Your search keyword '"Gourse RL"' showing total 155 results

1. 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

2. Regulation of Chlamydia Gene Expression by Tandem Promoters with Different Temporal Patterns

Author

Ming Tan, Christopher J. Rosario, and Gourse, RL

Subjects

0301 basic medicine, Time Factors, Operon, 030106 microbiology, Sigma Factor, Biology, 2.2 Factors relating to physical environment, Microbiology, Medical and Health Sciences, Promoter Regions, Sexually Transmitted Diseases/Herpes, 03 medical and health sciences, chemistry.chemical_compound, Bacterial Proteins, Genetic, Sigma factor, RNA polymerase, Gene expression, Transcriptional regulation, Genetics, 2.2 Factors relating to the physical environment, Aetiology, Chlamydia, Molecular Biology, Gene, Regulation of gene expression, Agricultural and Veterinary Sciences, Bacterial, Promoter, Articles, Biological Sciences, Infectious Diseases, chemistry, Gene Expression Regulation, Sexually Transmitted Infections, Infection, Transcription, Biotechnology

Abstract

Chlamydia is a genus of pathogenic bacteria with an unusual intracellular developmental cycle marked by temporal waves of gene expression. The three main temporal groups of chlamydial genes are proposed to be controlled by separate mechanisms of transcriptional regulation. However, we have noted genes with discrepancies, such as the early gene dnaK and the midcycle genes bioY and pgk , which have promoters controlled by the late transcriptional regulators EUO and σ 28 . To resolve this issue, we analyzed the promoters of these three genes in vitro and in Chlamydia trachomatis bacteria grown in cell culture. Transcripts from the σ 28 -dependent promoter of each gene were detected only at late times in the intracellular infection, bolstering the role of σ 28 RNA polymerase in late gene expression. In each case, however, expression prior to late times was due to a second promoter that was transcribed by σ 66 RNA polymerase, which is the major form of chlamydial polymerase. These results demonstrate that chlamydial genes can be transcribed from tandem promoters with different temporal profiles, leading to a composite expression pattern that differs from the expression profile of a single promoter. In addition, tandem promoters allow a gene to be regulated by multiple mechanisms of transcriptional regulation, such as DNA supercoiling or late regulation by EUO and σ 28 . We discuss how tandem promoters broaden the repertoire of temporal gene expression patterns in the chlamydial developmental cycle and can be used to fine-tune the expression of specific genes. IMPORTANCE Chlamydia is a pathogenic bacterium that is responsible for the majority of infectious disease cases reported to the CDC each year. It causes an intracellular infection that is characterized by coordinated expression of chlamydial genes in temporal waves. Chlamydial transcription has been shown to be regulated by DNA supercoiling, alternative forms of RNA polymerase, and transcription factors, but the number of transcription factors found in Chlamydia is far fewer than the number found in most bacteria. This report describes the use of tandem promoters that allow the temporal expression of a gene or operon to be controlled by more than one regulatory mechanism. This combinatorial strategy expands the range of expression patterns that are available to regulate chlamydial genes.

Published

2015

3. Chlamydia trachomatis Type III Secretion Proteins Regulate Transcription

Author

Anatoly Slepenkin, Ellena M. Peterson, Brett R. Hanson, Ming Tan, and Gourse, RL

Subjects

Enzymologic, Transcription, Genetic, Down-Regulation, Chlamydia trachomatis, Sigma Factor, medicine.disease_cause, 2.2 Factors relating to physical environment, Medical and Health Sciences, Microbiology, Gene Expression Regulation, Enzymologic, Sexually Transmitted Diseases/Herpes, chemistry.chemical_compound, Bacterial Proteins, Genetic, Sigma factor, Transcription (biology), RNA polymerase, Gene expression, medicine, Type III Secretion Systems, Genetics, Humans, 2.2 Factors relating to the physical environment, Aetiology, Molecular Biology, Gene, Regulation of gene expression, biology, Agricultural and Veterinary Sciences, Bacterial, Gene Expression Regulation, Bacterial, Articles, DNA-Directed RNA Polymerases, Biological Sciences, Molecular biology, Infectious Diseases, chemistry, Gene Expression Regulation, Chaperone (protein), Hela Cells, biology.protein, Sexually Transmitted Infections, Infection, Transcription, HeLa Cells

Abstract

The Scc4 protein (CT663) of the pathogenic bacterium Chlamydia has been described as a type III secretion (T3S) chaperone as well as an inhibitor of RNA polymerase. To examine if these roles are connected, we first investigated physical interactions between Chlamydia trachomatis Scc4 and the T3S chaperone Scc1 and a T3S substrate, CopN. In a yeast 3-hybrid assay, Scc4, Scc1, and CopN were all required to detect an interaction, which suggests that these proteins form a trimolecular complex. We also detected interactions between any two of these three T3S proteins in a pulldown assay using only recombinant proteins. We next determined whether these interactions affected the function of Scc4 as an inhibitor of RNA transcription. Using Escherichia coli as a heterologous in vivo system, we demonstrated that expression of C. trachomatis Scc4 led to a drastic decrease in transcript levels for multiple genes. However, coexpression of Scc4 with Scc1, CopN, or both alleviated Scc4-mediated inhibition of transcription. Scc4 expression also severely impaired E. coli growth, but this growth defect was reversed by coexpression of Scc4 with Scc1, CopN, or both, suggesting that the inhibitory effect of Scc4 on transcription and growth can be antagonized by interactions between Scc4, Scc1, and CopN. These findings suggest that the dual functions of Scc4 may serve as a bridge to link T3S and the regulation of gene expression in Chlamydia . IMPORTANCE This study investigates a novel mechanism for regulating gene expression in the pathogenic bacterium Chlamydia . The Chlamydia type III secretion (T3S) chaperone Scc4 has been shown to inhibit transcription by RNA polymerase. This study describes physical interactions between Scc4 and the T3S proteins Scc1 and CopN. Furthermore, Chlamydia Scc1 and CopN antagonized the inhibitory effects of Scc4 on transcription and growth in a heterologous Escherichia coli system. These results provide evidence that transcription in Chlamydia can be regulated by the T3S system through interactions between T3S proteins.

Published

2015

4. Identification and characterization of RNA binding sites for (p)ppGpp using RNA-DRaCALA.

Author

Jagodnik J, Tjaden B, Ross W, and Gourse RL

Subjects

Binding Sites, Ligands, Riboswitch, RNA, Bacterial genetics, Aptamers, Nucleotide chemistry, Guanosine Pentaphosphate metabolism, Biochemistry methods

Abstract

Ligand-binding RNAs (RNA aptamers) are widespread in the three domains of life, serving as sensors of metabolites and other small molecules. When aptamers are embedded within RNA transcripts as components of riboswitches, they can regulate gene expression upon binding their ligands. Previous methods for biochemical validation of computationally predicted aptamers are not well-suited for rapid screening of large numbers of RNA aptamers. Therefore, we utilized DRaCALA (Differential Radial Capillary Action of Ligand Assay), a technique designed originally to study protein-ligand interactions, to examine RNA-ligand binding, permitting rapid screening of dozens of RNA aptamer candidates concurrently. Using this method, which we call RNA-DRaCALA, we screened 30 ykkC family subtype 2a RNA aptamers that were computationally predicted to bind (p)ppGpp. Most of the aptamers bound both ppGpp and pppGpp, but some strongly favored only ppGpp or pppGpp, and some bound neither. Expansion of the number of biochemically verified sites allowed construction of more accurate secondary structure models and prediction of key features in the aptamers that distinguish a ppGpp from a pppGpp binding site. To demonstrate that the method works with other ligands, we also used RNA DRaCALA to analyze aptamer binding by thiamine pyrophosphate., (© The Author(s) 2023. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2023

5. Homologs of the Escherichia coli F Element Protein TraR, Including Phage Lambda Orf73, Directly Reprogram Host Transcription.

Author

Gopalkrishnan S, Ross W, Akbari MS, Li X, Haycocks JRJ, Grainger DC, Court DL, and Gourse RL

Subjects

Bacteriophage lambda genetics, DNA-Directed RNA Polymerases genetics, DNA-Directed RNA Polymerases metabolism, Gene Expression Regulation, Bacterial, Guanosine Tetraphosphate metabolism, Transcription Factors metabolism, Transcription, Genetic, Escherichia coli genetics, Escherichia coli metabolism, Escherichia coli Proteins metabolism

Abstract

Bacterial cells and their associated plasmids and bacteriophages encode numerous small proteins of unknown function. One example, the 73-amino-acid protein TraR, is encoded by the transfer operon of the conjugative F plasmid of Escherichia coli. TraR is a distant homolog of DksA, a protein found in almost all proteobacterial species that is required for ppGpp to regulate transcription during the stringent response. TraR and DksA increase or decrease transcription initiation depending on the kinetic features of the promoter by binding directly to RNA polymerase without binding to DNA. Unlike DksA, whose full activity requires ppGpp as a cofactor, TraR is fully active by itself and unaffected by ppGpp. TraR belongs to a family of divergent proteins encoded by proteobacterial bacteriophages and other mobile elements. Here, we experimentally addressed whether other members of the TraR family function like the F element-encoded TraR. Purified TraR and all 5 homologs that were examined bound to RNA polymerase, functioned at lower concentrations than DksA, and complemented a dksA -null strain for growth on minimal medium. One of the homologs, λ Orf73, encoded by bacteriophage lambda, was examined in greater detail. λ Orf73 slowed host growth and increased phage burst size. Mutational analysis suggested that λ Orf73 and TraR have a similar mechanism for inhibiting rRNA and r-protein promoters. We suggest that TraR and its homologs regulate host transcription to divert cellular resources to phage propagation or conjugation without induction of ppGpp and a stringent response. IMPORTANCE TraR is a distant homolog of the transcription factor DksA and the founding member of a large family of small proteins encoded by proteobacterial phages and conjugative plasmids. Reprogramming transcription during the stringent response requires the interaction of DksA not only with RNA polymerase but also with the stress-induced regulatory nucleotide ppGpp. We show here that five phage TraR homologs by themselves, without ppGpp, regulate transcription of host promoters, mimicking the effects of DksA and ppGpp together. During a stringent response, ppGpp independently binds directly to, and inhibits the activities of, many proteins in addition to RNA polymerase, including translation factors, enzymes needed for ribonucleotide biosynthesis, and other metabolic enzymes. Here, we suggest a physiological role for TraR-like proteins: bacteriophages utilize TraR homologs to reprogram host transcription in the absence of ppGpp induction and thus without inhibiting host enzymes needed for phage development.

