animals, Amino Acid Sequence, Nuclear Magnetic Resonance, Biomolecular, Cisplatin, Nuclear Proteins, Molecular biology, Peptide Fragments, Rats, DNA-Binding Proteins, Cross-Linking Reagents, chemistry, Mutagenesis, Site-Directed, HMGN Proteins, Electrophoresis, Polyacrylamide Gel, Copper, DNA, DNA Damage, Phenanthrolines, Protein Binding, medicine.drug

Abstract

Nhp6A is an abundant non-histone chromatin-associated protein in Saccharomyces cerevisiae that contains a minor groove DNA binding motif called the HMG box. In this report, we show that Nhp6Ap binds to cisplatin intrastrand cross-links on duplex DNA with a 40-fold greater affinity than to unmodified DNA with the same sequence. Nevertheless, Nhp6Ap bound to cisplatinated DNA readily exchanges onto unmodified DNA. Phenanthroline-copper footprinting and two-dimensional NMR on complexes of wild-type and mutant Nhp6Ap with DNA were employed to probe the mode of binding to the cisplatin lesion. Recognition of the cisplatin adduct requires a surface-exposed phenylalanine on Nhp6Ap that promotes bending of DNA by inserting into the helix from the minor groove. We propose that Nhp6Ap targets the cisplatin adduct by means of intercalation by the phenylalanine and that it can bind in either orientation with respect to the DNA lesion. A methionine, which also inserts between base pairs and functions in target selection on unmodified DNA, plays no apparent role in recognition of the cisplatin lesion. Basic amino acids within the N-terminal arm of Nhp6Ap are required for high-affinity binding to the cisplatin adduct as well as to unmodified DNA. Cisplatin mediates its cytotoxicity by forming covalent adducts on DNA, and we find that Deltanhp6a/b mutants are hypersensitive to cisplatin in comparison with the wild-type strain. In contrast, Deltanhp6a/b mutants are slightly more resistant to hydrogen peroxide and ultraviolet irradiation. Therefore, Nhp6A/Bp appears to directly or indirectly function in yeast to enhance cellular resistance to cisplatin.

Published

2002

39. Testing water-mediated DNA recognition by the Hin recombinase

Author

Thang Kien Chiu, Reid C. Johnson, Richard E. Dickerson, and Catherine S. Sohn

Subjects

Protein Conformation, Stereochemistry, Molecular Sequence Data, Mutant, Helix-turn-helix, Biology, Crystallography, X-Ray, Article, General Biochemistry, Genetics and Molecular Biology, chemistry.chemical_compound, Protein structure, Amino Acid Sequence, Molecular Biology, Peptide sequence, DNA Nucleotidyltransferases, Base Sequence, General Immunology and Microbiology, General Neuroscience, Water, DNA, Molecular biology, Thymine, chemistry, Hin recombinase

Abstract

The Hin recombinase specifically recognizes its DNA-binding site by means of both major and minor groove interactions. A previous X-ray structure, together with new structures of the Hin DNA-binding domain bound to a recombination half-site that were solved as part of the present study, have revealed that two ordered water molecules are present within the major groove interface. In this report, we test the importance of these waters directly by X-ray crystal structure analysis of complexes with four mutant DNA sequences. These structures, combined with their Hin-binding properties, provide strong support for the critical importance of one of the intermediate waters. A lesser but demonstrable role is ascribed to the second water molecule. The mutant structures also illustrate the prominent roles of thymine methyls both in stabilizing intermediate waters and in interfering with water or amino acid side chain interactions with DNA.