Published

2022

6. Rhodobacter sphaeroides CarD Negatively Regulates Its Own Promoter.

Author

Henry KK, Ross W, and Gourse RL

Subjects

Bacterial Proteins genetics, Base Sequence, Rhodobacter sphaeroides genetics, Transcription Factors genetics, Transcription, Genetic, Bacterial Proteins metabolism, Gene Expression Regulation, Bacterial, Promoter Regions, Genetic, Rhodobacter sphaeroides metabolism, Transcription Factors metabolism

Abstract

Bioinformatic analysis showed previously that a majority of promoters in the photoheterotrophic alphaproteobacterium Rhodobacter sphaeroides lack the thymine at the last position of the -10 element (-7T), a base that is very highly conserved in promoters in bacteria other than alphaproteobacteria. The absence of -7T was correlated with low promoter activity using purified R. sphaeroides RNA polymerase (RNAP), but the transcription factor CarD compensated by activating almost all promoters lacking -7T tested in vitro , including rRNA promoters. Here, we show that a previously uncharacterized R. sphaeroides promoter, the promoter for carD itself, has high basal activity relative to other tested R. sphaeroides promoters despite lacking -7T, and its activity is inhibited rather than activated by CarD. This high basal activity is dependent on a consensus-extended -10 element (TGn) and specific features in the spacer immediately upstream of the extended -10 element. CarD negatively autoregulates its own promoter by producing abortive transcripts, limiting promoter escape, and reducing full-length mRNA synthesis. This mechanism of negative regulation differs from that employed by classical repressors, in which the transcription factor competes with RNA polymerase for binding to the promoter, and with the mechanism of negative regulation used by transcription factors like DksA/ppGpp and TraR that allosterically inhibit the rate of open complex formation. IMPORTANCE R. sphaeroides CarD activates many promoters by binding directly to RNAP and DNA just upstream of the -10 element. In contrast, we show here that CarD inhibits its own promoter using the same interactions with RNAP and DNA used for activation. Inhibition results from increasing abortive transcript formation, thereby decreasing promoter escape and full-length RNA synthesis. We propose that the combined interactions of RNAP with CarD, with the extended -10 element and with features in the adjacent -10/-35 spacer DNA, stabilize the promoter complex, reducing promoter clearance. These findings support previous predictions that the effects of CarD on transcription can be either positive or negative, depending on the kinetic properties of the specific promoter.

Published

2021

7. A majority of Rhodobacter sphaeroides promoters lack a crucial RNA polymerase recognition feature, enabling coordinated transcription activation.

Author

Henry KK, Ross W, Myers KS, Lemmer KC, Vera JM, Landick R, Donohue TJ, and Gourse RL

Subjects

Bacterial Proteins genetics, Gene Expression Regulation, Bacterial genetics, Transcription Factors genetics, DNA-Directed RNA Polymerases genetics, Promoter Regions, Genetic genetics, Rhodobacter sphaeroides genetics, Transcription, Genetic genetics, Transcriptional Activation genetics

Abstract

Using an in vitro transcription system with purified RNA polymerase (RNAP) to investigate rRNA synthesis in the photoheterotrophic α-proteobacterium Rhodobacter sphaeroides , we identified a surprising feature of promoters recognized by the major holoenzyme. Transcription from R. sphaeroides rRNA promoters was unexpectedly weak, correlating with absence of -7T, the very highly conserved thymine found at the last position in -10 elements of promoters in most bacterial species. Thymine substitutions for adenine at position -7 in the three rRNA promoters strongly increased intrinsic promoter activity, indicating that R. sphaeroides RNAP can utilize -7T when present. rRNA promoters were activated by purified R. sphaeroides CarD, a transcription factor found in many bacterial species but not in β- and γ-proteobacteria. Overall, CarD increased the activity of 15 of 16 native R. sphaeroides promoters tested in vitro that lacked -7T, whereas it had no effect on three of the four native promoters that contained -7T. Genome-wide bioinformatic analysis of promoters from R. sphaeroides and two other α-proteobacterial species indicated that 30 to 43% contained -7T, whereas 90 to 99% of promoters from non-α-proteobacteria contained -7T. Thus, promoters lacking -7T appear to be widespread in α-proteobacteria and may have evolved away from consensus to enable their coordinated regulation by transcription factors like CarD. We observed a strong reduction in R. sphaeroides CarD levels when cells enter stationary phase, suggesting that reduced activation by CarD may contribute to inhibition of rRNA transcription when cells enter stationary phase, the stage of growth when bacterial ribosome synthesis declines., Competing Interests: The authors declare no competing interest., (Copyright © 2020 the Author(s). Published by PNAS.)

Published

2020

8. Guanosine Tetraphosphate Has a Similar Affinity for Each of Its Two Binding Sites on Escherichia coli RNA Polymerase.

Author

Myers AR, Thistle DP, Ross W, and Gourse RL

Abstract

During nutrient deprivation, the bacterial cell undergoes a stress response known as the stringent response. This response is characterized by induction of the nucleotide derivative guanosine tetraphosphate (ppGpp) that dramatically modulates the cell's transcriptome. In Escherichia coli , ppGpp regulates transcription of as many as 750 genes within 5 min of induction by binding directly to RNA polymerase (RNAP) at two sites ~60 Å apart. One proposal for the presence of two sites is that they have different affinities for ppGpp, expanding the dynamic range over which ppGpp acts. We show here, primarily using the Differential Radial Capillary Action of Ligand Assay (DRaCALA), that ppGpp has a similar affinity for each site, contradicting the proposal. Because the ppGpp binding sites are formed by interactions of the β' subunit of RNAP with two small protein factors, the ω subunit of RNAP which contributes to Site 1 and the transcription factor DksA which contributes to Site 2, variation in the concentrations of ω or DksA potentially could differentially regulate ppGpp occupancy of the two sites. It was shown previously that DksA varies little at different growth rates or growth phases, but little is known about variation of the ω concentration. Therefore, we raised an anti-ω antibody and performed Western blots at different times in growth and during a stringent response. We show here that ω, like DksA, changes little with growth conditions. Together, our data suggest that the two ppGpp binding sites fill in parallel, and occupancy with changing nutritional conditions is determined by variation in the ppGpp concentration, not by variation in ω or DksA., (Copyright © 2020 Myers, Thistle, Ross and Gourse.)

Published

2020

9. Reverse engineering of fatty acid-tolerant Escherichia coli identifies design strategies for robust microbial cell factories.

Author

Chen Y, Boggess EE, Ocasio ER, Warner A, Kerns L, Drapal V, Gossling C, Ross W, Gourse RL, Shao Z, Dickerson J, Mansell TJ, and Jarboe LR

Subjects

Amino Acid Substitution, Caprylates metabolism, DNA-Directed RNA Polymerases genetics, DNA-Directed RNA Polymerases metabolism, Escherichia coli genetics, Escherichia coli metabolism, Escherichia coli Proteins genetics, Escherichia coli Proteins metabolism, Glucosyltransferases genetics, Glucosyltransferases metabolism, Metabolic Engineering, Mutation, Missense

Abstract

Adaptive laboratory evolution is often used to improve the performance of microbial cell factories. Reverse engineering of evolved strains enables learning and subsequent incorporation of novel design strategies via the design-build-test-learn cycle. Here, we reverse engineer a strain of Escherichia coli previously evolved for increased tolerance of octanoic acid (C8), an attractive biorenewable chemical, resulting in increased C8 production, increased butanol tolerance, and altered membrane properties. Here, evolution was determined to have occurred first through the restoration of WaaG activity, involved in the production of lipopolysaccharides, then an amino acid change in RpoC, a subunit of RNA polymerase, and finally mutation of the BasS-BasR two component system. All three mutations were required in order to reproduce the increased growth rate in the presence of 20 mM C8 and increased cell surface hydrophobicity; the WaaG and RpoC mutations both contributed to increased C8 titers, with the RpoC mutation appearing to be the major driver of this effect. Each of these mutations contributed to changes in the cell membrane. Increased membrane integrity and rigidity and decreased abundance of extracellular polymeric substances can be attributed to the restoration of WaaG. The increase in average lipid tail length can be attributed to the RpoC H419P mutation, which also confers tolerance to other industrially-relevant inhibitors, such as furfural, vanillin and n-butanol. The RpoC H419P mutation may impact binding or function of the stringent response alarmone ppGpp to RpoC site 1. Each of these mutations provides novel strategies for engineering microbial robustness, particularly at the level of the microbial cell membrane., (Copyright © 2020 International Metabolic Engineering Society. Published by Elsevier Inc. All rights reserved.)

Published

2020

10. Stepwise Promoter Melting by Bacterial RNA Polymerase.

Author

Chen J, Chiu C, Gopalkrishnan S, Chen AY, Olinares PDB, Saecker RM, Winkelman JT, Maloney MF, Chait BT, Ross W, Gourse RL, Campbell EA, and Darst SA

Subjects

Cryoelectron Microscopy, DNA-Directed RNA Polymerases chemistry, Escherichia coli genetics, Nucleic Acid Conformation, Protein Binding genetics, Protein Conformation, DNA-Directed RNA Polymerases genetics, Promoter Regions, Genetic genetics, RNA, Bacterial genetics, Transcription Initiation, Genetic

Abstract

Transcription initiation requires formation of the open promoter complex (RPo). To generate RPo, RNA polymerase (RNAP) unwinds the DNA duplex to form the transcription bubble and loads the DNA into the RNAP active site. RPo formation is a multi-step process with transient intermediates of unknown structure. We use single-particle cryoelectron microscopy to visualize seven intermediates containing Escherichia coli RNAP with the transcription factor TraR en route to forming RPo. The structures span the RPo formation pathway from initial recognition of the duplex promoter in a closed complex to the final RPo. The structures and supporting biochemical data define RNAP and promoter DNA conformational changes that delineate steps on the pathway, including previously undetected transient promoter-RNAP interactions that contribute to populating the intermediates but do not occur in RPo. Our work provides a structural basis for understanding RPo formation and its regulation, a major checkpoint in gene expression throughout evolution., Competing Interests: Declaration of Interests The authors declare no competing interests., (Copyright © 2020 Elsevier Inc. All rights reserved.)

Published

2020

11. Deciphering the RNA capping process in bacteria.

Author

Jagodnik J and Gourse RL

Subjects

Gene Expression, Bacteria, RNA Caps

Abstract

Competing Interests: The authors declare no competing interest.

Published

2020

12. E. coli TraR allosterically regulates transcription initiation by altering RNA polymerase conformation.

Author

Chen J, Gopalkrishnan S, Chiu C, Chen AY, Campbell EA, Gourse RL, Ross W, and Darst SA

Subjects

Base Sequence, Carrier Proteins, Cryoelectron Microscopy, DNA, Bacterial metabolism, Escherichia coli Proteins chemistry, Escherichia coli Proteins genetics, Models, Molecular, Mutagenesis, Site-Directed, Promoter Regions, Genetic, Protein Conformation, RNA, Bacterial metabolism, Transcription Factors chemistry, Transcriptional Activation, DNA-Directed RNA Polymerases metabolism, Escherichia coli metabolism, Escherichia coli Proteins metabolism, Nucleic Acid Conformation, Transcription Factors metabolism, Transcription Initiation, Genetic physiology

Abstract

TraR and its homolog DksA are bacterial proteins that regulate transcription initiation by binding directly to RNA polymerase (RNAP) rather than to promoter DNA. Effects of TraR mimic the combined effects of DksA and its cofactor ppGpp, but the structural basis for regulation by these factors remains unclear. Here, we use cryo-electron microscopy to determine structures of Escherichia coli RNAP, with or without TraR, and of an RNAP-promoter complex. TraR binding induced RNAP conformational changes not seen in previous crystallographic analyses, and a quantitative analysis revealed TraR-induced changes in RNAP conformational heterogeneity. These changes involve mobile regions of RNAP affecting promoter DNA interactions, including the βlobe, the clamp, the bridge helix, and several lineage-specific insertions. Using mutational approaches, we show that these structural changes, as well as effects on σ 70 region 1.1, are critical for transcription activation or inhibition, depending on the kinetic features of regulated promoters., Competing Interests: JC, SG, CC, AC, EC, RG, WR, SD No competing interests declared, (© 2019, Chen et al.)

Published

2019

13. Structural basis for transcription activation by Crl through tethering of σ S and RNA polymerase.

Author

Cartagena AJ, Banta AB, Sathyan N, Ross W, Gourse RL, Campbell EA, and Darst SA

Subjects

Bacterial Proteins genetics, Cryoelectron Microscopy, DNA-Directed RNA Polymerases genetics, DNA-Directed RNA Polymerases metabolism, Gene Expression Regulation, Bacterial, Models, Molecular, Mutation, Promoter Regions, Genetic, Protein Binding, Protein Conformation, Sigma Factor genetics, Sigma Factor metabolism, Transcription Factors genetics, Bacterial Proteins chemistry, Bacterial Proteins metabolism, DNA-Directed RNA Polymerases chemistry, Sigma Factor chemistry, Transcription Factors metabolism, Transcriptional Activation

Abstract

In bacteria, a primary σ-factor associates with the core RNA polymerase (RNAP) to control most transcription initiation, while alternative σ-factors are used to coordinate expression of additional regulons in response to environmental conditions. Many alternative σ-factors are negatively regulated by anti-σ-factors. In Escherichia coli , Salmonella enterica , and many other γ-proteobacteria, the transcription factor Crl positively regulates the alternative σ S -regulon by promoting the association of σ S with RNAP without interacting with promoter DNA. The molecular mechanism for Crl activity is unknown. Here, we determined a single-particle cryo-electron microscopy structure of Crl-σ S -RNAP in an open promoter complex with a σ S -regulon promoter. In addition to previously predicted interactions between Crl and domain 2 of σ S (σ S 2 ), the structure, along with p -benzoylphenylalanine cross-linking, reveals that Crl interacts with a structural element of the RNAP β'-subunit that we call the β'-clamp-toe (β'CT). Deletion of the β'CT decreases activation by Crl without affecting basal transcription, highlighting the functional importance of the Crl-β'CT interaction. We conclude that Crl activates σ S -dependent transcription in part through stabilizing σ S -RNAP by tethering σ S 2 and the β'CT. We propose that Crl, and other transcription activators that may use similar mechanisms, be designated σ-activators., Competing Interests: The authors declare no conflict of interest.

Published

2019

14. Genome-wide effects on Escherichia coli transcription from ppGpp binding to its two sites on RNA polymerase.

Author

Sanchez-Vazquez P, Dewey CN, Kitten N, Ross W, and Gourse RL

Subjects

Escherichia coli Proteins chemistry, Escherichia coli Proteins genetics, Escherichia coli Proteins metabolism, Gene Expression Regulation, Bacterial genetics, Genome, Bacterial genetics, Promoter Regions, Genetic genetics, Transcriptome, Binding Sites genetics, DNA-Directed RNA Polymerases chemistry, DNA-Directed RNA Polymerases genetics, DNA-Directed RNA Polymerases metabolism, Escherichia coli genetics, Guanosine Tetraphosphate chemistry, Guanosine Tetraphosphate genetics, Guanosine Tetraphosphate metabolism, Transcription, Genetic genetics

Abstract

The second messenger nucleotide ppGpp dramatically alters gene expression in bacteria to adjust cellular metabolism to nutrient availability. ppGpp binds to two sites on RNA polymerase (RNAP) in Escherichia coli , but it has also been reported to bind to many other proteins. To determine the role of the RNAP binding sites in the genome-wide effects of ppGpp on transcription, we used RNA-seq to analyze transcripts produced in response to elevated ppGpp levels in strains with/without the ppGpp binding sites on RNAP. We examined RNAs rapidly after ppGpp production without an accompanying nutrient starvation. This procedure enriched for direct effects of ppGpp on RNAP rather than for indirect effects on transcription resulting from starvation-induced changes in metabolism or on secondary events from the initial effects on RNAP. The transcriptional responses of all 757 genes identified after 5 minutes of ppGpp induction depended on ppGpp binding to RNAP. Most (>75%) were not reported in earlier studies. The regulated transcripts encode products involved not only in translation but also in many other cellular processes. In vitro transcription analysis of more than 100 promoters from the in vivo dataset identified a large collection of directly regulated promoters, unambiguously demonstrated that most effects of ppGpp on transcription in vivo were direct, and allowed comparison of DNA sequences from inhibited, activated, and unaffected promoter classes. Our analysis greatly expands our understanding of the breadth of the stringent response and suggests promoter sequence features that contribute to the specific effects of ppGpp., Competing Interests: The authors declare no conflict of interest.

Published

2019

15. Transcriptional Responses to ppGpp and DksA.

Author

Gourse RL, Chen AY, Gopalkrishnan S, Sanchez-Vazquez P, Myers A, and Ross W

Subjects

DNA-Directed RNA Polymerases metabolism, Guanosine Pentaphosphate metabolism, Gene Expression Regulation, Bacterial, Guanosine Tetraphosphate metabolism, Proteobacteria genetics, Proteobacteria metabolism, Stress, Physiological, Transcription Factors metabolism

Abstract

The stringent response to nutrient deprivation is a stress response found throughout the bacterial domain of life. Although first described in proteobacteria for matching ribosome synthesis to the cell's translation status and for preventing formation of defective ribosomal particles, the response is actually much broader, regulating many hundreds of genes-some positively, some negatively. Utilization of the signaling molecules ppGpp and pppGpp for this purpose is ubiquitous in bacterial evolution, although the mechanisms employed vary. In proteobacteria, the signaling molecules typically bind to two sites on RNA polymerase, one at the interface of the β' and ω subunits and one at the interface of the β' secondary channel and the transcription factor DksA. The β' secondary channel is targeted by other transcription regulators as well. Although studies on the transcriptional outputs of the stringent response date back at least 50 years, the mechanisms responsible are only now coming into focus.

Published

2018

16. Linking glucose metabolism to the stringent response through the PTS.

Author

Gourse RL and Bouveret E

Subjects

Glucose, Carbohydrate Metabolism, Phosphoenolpyruvate Sugar Phosphotransferase System

Abstract

Competing Interests: The authors declare no conflict of interest.

Published

2018

17. DksA and ppGpp Regulate the σ S Stress Response by Activating Promoters for the Small RNA DsrA and the Anti-Adapter Protein IraP.

Author

Girard ME, Gopalkrishnan S, Grace ED, Halliday JA, Gourse RL, and Herman C

Subjects

Escherichia coli genetics, Escherichia coli Proteins genetics, Gene Expression Regulation, Bacterial, Promoter Regions, Genetic, Pyrophosphatases genetics, RNA, Small Untranslated genetics, Sigma Factor genetics, Stress, Physiological, Escherichia coli metabolism, Escherichia coli Proteins metabolism, Pyrophosphatases metabolism, RNA, Small Untranslated metabolism, Sigma Factor metabolism

Abstract

σ S is an alternative sigma factor, encoded by the rpoS gene, that redirects cellular transcription to a large family of genes in response to stressful environmental signals. This so-called σ S general stress response is necessary for survival in many bacterial species and is controlled by a complex, multifactorial pathway that regulates σ S levels transcriptionally, translationally, and posttranslationally in Escherichia coli It was shown previously that the transcription factor DksA and its cofactor, ppGpp, are among the many factors governing σ S synthesis, thus playing an important role in activation of the σ S stress response. However, the mechanisms responsible for the effects of DksA and ppGpp have not been elucidated fully. We describe here how DksA and ppGpp directly activate the promoters for the anti-adaptor protein IraP and the small regulatory RNA DsrA, thereby indirectly influencing σ S levels. In addition, based on effects of DksA N88I , a previously identified DksA variant with increased affinity for RNA polymerase (RNAP), we show that DksA can increase σ S activity by another indirect mechanism. We propose that by reducing rRNA transcription, DksA and ppGpp increase the availability of core RNAP for binding to σ S and also increase transcription from other promoters, including P dsrA and P iraP By improving the translation and stabilization of σ S , as well as the ability of other promoters to compete for RNAP, DksA and ppGpp contribute to the switch in the transcription program needed for stress adaptation. IMPORTANCE Bacteria spend relatively little time in log phase outside the optimized environment found in a laboratory. They have evolved to make the most of alternating feast and famine conditions by seamlessly transitioning between rapid growth and stationary phase, a lower metabolic mode that is crucial for long-term survival. One of the key regulators of the switch in gene expression that characterizes stationary phase is the alternative sigma factor σ S Understanding the factors governing σ S activity is central to unraveling the complexities of growth, adaptation to stress, and pathogenesis. Here, we describe three mechanisms by which the RNA polymerase binding factor DksA and the second messenger ppGpp regulate σ S levels., (Copyright © 2017 American Society for Microbiology.)