Published

2002

40. Architecture of fis-activated transcription complexes at the Escherichia coli rrnB P1 and rrnE P1 promoters

Author

Reid C. Johnson, Wilma Ross, Richard L. Gourse, Sarah M. McLeod, Sarah E. Aiyar, Mark S. Thomas, and Christine A. Hirvonen

Subjects

Integration Host Factors, Models, Molecular, Transcription, Genetic, Macromolecular Substances, Protein subunit, DNA Footprinting, Biology, chemistry.chemical_compound, Structural Biology, Transcription (biology), Factor For Inversion Stimulation Protein, RNA polymerase, Escherichia coli, rRNA Operon, Promoter Regions, Genetic, Protein Structure, Quaternary, Molecular Biology, Transcription factor, G alpha subunit, Genetics, Binding Sites, Base Sequence, Hydroxyl Radical, Activator (genetics), Escherichia coli Proteins, Promoter, Protein Subunits, chemistry, Trans-Activators, Nucleic Acid Conformation, Carrier Proteins, Dimerization, DNA, Protein Binding

Abstract

The transcription factor Fis activates the Escherichia coli rRNA promoters rrnB P1 and rrnE P1 by binding to sites centered at -71 and -72, respectively, and interacting with the C-terminal domain of the alpha subunit of RNA polymerase (RNAP alphaCTD). To understand the mechanism of activation by Fis at these promoters, we used oriented alpha-heterodimeric RNAPs and heterodimers of Fis to determine whether one or both subunits of alpha and Fis participate in the alphaCTD-Fis interaction. Our results imply that only one alphaCTD in the alpha dimer and only one activation-proficient subunit in the Fis dimer are required for activation by Fis. A library of alanine substitutions in alpha was used to identify the alphaCTD determinants required for Fis-dependent transcription at rrnB P1 and rrnE P1. We propose that the transcriptional activation region of the promoter-proximal subunit of the Fis dimer interacts with a determinant that includes E273 of one alphaCTD to activate transcription. We further suggest that the Fis contact to alphaCTD results in alphaCTD interactions with DNA that differ somewhat from those that occur at UP elements in the absence of Fis. The accompanying paper shows that the 273 determinant on alphaCTD is also targeted by Fis at the proP P2 promoter where the activator binds overlapping the -35 hexamer. Thus, similar Fis-alphaCTD interactions are used for activation of transcription when the activator is bound at very different positions on the DNA.

Published

2002

41. The C-terminal domains of the RNA polymerase α subunits: contact site with fis and localization during co-activation with CRP at the Escherichia coli proP P2 promoter

Author

Reid C. Johnson, Sarah E. Aiyar, Richard L. Gourse, and Sarah M. McLeod

Subjects

Integration Host Factors, Models, Molecular, Transcriptional Activation, Cyclic AMP Receptor Protein, Protein subunit, Random hexamer, Biology, chemistry.chemical_compound, Transactivation, Structural Biology, Transcription (biology), Factor For Inversion Stimulation Protein, RNA polymerase, Escherichia coli, Promoter Regions, Genetic, Molecular Biology, Binding Sites, Symporters, Escherichia coli Proteins, Promoter, DNA-Directed RNA Polymerases, Gene Expression Regulation, Bacterial, Molecular biology, Protein Structure, Tertiary, Protein Subunits, A-site, chemistry, Genes, Bacterial, Mutation, Carrier Proteins, Dimerization, DNA, Protein Binding

Abstract

Fis is a versatile transactivator that functions at many different promoters. Fis activates transcription at the RpoS-dependent proP P2 promoter when bound to a site that overlaps the minus sign35 hexamer by a mechanism that requires the C-terminal domain of the alpha subunit of RNA polymerase (alphaCTD). The region on Fis responsible for activating transcription through the alphaCTD has been localized to a short beta-turn near the DNA-binding determinant on one subunit of the Fis homodimer. We report here that Fis-dependent activation of proP P2 transcription requires two discrete regions on the alphaCTD. One region, consisting of residues 264-265 and 296-297, mediates DNA binding. A second patch, comprising amino acid residues 271-273, forms a ridge on the surface of the alphaCTD that we propose interacts with Fis. The accompanying paper shows that these same regions on alphaCTD are utilized for transcriptional activation at the rrnB and rrnE P1 promoters by Fis bound to a site upstream of the core promoter (centered at minus sign71/minus sign72). In addition to stimulation of proP P2 transcription by Fis, CRP co-activates this promoter when bound to a remote site upstream from the promoter (centered at -121.5). RNA polymerase preparations lacking one alphaCTD of the alpha dimer were employed to demonstrate that the beta'-associated alpha(II)CTD was utilized preferentially by Fis at proP P2 in the presence and absence of CRP. These experiments define the overall architecture of the proP P2 initiation complex where Fis and CRP each function through a different alphaCTD.

Published

2002

42. Major Nucleoid Proteins in the Structure and Function of theEscherichia coliChromosome

Author

Reid C. Johnson, Jeffrey F. Gardner, John W. Schmidt, and Lianna M. Johnson

Subjects

Genetics, Base pair, Mutant, Consensus sequence, DNA replication, bacteria, DNA supercoil, Chromosome, Nucleoid, Biology, Gene

Abstract

This chapter focuses on the major nucleoid-associated proteins and summarizes one's current knowledge of how these proteins contribute to the structure of the nucleoid and function in specific reactions involving the chromosome. The current view is that the Escherichia coli nucleoid is dominated by five different proteins: HU, integration host factor (IHF), H-NS, StpA and Fis under nutrient-rich exponential growth conditions. HU mutant cells display the most severe and varied phenotypes in comparison to strains containing mutations in the other major nucleoid proteins. Supercoiling of chromosomal and plasmid DNA is partially relaxed in mutants lacking HU, supporting an in vivo role for HU in regulating the degree of supercoiling. HU plays several interconnected roles in DNA replication and appears to be involved in several steps involving initiation of chromosomal DNA synthesis, chromosomal partitioning, and cell division. The genes that were differentially expressed were examined for putative IHF binding sites in the 500 bp upstream of the transcription initiation site. The criteria for identifying high-affinity sites were that the sites must have a 12 out of 13 bp match with the core consensus sequence and that at least 10 of the 15 bp 5' (upstream) to the core consensus must be dA-dT base pairs. The study identified 46 candidates that matched the criteria, some of which were documented in other studies. The study also identified seven genes, including ihfA, that were expressed only when IHF was present and eight genes that were expressed only in IHF-deficient cells.

Published

2014

43. Nuclear Localization of theSaccharomyces cerevisiaeHMG Protein NHP6A Occurs by a Ran-Independent Nonclassical Pathway

Author

Yi-Meng Yen, Paul M. Roberts, and Reid C. Johnson

Subjects

Nuclear cap-binding protein complex, Cell Biology, Importin, Biology, Biochemistry, Cell biology, Structural Biology, Ran, Genetics, Nuclear lamina, Nuclear transport, Nuclear protein, Nuclear export signal, Molecular Biology, Nuclear localization sequence

Abstract

The Saccharomyces cerevisiae non-histone protein 6-A (NHP6A) is a member of the high-mobility group 1/2 protein family that bind and bend DNA of mixed sequence. NHP6A has only one high-mobility group 1/2 DNA binding domain and also requires a 16-amino-acid basic tail at its N-terminus for DNA binding. We show in this report that nuclear accumulation of NHP6A is strictly correlated with its DNA binding properties since only nonhistone protein 6 A-green fluorescent protein chimeras that were competent for DNA binding were localized to the nucleus. Despite the requirement for basic residues within the N-terminal segment for DNA binding and nuclear accumulation, this region does not appear to contain a nuclear localization signal. Moreover, NHP6A does not bind to the yeast nuclear localization signal receptor SRP1 and nuclear targeting of NHP6A does not require the function of the 14 different importins. Unlike histone H2B1 which contains a classical nuclear localization signal, entry of NHP6A into the nucleus was found to be independent of Ran as judged by coexpression of Ran GTPase mutants and was shown to occur at 0 degrees C after a 15-min induction. These unusual properties lead us to suggest that NHP6A entry into the nucleus proceeds by a nonclassical Ran-independent pathway.