Published

2017

18. Roles of Transcriptional and Translational Control Mechanisms in Regulation of Ribosomal Protein Synthesis in Escherichia coli.

Author

Burgos HL, O'Connor K, Sanchez-Vazquez P, and Gourse RL

Subjects

5' Untranslated Regions, Feedback, Physiological, Guanosine Tetraphosphate metabolism, RNA, Ribosomal biosynthesis, Escherichia coli genetics, Escherichia coli metabolism, Gene Expression Regulation, Protein Biosynthesis, Ribosomal Proteins biosynthesis, Transcription, Genetic

Abstract

Bacterial ribosome biogenesis is tightly regulated to match nutritional conditions and to prevent formation of defective ribosomal particles. In Escherichia coli , most ribosomal protein (r-protein) synthesis is coordinated with rRNA synthesis by a translational feedback mechanism: when r-proteins exceed rRNAs, specific r-proteins bind to their own mRNAs and inhibit expression of the operon. It was recently discovered that the second messenger nucleotide guanosine tetra and pentaphosphate (ppGpp), which directly regulates rRNA promoters, is also capable of regulating many r-protein promoters. To examine the relative contributions of the translational and transcriptional control mechanisms to the regulation of r-protein synthesis, we devised a reporter system that enabled us to genetically separate the cis -acting sequences responsible for the two mechanisms and to quantify their relative contributions to regulation under the same conditions. We show that the synthesis of r-proteins from the S20 and S10 operons is regulated by ppGpp following shifts in nutritional conditions, but most of the effect of ppGpp required the 5' region of the r-protein mRNA containing the target site for translational feedback regulation and not the promoter. These results suggest that most regulation of the S20 and S10 operons by ppGpp following nutritional shifts is indirect and occurs in response to changes in rRNA synthesis. In contrast, we found that the promoters for the S20 operon were regulated during outgrowth, likely in response to increasing nucleoside triphosphate (NTP) levels. Thus, r-protein synthesis is dynamic, with different mechanisms acting at different times. IMPORTANCE Bacterial cells have evolved complex and seemingly redundant strategies to regulate many high-energy-consuming processes. In E. coli , synthesis of ribosomal components is tightly regulated with respect to nutritional conditions by mechanisms that act at both the transcription and translation steps. In this work, we conclude that NTP and ppGpp concentrations can regulate synthesis of ribosomal proteins, but most of the effect of ppGpp is indirect as a consequence of translational feedback in response to changes in rRNA levels. Our results illustrate how effects of seemingly redundant regulatory mechanisms can be separated in time and that even when multiple mechanisms act concurrently their contributions are not necessarily equivalent., (Copyright © 2017 American Society for Microbiology.)

Published

2017

19. Dissection of the molecular circuitry controlling virulence in Francisella tularensis .

Author

Cuthbert BJ, Ross W, Rohlfing AE, Dove SL, Gourse RL, Brennan RG, and Schumacher MA

Subjects

Adhesins, Bacterial chemistry, Adhesins, Bacterial genetics, Bioterrorism prevention & control, Cells, Cultured, Crystallography, DNA-Binding Proteins chemistry, DNA-Binding Proteins genetics, DNA-Directed RNA Polymerases metabolism, Gene Expression Regulation, Bacterial, Guanosine Tetraphosphate genetics, Humans, Macrophages metabolism, Protein Conformation, Transcription, Genetic, Virulence genetics, Adhesins, Bacterial metabolism, DNA-Binding Proteins metabolism, Francisella tularensis pathogenicity, Genomic Islands genetics, Guanosine Tetraphosphate metabolism, Tularemia microbiology

Abstract

Francisella tularensis, the etiological agent of tularemia, is one of the most infectious bacteria known. Because of its extreme pathogenicity, F. tularensis is classified as a category A bioweapon by the US government. F. tularensis virulence stems from genes encoded on the Francisella pathogenicity island (FPI). An unusual set of Francisella regulators-the heteromeric macrophage growth locus protein A (MglA)-stringent starvation protein A (SspA) complex and the DNA-binding protein pathogenicity island gene regulator (PigR)-activates FPI transcription and thus is essential for virulence. Intriguingly, the second messenger, guanosine-tetraphosphate (ppGpp), which is produced during infection, is also involved in coordinating Francisella virulence; however, its role has been unclear. Here we identify MglA-SspA as a novel ppGpp-binding complex and describe structures of apo- and ppGpp-bound MglA-SspA. We demonstrate that MglA-SspA, which binds RNA polymerase (RNAP), also interacts with the C-terminal domain of PigR, thus anchoring the (MglA-SspA)-RNAP complex to the FPI promoter. Furthermore, we show that MglA-SspA must be bound to ppGpp to mediate high-affinity interactions with PigR. Thus, these studies unveil a novel pathway different from those described previously for regulation of transcription by ppGpp. The data also indicate that F. tularensis pathogenesis is controlled by a highly interconnected molecular circuitry in which the virulence machinery directly senses infection via a small molecule stress signal., (© 2017 Cuthbert et al.; Published by Cold Spring Harbor Laboratory Press.)

Published

2017

20. TraR directly regulates transcription initiation by mimicking the combined effects of the global regulators DksA and ppGpp.

Author

Gopalkrishnan S, Ross W, Chen AY, and Gourse RL

Subjects

Allosteric Site, Catalytic Domain, DNA-Directed RNA Polymerases metabolism, Escherichia coli metabolism, Escherichia coli Proteins metabolism, Evolution, Molecular, Promoter Regions, Genetic, Protein Domains, Ribosomes metabolism, Transcription Factors metabolism, Transcription, Genetic, Escherichia coli Proteins genetics, Gene Expression Regulation, Bacterial, Guanosine Tetraphosphate metabolism, Transcription Factors genetics

Abstract

The Escherichia coli F element-encoded protein TraR is a distant homolog of the chromosome-encoded transcription factor DksA. Here we address the mechanism by which TraR acts as a global regulator, inhibiting some promoters and activating others. We show that TraR regulates transcription directly in vitro by binding to the secondary channel of RNA polymerase (RNAP) using interactions similar, but not identical, to those of DksA. Even though it binds to RNAP with only slightly higher affinity than DksA and is only half the size of DksA, TraR by itself inhibits transcription as strongly as DksA and ppGpp combined and much more than DksA alone. Furthermore, unlike DksA, TraR activates transcription even in the absence of ppGpp. TraR lacks the residues that interact with ppGpp in DksA, and TraR binding to RNAP uses the residues in the β' rim helices that contribute to the ppGpp binding site in the DksA-ppGpp-RNAP complex. Thus, unlike DksA, TraR does not bind ppGpp. We propose a model in which TraR mimics the effects of DksA and ppGpp together by binding directly to the region of the RNAP secondary channel that otherwise binds ppGpp, and its N-terminal region, like the coiled-coil tip of DksA, engages the active-site region of the enzyme and affects transcription allosterically. These data provide insights into the function not only of TraR but also of an evolutionarily widespread and diverse family of TraR-like proteins encoded by bacteria, as well as bacteriophages and other extrachromosomal elements., Competing Interests: The authors declare no conflict of interest.

Published

2017

21. Classic Spotlights: Selected Highlights from the First 100 Years of the Journal of Bacteriology .

Author

Armitage JP, Becker A, Christie PJ, de Boer PAJ, DiRita VJ, Gourse RL, Henkin TM, Margolin W, Metcalf WW, Mullineaux CW, O'Toole GA, Parkinson JS, Schneewind O, Silhavy TJ, Stock AM, and Zhulin IB

Subjects

History, 20th Century, History, 21st Century, Bacteriology, Periodicals as Topic history

Published

2017

22. Open complex DNA scrunching: A key to transcription start site selection and promoter escape.

Author

Winkelman JT and Gourse RL

Subjects

Escherichia coli metabolism, Escherichia coli Proteins metabolism, DNA-Directed RNA Polymerases metabolism, Escherichia coli genetics, Promoter Regions, Genetic, Transcription Initiation Site

Abstract

Bacterial RNA polymerase-promoter open complexes can exist in a range of states in which the leading edge of the enzyme moves but the trailing edge does not, a phenomenon we refer to as "open complex scrunching." Here we describe how open complex scrunching can determine the position of the transcription start site for some promoters, modulate the level of expression, and potentially could be targeted by factors to regulate transcription. We suggest that open complex scrunching at the extraordinarily active ribosomal RNA promoters might have evolved to initiate transcription at an unusual position relative to the core promoter elements in order to maximize the rate of promoter escape., (© 2017 WILEY Periodicals, Inc.)

Published

2017

23. Colocalization of distant chromosomal loci in space in E. coli: a bacterial nucleolus.

Author

Gaal T, Bratton BP, Sanchez-Vazquez P, Sliwicki A, Sliwicki K, Vegel A, Pannu R, and Gourse RL

Subjects

Chromosomes, Bacterial chemistry, Operon genetics, Promoter Regions, Genetic genetics, RNA, Bacterial genetics, RNA, Bacterial metabolism, Rec A Recombinases metabolism, Chromosomes, Bacterial genetics, Escherichia coli genetics, Nucleolus Organizer Region

Abstract

The spatial organization of DNA within the bacterial nucleoid remains unclear. To investigate chromosome organization in Escherichia coli, we examined the relative positions of the ribosomal RNA (rRNA) operons in space. The seven rRNA operons are nearly identical and separated from each other by as much as 180° on the circular genetic map, a distance of ≥2 million base pairs. By inserting binding sites for fluorescent proteins adjacent to the rRNA operons and then examining their positions pairwise in live cells by epifluorescence microscopy, we found that all but rrnC are in close proximity. Colocalization of the rRNA operons required the rrn P1 promoter region but not the rrn P2 promoter or the rRNA structural genes and occurred with and without active transcription. Non-rRNA operon pairs did not colocalize, and the magnitude of their physical separation generally correlated with that of their genetic separation. Our results show that E. coli bacterial chromosome folding in three dimensions is not dictated entirely by genetic position but rather includes functionally related, genetically distant loci that come into close proximity, with rRNA operons forming a structure reminiscent of the eukaryotic nucleolus., (© 2016 Gaal et al.; Published by Cold Spring Harbor Laboratory Press.)