Published

2001

44. Coactivation of the RpoS-Dependent proP P2 Promoter by Fis and Cyclic AMP Receptor Protein

Author

Jimin Xu, Sarah M. McLeod, and Reid C. Johnson

Subjects

DNA, Bacterial, Integration Host Factors, Transcriptional Activation, Cyclic AMP Receptor Protein, Molecular Sequence Data, DNA Footprinting, DNA footprinting, Sigma Factor, Genetics and Molecular Biology, Biology, Microbiology, chemistry.chemical_compound, Bacterial Proteins, Sigma factor, Transcription (biology), Factor For Inversion Stimulation Protein, RNA polymerase, Binding site, Promoter Regions, Genetic, Molecular Biology, Binding Sites, Base Sequence, Symporters, Escherichia coli Proteins, Drug Synergism, DNA-Directed RNA Polymerases, Molecular biology, chemistry, Electrophoresis, Polyacrylamide Gel, Carrier Proteins, rpoS

Abstract

The Escherichia coli proP P2 promoter, which directs the expression of an integral membrane transporter of proline, glycine betaine, and other osmoprotecting compounds, is induced upon entry into stationary phase to protect cells from osmotic shock. Transcription from the P2 promoter is completely dependent on RpoS (ς 38 ) and Fis. Fis activates transcription by binding to a site centered at −41, which overlaps the promoter, where it makes a specific contact with the C-terminal domain of the α subunit of RNA polymerase (α-CTD). We show here that Fis and cyclic AMP (cAMP) receptor protein (CRP)-cAMP collaborate to activate transcription synergistically in vitro. Coactivation both in vivo and in vitro is dependent on CRP binding to a site centered at −121.5, but CRP without Fis provides little activation. The contribution by CRP requires the correct helical phasing of the CRP site and a functional activation region 1 on CRP. We provide evidence that coactivation is achieved by Fis and CRP independently contacting each of the two α-CTDs. Efficient transcription in vitro requires that both activators must be preincubated with the DNA prior to addition of RNA polymerase.

Published

2000

45. The cAMP receptor protein CRP can function as an osmoregulator of transcription in Escherichia coli

Author

Lenore Landis, Reid C. Johnson, and Jimin Xu

Subjects

DNA, Bacterial, Cyclic AMP Receptor Protein, Transcription, Genetic, Molecular Sequence Data, Catabolite repression, Repressor, lac operon, Lac repressor, Biology, Bacterial Proteins, stomatognathic system, Cyclic AMP, Escherichia coli, Lac Repressors, Genetics, Promoter Regions, Genetic, Derepression, Base Sequence, Symporters, Osmotic concentration, Escherichia coli Proteins, Osmolar Concentration, Promoter, Gene Expression Regulation, Bacterial, Water-Electrolyte Balance, Molecular biology, humanities, Repressor Proteins, Lac Operon, cAMP receptor protein, biology.protein, Carrier Proteins, Research Paper, Developmental Biology

Abstract

Transcription of the P1 promoter of the Escherichia coli proP gene, which encodes a transporter of osmoprotectants, is strongly induced by a shift to hyperosmotic media. Unlike most other osmotically regulated promoters, the induction occurs for a brief period of time, corresponding to the replacement of intracellular K(+) glutamate with osmoprotecting compounds. This burst of proP transcription is correlated with the osmolarity-dependent binding of the cAMP receptor protein CRP to a site within the proP P1 promoter. We show that CRP-cAMP functions as an osmotically sensitive repressor of proP P1 transcription in vitro. Binding of CRP to the proP promoter in vivo is transiently destabilized after a hyperosmotic shift with kinetics that correspond to the derepression of transcription, whereas Fis and Lac repressor binding is not osmotically sensitive. Similar osmotic regulation of proP P1 transcription by the CRP* mutant implies that binding of cAMP is not responsible for the unusual osmotic sensitivity of CRP activity. Osmotic regulation of CRP activity is not limited to proP. Activation of the lac promoter by CRP is also transiently inhibited after an osmotic upshift, as is the binding of CRP to the galdelta4P1 promoter. These findings suggest that CRP functions in certain contexts to regulate gene expression in response to osmotic changes, in addition to its role in catabolite control.