Published

2016

24. Classic Spotlight: the Heat Shock Response and the Discovery of Alternative Sigma Factors in Escherichia coli.

Author

Gourse RL

Subjects

Bacillus subtilis genetics, Bacillus subtilis physiology, Bacteriology history, History, 20th Century, Escherichia coli genetics, Escherichia coli physiology, Gene Expression Regulation, Bacterial, Heat-Shock Response, Sigma Factor genetics, Sigma Factor metabolism

Published

2016

25. ppGpp Binding to a Site at the RNAP-DksA Interface Accounts for Its Dramatic Effects on Transcription Initiation during the Stringent Response.

Author

Ross W, Sanchez-Vazquez P, Chen AY, Lee JH, Burgos HL, and Gourse RL

Subjects

Amino Acid Sequence, Binding Sites, Conserved Sequence, DNA-Directed RNA Polymerases chemistry, DNA-Directed RNA Polymerases genetics, Escherichia coli genetics, Escherichia coli Proteins chemistry, Escherichia coli Proteins genetics, Evolution, Molecular, Gene Expression Regulation, Bacterial, Models, Molecular, Protein Binding, Protein Conformation, Structure-Activity Relationship, DNA-Directed RNA Polymerases metabolism, Escherichia coli metabolism, Escherichia coli Proteins metabolism, Guanosine Tetraphosphate metabolism, Stress, Physiological, Transcription Initiation, Genetic

Abstract

Throughout the bacterial domain, the alarmone ppGpp dramatically reprograms transcription following nutrient limitation. This "stringent response" is critical for survival and antibiotic tolerance and is a model for transcriptional regulation by small ligands. We report that ppGpp binds to two distinct sites 60 Å apart on E. coli RNA polymerase (RNAP), one characterized previously (site 1) and a second identified here at an interface of RNAP and the transcription factor DksA (site 2). The location and unusual tripartite nature of site 2 account for the DksA-ppGpp synergism and suggest mechanisms for ppGpp enhancement of DksA's effects on RNAP. Site 2 binding results in the majority of ppGpp's effects on transcription initiation in vitro and in vivo, and strains lacking site 2 are severely impaired for growth following nutritional shifts. Filling of the two sites at different ppGpp concentrations would expand the dynamic range of cellular responses to changes in ppGpp levels., (Copyright © 2016 Elsevier Inc. All rights reserved.)

Published

2016

26. Coexpression of Escherichia coli obgE, Encoding the Evolutionarily Conserved Obg GTPase, with Ribosomal Proteins L21 and L27.

Author

Maouche R, Burgos HL, My L, Viala JP, Gourse RL, and Bouveret E

Subjects

Base Sequence, Escherichia coli enzymology, Escherichia coli metabolism, Escherichia coli Proteins genetics, Molecular Sequence Data, Monomeric GTP-Binding Proteins genetics, Operon, Phylogeny, Ribosomal Proteins genetics, Transcription, Genetic, Escherichia coli genetics, Escherichia coli Proteins metabolism, Evolution, Molecular, Gene Expression Regulation, Bacterial, Monomeric GTP-Binding Proteins metabolism, Ribosomal Proteins metabolism

Abstract

Unlabelled: Multiple essential small GTPases are involved in the assembly of the ribosome or in the control of its activity. Among them, ObgE (CgtA) has been shown recently to act as a ribosome antiassociation factor that binds to ppGpp, a regulator whose best-known target is RNA polymerase. The present study was aimed at elucidating the expression of obgE in Escherichia coli We show that obgE is cotranscribed with ribosomal protein genes rplU and rpmA and with a gene of unknown function, yhbE We show here that about 75% of the transcripts terminate before obgE, because there is a transcriptional terminator between rpmA and yhbE As expected for ribosomal protein operons, expression was highest during exponential growth, decreased during entry into stationary phase, and became almost undetectable thereafter. Expression of the operon was derepressed in mutants lacking ppGpp or DksA. However, regulation by these factors appears to occur post-transcription initiation, since no effects of ppGpp and DksA on rplU promoter activity were observed in vitro, Importance: The conserved and essential ObgE GTPase binds to the ribosome and affects its assembly. ObgE has also been reported to impact chromosome segregation, cell division, resistance to DNA damage, and, perhaps most interestingly, persister formation and antibiotic tolerance. However, it is unclear whether these effects are related to its role in ribosome formation. Despite its importance, no studies on ObgE expression have been reported. We demonstrate here that obgE is expressed from an operon encoding two ribosomal proteins, that the operon's expression varies with the growth phase, and that it is dependent on the transcription regulators ppGpp and DksA. Our results thus demonstrate that obgE expression is coupled to ribosomal gene expression., (Copyright © 2016, American Society for Microbiology. All Rights Reserved.)

Published

2016

27. Classic Spotlight: Studies of the Stringent Response.

Author

Gourse RL and Crosson S

Subjects

Amino Acids metabolism, Bacteria metabolism, Bacterial Proteins, Transcription Factor RelA metabolism, Bacteria genetics, Bacterial Physiological Phenomena, RNA, Bacterial biosynthesis, Transcription Factor RelA genetics

Published

2016

28. Classic Spotlight: Visualization of Bacterial Genes in Action.

Author

Gourse RL and Condon C

Subjects

RNA, Ribosomal genetics, Escherichia coli genetics, RNA, Ribosomal biosynthesis, Ribonuclease III metabolism, Transcription, Genetic genetics

Published

2016

29. Open complex scrunching before nucleotide addition accounts for the unusual transcription start site of E. coli ribosomal RNA promoters.

Author

Winkelman JT, Chandrangsu P, Ross W, and Gourse RL

Subjects

DNA-Directed RNA Polymerases genetics, DNA-Directed RNA Polymerases metabolism, Evolution, Molecular, Gene Expression Regulation, Bacterial, Mutation, Nucleic Acid Conformation, Nucleotides genetics, Nucleotides metabolism, Transcription, Genetic, rRNA Operon genetics, Escherichia coli genetics, Promoter Regions, Genetic genetics, Transcription Initiation Site

Abstract

Most Escherichia coli promoters initiate transcription with a purine 7 or 8 nt downstream from the -10 hexamer, but some promoters, including the ribosomal RNA promoter rrnB P1, start 9 nt from the -10 element. We identified promoter and RNA polymerase determinants of this noncanonical rrnB P1 start site using biochemical and genetic approaches including mutational analysis of the promoter, Fe(2+) cleavage assays to monitor template strand positions near the active-site, and Bpa cross-linking to map the path of open complex DNA at amino acid and nucleotide resolution. We find that mutations in several promoter regions affect transcription start site (TSS) selection. In particular, we show that the absence of strong interactions between the discriminator region and σ region 1.2 and between the extended -10 element and σ region 3.0, identified previously as a determinant of proper regulation of rRNA promoters, is also required for the unusual TSS. We find that the DNA in the single-stranded transcription bubble of the rrnB P1 promoter complex expands and is "scrunched" into the active site channel of RNA polymerase, similar to the situation in initial transcribing complexes. However, in the rrnB P1 open complex, scrunching occurs before RNA synthesis begins. We find that the scrunched open complex exhibits reduced abortive product synthesis, suggesting that scrunching and unusual TSS selection contribute to the extraordinary transcriptional activity of rRNA promoters by increasing promoter escape, helping to offset the reduction in promoter activity that would result from the weak interactions with σ.

Published

2016

30. Multiplexed protein-DNA cross-linking: Scrunching in transcription start site selection.

Author

Winkelman JT, Vvedenskaya IO, Zhang Y, Zhang Y, Bird JG, Taylor DM, Gourse RL, Ebright RH, and Nickels BE

Subjects

Crystallography, X-Ray, DNA chemistry, DNA genetics, Gene Library, Nucleic Acid Conformation, Bacteria genetics, Promoter Regions, Genetic, RNA, Messenger biosynthesis, Transcription Initiation Site, Transcription Initiation, Genetic

Abstract

In bacterial transcription initiation, RNA polymerase (RNAP) selects a transcription start site (TSS) at variable distances downstream of core promoter elements. Using next-generation sequencing and unnatural amino acid-mediated protein-DNA cross-linking, we have determined, for a library of 4(10) promoter sequences, the TSS, the RNAP leading-edge position, and the RNAP trailing-edge position. We find that a promoter element upstream of the TSS, the "discriminator," participates in TSS selection, and that, as the TSS changes, the RNAP leading-edge position changes, but the RNAP trailing-edge position does not change. Changes in the RNAP leading-edge position, but not the RNAP trailing-edge position, are a defining hallmark of the "DNA scrunching" that occurs concurrent with RNA synthesis in initial transcription. We propose that TSS selection involves DNA scrunching prior to RNA synthesis., (Copyright © 2016, American Association for the Advancement of Science.)

Published

2016

31. In vitro evidence that RNA Polymerase acetylation and acetyl phosphate-dependent CpxR phosphorylation affect cpxP transcription regulation.

Author

Lima BP, Lennon CW, Ross W, Gourse RL, and Wolfe AJ

Subjects

Acetylation, Escherichia coli enzymology, Escherichia coli genetics, Escherichia coli Proteins genetics, Membrane Proteins genetics, Phosphorylation, Promoter Regions, Genetic genetics, Protein Processing, Post-Translational, Regulon, Bacterial Proteins metabolism, DNA-Directed RNA Polymerases metabolism, Escherichia coli metabolism, Escherichia coli Proteins biosynthesis, Gene Expression Regulation, Bacterial genetics, Membrane Proteins biosynthesis, Organophosphates chemistry

Abstract

The central metabolite acetyl phosphate (acP) has long been proposed to influence transcription regulation by directly transferring its phosphoryl group to a number of response regulators in many bacterial species. Here, we provide in vitro evidence for this proposition and demonstrate, using an in vitro transcription system, that acP-dependent phosphorylation of aspartate 51 of CpxR induces transcription of one of its regulon members in E. coli, cpxP. We also used this in vitro transcription system to extend our previously reported in vivo data that hypothesized that acetylation of RNA polymerase (RNAP) influences acP-dependent cpxP transcription, using glutamine as a genetic mimic for acetylated arginine 291 of the carboxy-terminal domain of RNAP α subunit. The data we present here lend strong support to the hypothesis that acP has a direct effect on transcription regulation in E. coli via phosphorylation of CpxR, and that RNAP acetylation can modulate this response., (© FEMS 2016. All rights reserved. For permissions, please e-mail: journals.permissions@oup.com.)

Published

2016

32. Crosslink Mapping at Amino Acid-Base Resolution Reveals the Path of Scrunched DNA in Initial Transcribing Complexes.

Author

Winkelman JT, Winkelman BT, Boyce J, Maloney MF, Chen AY, Ross W, and Gourse RL

Subjects

Amino Acids chemistry, Base Sequence, Cross-Linking Reagents, Crystallography, X-Ray, DNA, Bacterial genetics, DNA-Directed RNA Polymerases chemistry, DNA-Directed RNA Polymerases genetics, DNA-Directed RNA Polymerases metabolism, Escherichia coli genetics, Escherichia coli metabolism, Escherichia coli Proteins chemistry, Escherichia coli Proteins genetics, Escherichia coli Proteins metabolism, Models, Molecular, Nucleic Acid Conformation, Promoter Regions, Genetic, Protein Conformation, Transcription, Genetic, rRNA Operon, DNA, Bacterial chemistry, DNA, Bacterial metabolism

Abstract

RNA polymerase binds tightly to DNA to recognize promoters with high specificity but then releases these contacts during the initial stage of transcription. We report a site-specific crosslinking approach to map the DNA path in bacterial transcription intermediates at amino acid and nucleotide resolution. After validating the approach by showing that the DNA path in open complexes (RPO) is the same as in high-resolution X-ray structures, we define the path following substrate addition in "scrunched" complexes (RPITC). The DNA bulges that form within the transcription bubble in RPITC are positioned differently on the two strands. Our data suggest that the non-template strand bulge is extruded into solvent in complexes containing a 5-mer RNA, whereas the template strand bulge remains within the template strand tunnel, exerting stress on interactions between the β flap, β' clamp, and σ3.2. We propose that this stress contributes to σ3.2 displacement from the RNA exit channel, facilitating promoter escape., (Copyright © 2015 Elsevier Inc. All rights reserved.)

Published

2015

33. TRANSCRIPTION. Structures of the RNA polymerase-σ54 reveal new and conserved regulatory strategies.

Author

Yang Y, Darbari VC, Zhang N, Lu D, Glyde R, Wang YP, Winkelman JT, Gourse RL, Murakami KS, Buck M, and Zhang X

Subjects

Crystallography, X-Ray, Enzyme Stability, Holoenzymes chemistry, Protein Conformation, Protein Structure, Tertiary, RNA Polymerase Sigma 54 genetics, Evolution, Molecular, Gene Expression Regulation, RNA Polymerase Sigma 54 chemistry, Transcription, Genetic

Abstract

Transcription by RNA polymerase (RNAP) in bacteria requires specific promoter recognition by σ factors. The major variant σ factor (σ(54)) initially forms a transcriptionally silent complex requiring specialized adenosine triphosphate-dependent activators for initiation. Our crystal structure of the 450-kilodalton RNAP-σ(54) holoenzyme at 3.8 angstroms reveals molecular details of σ(54) and its interactions with RNAP. The structure explains how σ(54) targets different regions in RNAP to exert its inhibitory function. Although σ(54) and the major σ factor, σ(70), have similar functional domains and contact similar regions of RNAP, unanticipated differences are observed in their domain arrangement and interactions with RNAP, explaining their distinct properties. Furthermore, we observe evolutionarily conserved regulatory hotspots in RNAPs that can be targeted by a diverse range of mechanisms to fine tune transcription., (Copyright © 2015, American Association for the Advancement of Science.)

Published

2015

34. Strategies from UW-Madison for rescuing biomedical research in the US.

Author

Kimble J, Bement WM, Chang Q, Cox BL, Drinkwater NR, Gourse RL, Hoskins AA, Huttenlocher A, Kreeger PK, Lambert PF, Mailick MR, Miyamoto S, Moss RL, O'Connor-Giles KM, Roopra A, Saha K, and Seidel HS

Subjects

Capital Financing, United States, Universities, Biomedical Research economics, Biomedical Research trends, Peer Review, Research methods, Peer Review, Research trends

Abstract

A cross-campus, cross-career stage and cross-disciplinary series of discussions at a large public university has produced a series of recommendations for addressing the problems confronting the biomedical research community in the US.

Published

2015

35. Activation of the σE-dependent stress pathway by conjugative TraR may anticipate conjugational stress.

Author

Grace ED, Gopalkrishnan S, Girard ME, Blankschien MD, Ross W, Gourse RL, and Herman C

Subjects

Escherichia coli genetics, Escherichia coli Proteins genetics, Gene Expression Regulation, Bacterial, Operon, Promoter Regions, Genetic, Sigma Factor metabolism, Stress, Physiological, Transcription Factors genetics, Transcriptional Activation, Conjugation, Genetic, Escherichia coli physiology, Escherichia coli Proteins metabolism, Sigma Factor genetics, Transcription Factors metabolism, Up-Regulation

Abstract

Horizontal gene transfer by conjugation plays a major role in bacterial evolution, allowing the acquisition of new traits, such as virulence and resistance to antibacterial agents. With the increased antibiotic resistance in bacterial pathogens, a better understanding of how bacteria modulate conjugation under changing environments and the genetic factors involved is needed. Despite the evolutionary advantages conjugation may confer, the process can be quite stressful for the donor cell. Here, we characterize the ability of TraR, encoded on the episomal F' plasmid, to upregulate the σ(E) extracytoplasmic stress pathway in Escherichia coli. TraR, a DksA homolog, modulates transcription initiation through the secondary channel of RNA polymerase. We show here that TraR activates transcription directly; however, unlike DksA, it does so without using ppGpp as a cofactor. TraR expression can stimulate the σ(E) extracytoplasmic stress response independently of the DegS/RseA signal transduction cascade. In the absence of TraR, bacteria carrying conjugative plasmids become more susceptible to external stress. We propose that TraR increases the concentrations of periplasmic chaperones and proteases by directly activating the transcription of σ(E)-dependent promoters; this increased protein folding capacity may prepare the bacterium to endure the periplasmic stress of sex pilus biosynthesis during mating., (Copyright © 2015, American Society for Microbiology. All Rights Reserved.)

Published

2015

36. Structure of the RNA polymerase assembly factor Crl and identification of its interaction surface with sigma S.

Author

Banta AB, Cuff ME, Lin H, Myers AR, Ross W, Joachimiak A, and Gourse RL

Subjects

Amino Acid Sequence, Bacterial Proteins chemistry, Bacterial Proteins genetics, Biological Evolution, Conserved Sequence, Crystallization, Models, Molecular, Molecular Sequence Data, Protein Conformation, Proteus mirabilis genetics, Proteus mirabilis metabolism, Sigma Factor genetics, Bacterial Proteins metabolism, Gene Expression Regulation, Bacterial physiology, Proteus mirabilis enzymology, Sigma Factor metabolism

Abstract

Bacteria utilize multiple sigma factors that associate with core RNA polymerase (RNAP) to control transcription in response to changes in environmental conditions. In Escherichia coli and Salmonella enterica, Crl positively regulates the σ(S) regulon by binding to σ(S) to promote its association with core RNAP. We recently characterized the determinants in σ(S) responsible for specific binding to Crl. However, little is known about the determinants in Crl required for this interaction. Here, we present the X-ray crystal structure of a Crl homolog from Proteus mirabilis in conjunction with in vivo and in vitro approaches that probe the Crl-σ(S) interaction in E. coli. We show that the P. mirabilis, Vibrio harveyi, and E. coli Crl homologs function similarly in E. coli, indicating that Crl structure and function are likely conserved throughout gammaproteobacteria. We utilize phylogenetic conservation and bacterial two-hybrid analyses to predict residues in Crl important for the interaction with σ(S). The results of p-benzoylphenylalanine (BPA)-mediated UV cross-linking studies further support the model in which an evolutionarily conserved central cleft is the surface on Crl that binds to σ(S). Within this conserved binding surface, we identify a key residue in Crl that is critical for activation of Eσ(S)-dependent transcription in vivo and in vitro. Our study provides a physical basis for understanding the σ(S)-Crl interaction., (Copyright © 2014, American Society for Microbiology. All Rights Reserved.)

Published

2014

37. A Rhodobacter sphaeroides protein mechanistically similar to Escherichia coli DksA regulates photosynthetic growth.

Author

Lennon CW, Lemmer KC, Irons JL, Sellman MI, Donohue TJ, Gourse RL, and Ross W

Subjects

Amino Acid Sequence, Amino Acids metabolism, Escherichia coli Proteins chemistry, Fatty Acids metabolism, Gene Deletion, Genetic Complementation Test, Models, Molecular, Molecular Sequence Data, Phenotype, Promoter Regions, Genetic, Protein Conformation, Rhodobacter sphaeroides growth & development, Sequence Alignment, Bacterial Proteins genetics, Bacterial Proteins metabolism, Escherichia coli Proteins genetics, Escherichia coli Proteins metabolism, Photosynthesis, Rhodobacter sphaeroides genetics, Rhodobacter sphaeroides metabolism

Abstract

ABSTRACT DksA is a global regulatory protein that, together with the alarmone ppGpp, is required for the "stringent response" to nutrient starvation in the gammaproteobacterium Escherichia coli and for more moderate shifts between growth conditions. DksA modulates the expression of hundreds of genes, directly or indirectly. Mutants lacking a DksA homolog exhibit pleiotropic phenotypes in other gammaproteobacteria as well. Here we analyzed the DksA homolog RSP2654 in the more distantly related Rhodobacter sphaeroides, an alphaproteobacterium. RSP2654 is 42% identical and similar in length to E. coli DksA but lacks the Zn finger motif of the E. coli DksA globular domain. Deletion of the RSP2654 gene results in defects in photosynthetic growth, impaired utilization of amino acids, and an increase in fatty acid content. RSP2654 complements the growth and regulatory defects of an E. coli strain lacking the dksA gene and modulates transcription in vitro with E. coli RNA polymerase (RNAP) similarly to E. coli DksA. RSP2654 reduces RNAP-promoter complex stability in vitro with RNAPs from E. coli or R. sphaeroides, alone and synergistically with ppGpp, suggesting that even though it has limited sequence identity to E. coli DksA (DksAEc), it functions in a mechanistically similar manner. We therefore designate the RSP2654 protein DksARsp. Our work suggests that DksARsp has distinct and important physiological roles in alphaproteobacteria and will be useful for understanding structure-function relationships in DksA and the mechanism of synergy between DksA and ppGpp. IMPORTANCE The role of DksA has been analyzed primarily in the gammaproteobacteria, in which it is best understood for its role in control of the synthesis of the translation apparatus and amino acid biosynthesis. Our work suggests that DksA plays distinct and important physiological roles in alphaproteobacteria, including the control of photosynthesis in Rhodobacter sphaeroides. The study of DksARsp, should be useful for understanding structure-function relationships in the protein, including those that play a role in the little-understood synergy between DksA and ppGpp.