Published

1999

46. Assembly of a Tightly Interwound DNA Recombination Complex Poised for Deletion

Author

John K. Heiss and Reid C. Johnson

Subjects

Genetics, Protein subunit, Cell, Biology, Cell biology, law.invention, Serine, chemistry.chemical_compound, medicine.anatomical_structure, chemistry, Structural Biology, law, Recombinase, medicine, Recombinant DNA, Molecular Biology, DNA

Abstract

In a recent issue of Molecular Cell, Mouw et al. (2008) report a crystal structure of a serine recombinase bound to a regulatory DNA site in an unexpected synaptic complex configuration, which forms the framework for a new model of the entire 12 subunit, 186 bp deletion complex.

Published

2008

47. Communication between Hin recombinase and Fis regulatory subunits during coordinate activation of Hin-catalyzed site-specific DNA inversion

Author

Stacy K. Merickel, Reid C. Johnson, and Michael J. Haykinson

Subjects

Integration Host Factors, Models, Molecular, Transcriptional Activation, Conformational change, Macromolecular Substances, Stereochemistry, Dimer, Protein subunit, Biology, Protein Structure, Secondary, chemistry.chemical_compound, Factor For Inversion Stimulation Protein, Genetics, Point Mutation, Enhancer, Recombination, Genetic, Invertasome, DNA, Recombinant Proteins, Enhancer Elements, Genetic, Biochemistry, chemistry, Chromosome Inversion, DNA Nucleotidyltransferases, DNA Transposable Elements, Mutagenesis, Site-Directed, Nucleic Acid Conformation, Hin recombinase, Carrier Proteins, Dimerization, Research Paper, Developmental Biology

Abstract

The Hin DNA invertase becomes catalytically activated when assembled in an invertasome complex containing two Fis dimers bound to an enhancer segment. The region of Fis responsible for transactivation of Hin contains a mobile β-hairpin arm that extends from each dimer subunit. We show here that whereas both Fis dimers must be capable of activating Hin, Fis heterodimers that have only one functional activating β-arm are sufficient to form catalytically competent invertasomes. Analysis of homodimer and heterodimer mixes of different Hin mutants suggests that Fis must activate each subunit of the two Hin dimers that participate in catalysis. These experiments also indicate that all four Hin subunits must be coordinately activated prior to initiation of the first chemical step of the reaction and that the process of activation is independent of the catalytic steps of recombination. We propose a molecular model for the invertasome structure that is consistent with current information on protein–DNA structures and the topology of the DNA strands within the recombination complex. In this model, a single Fis activation arm could contact amino acids from both Hin subunits at the dimer interface to induce a conformational change that coordinately positions the active sites close to the scissile phosphodiester bonds.

Published

1998

48. Conversion of a β-strand to anα-helix induced by a single-site mutation observed in the crystal structure of fis mutant pro26Ala

Author

Leah Corselli, Tzu-Ping Ko, Wei-Zen Yang, Reid C. Johnson, and Hanna S. Yuan

Subjects

Integration Host Factors, Models, Molecular, Conformational change, Stereochemistry, Protein subunit, Molecular Sequence Data, Mutant, Peptide, Biology, Crystallography, X-Ray, Biochemistry, Protein Structure, Secondary, Bacterial Proteins, Factor For Inversion Stimulation Protein, Escherichia coli, Amino Acid Sequence, Disulfides, Molecular Biology, Peptide sequence, Protein secondary structure, Alanine, chemistry.chemical_classification, Escherichia coli Proteins, chemistry, Mutation, Carrier Proteins, Dimerization, Alpha helix, Research Article

Abstract

The conversion from an alpha-helix to a beta-strand has received extensive attention since this structural change may induce many amyloidogenic proteins to self-assemble into fibrils and cause fatal diseases. Here we report the conversion of a peptide segment from a beta-strand to an alpha-helix by a single-site mutation as observed in the crystal structure of Fis mutant Pro26Ala determined at 2.0 A resolution. Pro26 in Fis occurs at the point where a flexible extended beta-hairpin arm leaves the core structure. Thus it can be classified as a "hinge proline" located at the C-terminal end of the beta2-strand and the N-terminal cap of the A alpha-helix. The replacement of Pro26 to alanine extends the A alpha-helix for two additional turns in one of the dimeric subunits; therefore, the structure of the peptide from residues 22 to 26 is converted from a beta-strand to an alpha-helix. This result confirms the structural importance of the proline residue located at the hinge region and may explain the mutant's reduced ability to activate Hin-catalyzed DNA inversion. The peptide (residues 20 to 26) in the second monomer subunit presumably retains its beta-strand conformation in the crystal; therefore, this peptide shows a "chameleon-like" character since it can adopt either an alpha-helix or a beta-strand structure in different environments. The structure of Pro26Ala provides an additional example where not only the protein sequence, but also non-local interactions determine the secondary structure of proteins.