Published

2014

38. Key features of σS required for specific recognition by Crl, a transcription factor promoting assembly of RNA polymerase holoenzyme.

Author

Banta AB, Chumanov RS, Yuan AH, Lin H, Campbell EA, Burgess RR, and Gourse RL

Subjects

DNA-Directed RNA Polymerases biosynthesis, Holoenzymes biosynthesis, Oligonucleotides genetics, Protein Interaction Mapping, Bacterial Proteins metabolism, DNA-Directed RNA Polymerases chemistry, Escherichia coli metabolism, Gene Expression Regulation, Bacterial physiology, Sigma Factor chemistry, Transcription Factors metabolism

Abstract

Bacteria use multiple sigma factors to coordinate gene expression in response to environmental perturbations. In Escherichia coli and other γ-proteobacteria, the transcription factor Crl stimulates σ(S)-dependent transcription during times of cellular stress by promoting the association of σ(S) with core RNA polymerase. The molecular basis for specific recognition of σ(S) by Crl, rather than the homologous and more abundant primary sigma factor σ(70), is unknown. Here we use bacterial two-hybrid analysis in vivo and p-benzoyl-phenylalanine cross-linking in vitro to define the features in σ(S) responsible for specific recognition by Crl. We identify residues in σ(S) conserved domain 2 (σ(S)2) that are necessary and sufficient to allow recognition of σ(70) conserved domain 2 by Crl, one near the promoter-melting region and the other at the position where a large nonconserved region interrupts the sequence of σ(70). We then use luminescence resonance energy transfer to demonstrate directly that Crl promotes holoenzyme assembly using these specificity determinants on σ(S). Our results explain how Crl distinguishes between sigma factors that are largely homologous and activates discrete sets of promoters even though it does not bind to promoter DNA.

Published

2013

39. Transcription of the Escherichia coli fatty acid synthesis operon fabHDG is directly activated by FadR and inhibited by ppGpp.

Author

My L, Rekoske B, Lemke JJ, Viala JP, Gourse RL, and Bouveret E

Subjects

Bacterial Proteins genetics, Escherichia coli genetics, Escherichia coli Proteins genetics, Escherichia coli Proteins metabolism, Gene Deletion, Promoter Regions, Genetic, Protein Binding, RNA, Bacterial genetics, RNA, Bacterial metabolism, Repressor Proteins genetics, Transcription Initiation, Genetic, Bacterial Proteins metabolism, Escherichia coli metabolism, Fatty Acids biosynthesis, Gene Expression Regulation, Bacterial physiology, Guanosine Tetraphosphate metabolism, Operon physiology, Repressor Proteins metabolism

Abstract

In Escherichia coli, FadR and FabR are transcriptional regulators that control the expression of fatty acid degradation and unsaturated fatty acid synthesis genes, depending on the availability of fatty acids. In this report, we focus on the dual transcriptional regulator FadR. In the absence of fatty acids, FadR represses the transcription of fad genes required for fatty acid degradation. However, FadR is also an activator, stimulating transcription of the products of the fabA and fabB genes responsible for unsaturated fatty acid synthesis. In this study, we show that FadR directly activates another fatty acid synthesis promoter, PfabH, which transcribes the fabHDG operon, indicating that FadR is a global regulator of both fatty acid degradation and fatty acid synthesis. We also demonstrate that ppGpp and its cofactor DksA, known primarily for their role in regulation of the synthesis of the translational machinery, directly inhibit transcription from the fabH promoter. ppGpp also inhibits the fadR promoter, thereby reducing transcription activation of fabH by FadR indirectly. Our study shows that both ppGpp and FadR have direct roles in the control of fatty acid promoters, linking expression in response to both translation activity and fatty acid availability.

Published

2013

40. RemA is a DNA-binding protein that activates biofilm matrix gene expression in Bacillus subtilis.

Author

Winkelman JT, Bree AC, Bate AR, Eichenberger P, Gourse RL, and Kearns DB

Subjects

Bacillus subtilis genetics, Bacillus subtilis metabolism, DNA, Bacterial metabolism, Gene Expression Profiling, Operon, Promoter Regions, Genetic, Protein Binding, Transcription, Genetic, Bacillus subtilis physiology, Biofilms growth & development, DNA-Binding Proteins metabolism, Gene Expression Regulation, Bacterial, Transcription Factors metabolism

Abstract

Biofilm formation in Bacillus subtilis requires expression of the eps and tapA-sipW-tasA operons to synthesize the extracellular matrix components, extracellular polysaccharide and TasA amyloid proteins, respectively. Expression of both operons is inhibited by the DNA-binding protein master regulator of biofilm formation SinR and activated by the protein RemA. Here we show that RemA is a DNA-binding protein that binds to multiple sites upstream of the promoters of both operons and is both necessary and sufficient for transcriptional activation in vivo and in vitro. We further show that SinR negatively regulates eps operon expression by occluding RemA binding and thus for the P(eps) promoter SinR functions as an anti-activator. Finally, transcriptional profiling indicated that RemA was primarily a regulator of the extracellular matrix genes, but it also activated genes involved in osmoprotection, leading to the identification of another direct target, the opuA operon., (© 2013 John Wiley & Sons Ltd.)

Published

2013

41. The magic spot: a ppGpp binding site on E. coli RNA polymerase responsible for regulation of transcription initiation.

Author

Ross W, Vrentas CE, Sanchez-Vazquez P, Gaal T, and Gourse RL

Subjects

Alleles, Amino Acid Sequence, Escherichia coli enzymology, Escherichia coli Proteins metabolism, Guanosine Tetraphosphate metabolism, Molecular Sequence Data, Mutation, Promoter Regions, Genetic, Protein Binding, Protein Subunits, Transcription, Genetic, Binding Sites genetics, DNA-Directed RNA Polymerases genetics, DNA-Directed RNA Polymerases metabolism, Escherichia coli genetics, Escherichia coli metabolism, Escherichia coli Proteins genetics, Guanosine Tetraphosphate genetics

Abstract

The global regulatory nucleotide ppGpp ("magic spot") regulates transcription from a large subset of Escherichia coli promoters, illustrating how small molecules can control gene expression promoter-specifically by interacting with RNA polymerase (RNAP) without binding to DNA. However, ppGpp's target site on RNAP, and therefore its mechanism of action, has remained unclear. We report here a binding site for ppGpp on E. coli RNAP, identified by crosslinking, protease mapping, and analysis of mutant RNAPs that fail to respond to ppGpp. A strain with a mutant ppGpp binding site displays properties characteristic of cells defective for ppGpp synthesis. The binding site is at an interface of two RNAP subunits, ω and β', and its position suggests an allosteric mechanism of action involving restriction of motion between two mobile RNAP modules. Identification of the binding site allows prediction of bacterial species in which ppGpp exerts its effects by targeting RNAP., (Copyright © 2013 Elsevier Inc. All rights reserved.)

Published

2013

42. Direct interactions between the coiled-coil tip of DksA and the trigger loop of RNA polymerase mediate transcriptional regulation.

Author

Lennon CW, Ross W, Martin-Tumasz S, Toulokhonov I, Vrentas CE, Rutherford ST, Lee JH, Butcher SE, and Gourse RL

Subjects

DNA-Directed RNA Polymerases chemistry, Escherichia coli genetics, Escherichia coli metabolism, Escherichia coli Proteins chemistry, Models, Molecular, Phenylalanine analogs & derivatives, Phenylalanine metabolism, Promoter Regions, Genetic genetics, Protein Binding, Protein Structure, Tertiary, Protein Subunits chemistry, Protein Subunits metabolism, DNA-Directed RNA Polymerases metabolism, Escherichia coli enzymology, Escherichia coli Proteins genetics, Escherichia coli Proteins metabolism, Gene Expression Regulation, Bacterial

Abstract

Escherichia coli DksA is a transcription factor that binds to RNA polymerase (RNAP) without binding to DNA, destabilizing RNAP-promoter interactions, sensitizing RNAP to the global regulator ppGpp, and regulating transcription of several hundred target genes, including those encoding rRNA. Previously, we described promoter sequences and kinetic properties that account for DksA's promoter specificity, but how DksA exerts its effects on RNAP has remained unclear. To better understand DksA's mechanism of action, we incorporated benzoyl-phenylalanine at specific positions in DksA and mapped its cross-links to RNAP, constraining computational docking of the two proteins. The resulting evidence-based model of the DksA-RNAP complex as well as additional genetic and biochemical approaches confirmed that DksA binds to the RNAP secondary channel, defined the orientation of DksA in the channel, and predicted a network of DksA interactions with RNAP that includes the rim helices and the mobile trigger loop (TL) domain. Engineered cysteine substitutions in the TL and DksA coiled-coil tip generated a disulfide bond between them, and the interacting residues were absolutely required for DksA function. We suggest that DksA traps the TL in a conformation that destabilizes promoter complexes, an interaction explaining the requirement for the DksA tip and its effects on transcription.

Published

2012

43. Role of the coiled-coil tip of Escherichia coli DksA in promoter control.

Author

Lee JH, Lennon CW, Ross W, and Gourse RL

Subjects

Amino Acid Sequence, DNA-Directed RNA Polymerases chemistry, Escherichia coli Proteins genetics, Models, Molecular, Molecular Sequence Data, Mutation, Protein Binding, Escherichia coli genetics, Escherichia coli Proteins chemistry, Gene Expression Regulation, Bacterial, Promoter Regions, Genetic

Abstract

Escherichia coli DksA works in conjunction with the small-molecule ppGpp to regulate transcription initiation negatively or positively, depending on the identity of the promoter. DksA is in a class of transcription factors that do not bind directly to DNA such as classical repressors or activators but rather bind in the RNA polymerase (RNAP) secondary channel such as the transcription elongation factors GreA and GreB in E. coli and TFIIS in eukaryotes. We found that substitution for either of two residues in its coiled-coil tip, D74 or A76, eliminates DksA function without affecting its apparent affinity for RNAP. The properties of DksA-Gre factor chimeras indicated that the coiled-coil tip is responsible for the DksA-specific effects on open complex formation. A conservative substitution at position 74, D74E, resulted in a loss of DksA function in both negative and positive control, and an E44D substitution at the analogous position in GreA resulted in a gain of function in both negative and positive control. That a single methylene group has such an extraordinary effect on these transcription factors highlights the critical nature of the identity of coiled-coil tip interactions with RNAP for open complex formation., (Copyright © 2011. Published by Elsevier Ltd.)

Published

2012

44. Suppression of a dnaKJ deletion by multicopy dksA results from non-feedback-regulated transcripts that originate upstream of the major dksA promoter.

Author

Chandrangsu P, Wang L, Choi SH, and Gourse RL

Subjects

Escherichia coli enzymology, Escherichia coli genetics, Escherichia coli Proteins metabolism, Feedback, Gene Expression, Gene Expression Regulation, Bacterial, HSP40 Heat-Shock Proteins metabolism, HSP70 Heat-Shock Proteins metabolism, Escherichia coli physiology, Escherichia coli Proteins biosynthesis, HSP40 Heat-Shock Proteins deficiency, HSP70 Heat-Shock Proteins deficiency, Promoter Regions, Genetic, Suppression, Genetic, Transcription, Genetic

Abstract

DksA is an RNA polymerase (RNAP) binding transcription factor that controls expression of a large number of genes in concert with the small-molecule "alarmone" ppGpp. DksA also aids in the resolution of conflicts between RNAP and DNA polymerase (DNAP) during genome replication. DksA was originally identified as a multicopy suppressor of the temperature sensitivity caused by deletion of the genes coding for the DnaKJ chaperone system. Here, we address a longstanding question regarding the role of DksA in ΔdnaKJ suppression. We demonstrate that DksA expression from a multicopy plasmid is necessary and sufficient for suppression, that overexpression occurs despite the fact that the major dksA promoter is feedback regulated in wild-type cells, and that weak, non-feedback-regulated transcription originating upstream of the major promoter for the dksA gene accounts for overexpression. We tentatively rule out three potential explanations for suppression related to known functions of DnaKJ. Because a determinant in DksA needed for the regulation of transcription initiation, but not for resolution of RNAP-DNAP conflicts, is needed to bypass the need for DnaKJ, we suggest that suppression results from an unidentified product whose promoter is directly or indirectly regulated by DksA.

Published

2012

45. CoSMoS unravels mysteries of transcription initiation.

Author

Gourse RL and Landick R

Abstract

Using a fluorescence method called colocalization single-molecule spectroscopy (CoSMoS), Friedman and Gelles dissect the kinetics of transcription initiation at a bacterial promoter. Ultimately, CoSMoS could greatly aid the study of the effects of DNA sequence and transcription factors on both prokaryotic and eukaryotic promoters., (Copyright © 2012 Elsevier Inc. All rights reserved.)

Published

2012

46. The dksA promoter is negatively feedback regulated by DksA and ppGpp.

Author

Chandrangsu P, Lemke JJ, and Gourse RL

Subjects

Escherichia coli metabolism, Gene Expression Regulation, Bacterial, Down-Regulation, Escherichia coli genetics, Escherichia coli Proteins genetics, Escherichia coli Proteins metabolism, Guanine Nucleotides metabolism, Promoter Regions, Genetic

Abstract

Escherichia coli DksA is an RNA polymerase (RNAP)-binding protein required for the regulation of a number of promoters, including those for the biosynthesis of rRNA, many ribosomal proteins, components of the flagellum, and several amino acids. Previous work demonstrated that DksA protein levels do not vary greatly in different growth conditions. We show here that DksA is a stable protein whose levels are kept constant by a negative feedback loop in which transcription from the dksA promoter is inhibited by DksA protein in conjunction with its cofactor ppGpp. We map the primary dksA promoter by primer extension, show that its activity increases in a strain lacking DksA, that the DksA protein accumulates when expressed from an exogenous promoter, that inhibition of transcription by DksA is direct since it occurs with purified components in vitro, and that inhibition correlates with effects of DksA on the lifetime of the dksA promoter complex. This work provides a mechanistic basis for the maintenance of constant cellular levels of DksA in E. coli and supports the model that transcription regulation by ppGpp/DksA derives from fluctuations in the concentrations of the small molecule cofactor rather than of DksA itself., (© 2011 Blackwell Publishing Ltd.)

Published

2011

47. Direct regulation of Escherichia coli ribosomal protein promoters by the transcription factors ppGpp and DksA.

Author

Lemke JJ, Sanchez-Vazquez P, Burgos HL, Hedberg G, Ross W, and Gourse RL

Subjects

Plasmids genetics, beta-Galactosidase, Escherichia coli genetics, Escherichia coli Proteins metabolism, Gene Expression Regulation, Bacterial genetics, Promoter Regions, Genetic genetics, Pyrophosphatases metabolism, Ribosomal Proteins genetics, Transcription Factors metabolism

Abstract

We show here that the promoters for many of the Escherichia coli ribosomal protein operons are regulated directly by two transcription factors, the small RNA polymerase-binding protein DksA and the nutritional stress-induced nucleotide ppGpp. ppGpp and DksA work together to inhibit transcription initiation from ribosomal protein promoters in vitro and in vivo. The degree of promoter regulation by ppGpp/DksA varies among the r-protein promoters, but some are inhibited almost as much as rRNA promoters. Thus, many r-protein operons are regulated at the level of transcription in addition to their control by the classic translational feedback systems discovered ~30 y ago. We conclude that direct control of r-protein promoters and rRNA promoters by the same signal, ppGpp/DksA, makes a major contribution to the balanced and coordinated synthesis rates of all of the ribosomal components.

Published

2011

48. An improved procedure for the purification of the Escherichia coli RNA polymerase omega subunit.

Author

Vrentas CE, Gaal T, Burgess RR, and Gourse RL

Subjects

DNA-Directed RNA Polymerases genetics, DNA-Directed RNA Polymerases metabolism, Escherichia coli genetics, Escherichia coli isolation & purification, DNA-Directed RNA Polymerases isolation & purification, Escherichia coli enzymology, Plasmids genetics, Plasmids metabolism

Abstract

We report an improved procedure for purification of the omega subunit of Escherichia coli RNA polymerase. In contrast to the original procedure, the revised procedure: (i) allows purification of omega entirely from the soluble fraction, obviating the need for denaturation/renaturation, (ii) results in >99% pure omega in only two chromatographic steps, and (iii) improves the yield of purified omega by at least 5-fold. Reconstitution of E. coli RNAP from omega purified by this procedure, as well as purified sigma and core RNAP lacking omega, produces active holoenzyme in vitro, and co-overexpression of omega from a plasmid containing rpoZ and an additional plasmid encoding the other RNAP core subunits results in production of active core enzyme in vivo.

Published

2010

49. DksA and ppGpp directly regulate transcription of the Escherichia coli flagellar cascade.

Author

Lemke JJ, Durfee T, and Gourse RL

Subjects

Escherichia coli Proteins genetics, Gene Deletion, Promoter Regions, Genetic, Escherichia coli physiology, Escherichia coli Proteins physiology, Flagellin biosynthesis, Gene Expression Regulation, Bacterial, Guanosine Tetraphosphate metabolism, Transcription, Genetic

Abstract

The components of the Escherichia coli flagella apparatus are synthesized in a three-level transcriptional cascade activated by the master regulator FlhDC. The cascade co-ordinates the synthesis rates of a large number of gene products with each other and with nutritional conditions. Recent genome-wide studies have reported that flagellar transcription is altered in cells lacking the transcription regulators DksA or ppGpp, but some or all reported effects could be indirect, and some are contradictory. We report here that the activities of promoters at all three levels of the cascade are much higher in strains lacking dksA, resulting in overproduction of flagellin and hyperflagellated cells. In vitro, DksA/ppGpp inhibits the flhDC promoter and the sigma(70)-dependent fliA promoter transcribing the gene for sigma(28). However, DksA and ppGpp do not affect the sigma(28)-dependent fliA promoter or the sigma(28)-dependent fliC promoter in vitro, suggesting that the dramatic effects on expression of those genes in vivo are mediated indirectly through direct effects of DksA/ppGpp on FlhDC and sigma(28) expression. We conclude that DksA/ppGpp inhibits expression of the flagellar cascade during stationary phase and following starvation, thereby co-ordinating flagella and ribosome assembly and preventing expenditure of scarce energy resources on synthesis of two of the cell's largest macromolecular complexes.

Published

2009

50. Escherichia coli DksA binds to Free RNA polymerase with higher affinity than to RNA polymerase in an open complex.

Author

Lennon CW, Gaal T, Ross W, and Gourse RL

Subjects

Binding Sites, Catalytic Domain, DNA, Bacterial genetics, DNA, Bacterial metabolism, DNA-Directed RNA Polymerases chemistry, DNA-Directed RNA Polymerases genetics, Escherichia coli Proteins genetics, Ferrous Compounds metabolism, Gene Expression Regulation, Bacterial, Holoenzymes, Models, Molecular, Protein Binding, Protein Conformation, DNA-Directed RNA Polymerases metabolism, Escherichia coli Proteins metabolism

Abstract

The transcription factor DksA binds in the secondary channel of RNA polymerase (RNAP) and alters transcriptional output without interacting with DNA. Here we present a quantitative assay for measuring DksA binding affinity and illustrate its utility by determining the relative affinities of DksA for three different forms of RNAP. Whereas the apparent affinities of DksA for RNAP core and holoenzyme are the same, the apparent affinity of DksA for RNAP decreases almost 10-fold in an open complex. These results suggest that the conformation of RNAP present in an open complex is not optimal for DksA binding and that DNA directly or indirectly alters the interface between the two proteins.

Published

2009