Published

1998

49. Determinants of DNA Binding and Bending by theSaccharomyces cerevisiae High Mobility Group Protein NHP6A That Are Important for Its Biological Activities

Author

Ben Wong, Yi-Meng Yen, and Reid C. Johnson

Subjects

Invertasome, chemistry.chemical_classification, HMG-box, Cell Biology, Biology, Biochemistry, Protein tertiary structure, Amino acid, DNA binding site, chemistry.chemical_compound, High-mobility group, chemistry, Transcription (biology), Molecular Biology, DNA

Abstract

The non-histone proteins 6A/B (NHP6A/B) ofSaccharomyces cerevisiae are high mobility group proteins that bind and severely bend DNA of mixed sequence. They exhibit high affinity for linear DNA and even higher affinity for microcircular DNA. The 16-amino acid basic segment located N-terminal to the high mobility group domain is required for stable complex formation on both linear and microcircular DNA. Although mutants lacking the N terminus are able to promote microcircle formation and Hin invertasome assembly at high protein concentrations, they are unable to form stable complexes with DNA, co-activate transcription, and complement the growth defect ofΔnhp6a/b mutants. A basic patch between amino acids 13 and 16 is critical for these activities, and a second basic patch between residues 8 and 10 is required for the formation of monomeric complexes with linear DNA. Mutational analysis suggests that proline 18 may direct the path of the N-terminal arm to facilitate DNA binding, whereas the conserved proline at position 21, tyrosine 28, and phenylalanine 31 function to maintain the tertiary structure of the high mobility group domain. Methionine 29, which may intercalate into DNA, is essential for NHP6A-induced microcircle formation of 75-bp but not 98-bp fragments in vitro, and for full growth complementation of Δnhp6a/b mutants in vivo.

Published

1998

50. The transactivation region of the Fis protein that controls site-specific DNA inversion contains extended mobile beta -hairpin arms

Author

Sarah E. Cramton, Reid C. Johnson, Leah Corselli, Wei-Zen Yang, Martin K. Safo, and Hanna S. Yuan

Subjects

Integration Host Factors, Models, Molecular, Beta hairpin, DNA Mutational Analysis, Molecular Sequence Data, Biology, Crystallography, X-Ray, Protein Structure, Secondary, General Biochemistry, Genetics and Molecular Biology, chemistry.chemical_compound, Transactivation, Factor For Inversion Stimulation Protein, Recombinase, Computer Simulation, Amino Acid Sequence, Cysteine, Saturated mutagenesis, Enhancer, Molecular Biology, Recombination, Genetic, Invertasome, General Immunology and Microbiology, General Neuroscience, chemistry, Biochemistry, DNA Nucleotidyltransferases, Trans-Activators, Biophysics, Carrier Proteins, Oxidation-Reduction, DNA, Research Article

Abstract

The Fis protein regulates site-specific DNA inversion catalyzed by a family of DNA invertases when bound to a cis-acting recombinational enhancer. As is often found for transactivation domains, previous crystal structures have failed to resolve the conformation of the N-terminal inversion activation region within the Fis dimer. A new crystal form of a mutant Fis protein now reveals that the activation region contains two beta-hairpin arms that protrude over 20 A from the protein core. Saturation mutagenesis identified the regulatory and structurally important amino acids. The most critical activating residues are located near the tips of the beta-arms. Disulfide cross-linking between the beta-arms demonstrated that they are highly flexible in solution and that efficient inversion activation can occur when the beta-arms are covalently linked together. The emerging picture for this regulatory motif is that contacts with the recombinase at the tip of the mobile beta-arms activate the DNA invertase in the context of an invertasome complex.

Published

1997