Your search keyword '"Dickeya chrysanthemi metabolism"' showing total 120 results

1. Trigalacturonate-producing pectate lyase PelQ1 from Saccharobesus litoralis with unique exolytic activity.

Author

Lian MQ, Furusawa G, and Teh AH

Subjects

Polysaccharide-Lyases metabolism, Dickeya chrysanthemi metabolism

Abstract

PelQ1 from Saccharobesus litoralis is a Ca 2+ -dependent pectate lyase belonging to the polysaccharide lyase family 1 (PL1). Although being an endolytic enzyme, it degraded polygalacturonate into predominantly unsaturated trimer in an exolytic manner with delayed production of dimer, tetramer and pentamer. The enzyme harbours a C-terminal domain from the carbohydrate-binding module family 13 (CBM13), whose presence facilitated the production of dimer. PelQ1's homology model showed that it possessed a well-conserved catalytic cleft, with R232 acting as the general base and R203 as the general acid. Structural comparison with DcPelC, a similar trimer-generating pectate lyase from Dickeya chrysanthemi EC16, implied that both enzymes' catalytic clefts encompassed at least eight subsites, i.e. -5 to +3. The unequal distribution of the subsites between the reducing and non-reducing ends of the cleavage site might be responsible for the exolytic generation of the trimer. As all but the -1, +1 and + 2 subsites could accommodate methylated galacturonate, this subclass of PL1 pectate lyases may function to help break up methylated pectin., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 Elsevier Ltd. All rights reserved.)

Published

2024

2. Development of a bioengineered Erwinia chrysanthemi asparaginase to enhance its anti-solid tumor potential for treating gastric cancer.

Author

Tam SY, Chung SF, Kim CF, To JC, So PK, Cheung KK, Chung WH, Wong KY, and Leung YC

Subjects

Humans, Animals, Mice, Asparaginase genetics, Asparaginase pharmacology, Asparaginase therapeutic use, Asparagine, Glutamine, Enterobacteriaceae metabolism, Serum Albumin, Antineoplastic Agents pharmacology, Antineoplastic Agents therapeutic use, Dickeya chrysanthemi genetics, Dickeya chrysanthemi metabolism, Stomach Neoplasms drug therapy

Abstract

Asparaginase has been traditionally applied for only treating acute lymphoblastic leukemia due to its ability to deplete asparagine. However, its ultimate anticancer potential for treating solid tumors has not yet been unleashed. In this study, we bioengineered Erwinia chrysanthemi asparaginase (ErWT), one of the US Food and Drug Administration-approved types of amino acid depleting enzymes, to achieve double amino acid depletions for treating a solid tumor. We constructed a fusion protein by joining an albumin binding domain (ABD) to ErWT via a linker (GGGGS) 5 to achieve ABD-ErS5. The ABD could bind to serum albumin to form an albumin-ABD-ErS5 complex, which could avoid renal clearance and escape from anti-drug antibodies, resulting in a remarkably prolonged elimination half-life of ABD-ErS5. Meanwhile, ABD-ErS5 did not only deplete asparagine but also glutamine for ∼2 weeks. A biweekly administration of ABD-ErS5 (1.5 mg/kg) significantly suppressed tumor growth in an MKN-45 gastric cancer xenograft model, demonstrating a novel approach for treating solid tumor depleting asparagine and glutamine. Multiple administrations of ABD-ErS5 did not cause any noticeable histopathological abnormalities of key organs, suggesting the absence of acute toxicity to mice. Our results suggest ABD-ErS5 is a potential therapeutic candidate for treating gastric cancer., Competing Interests: Declaration of competing interest The authors declare that they have no conflict of interest., (Copyright © 2023. Published by Elsevier B.V.)

Published

2023

3. The Right-Handed Parallel β-Helix Topology of Erwinia chrysanthemi Pectin Methylesterase Is Intimately Associated with Both Sequential Folding and Resistance to High Pressure.

Author

Guillerm J, Frère JM, Meersman F, and Matagne A

Subjects

Amino Acid Motifs, Circular Dichroism, Hydrogen-Ion Concentration, Kinetics, Linear Models, Models, Molecular, Pressure, Protein Binding, Protein Conformation, Protein Denaturation, Protein Folding, Protein Structure, Secondary, Spectrophotometry, Ultraviolet, Temperature, Thermodynamics, Carboxylic Ester Hydrolases chemistry, Dickeya chrysanthemi metabolism

Abstract

The complex topologies of large multi-domain globular proteins make the study of their folding and assembly particularly demanding. It is often characterized by complex kinetics and undesired side reactions, such as aggregation. The structural simplicity of tandem-repeat proteins, which are characterized by the repetition of a basic structural motif and are stabilized exclusively by sequentially localized contacts, has provided opportunities for dissecting their folding landscapes. In this study, we focus on the Erwinia chrysanthemi pectin methylesterase (342 residues), an all-β pectinolytic enzyme with a right-handed parallel β-helix structure. Chemicals and pressure were chosen as denaturants and a variety of optical techniques were used in conjunction with stopped-flow equipment to investigate the folding mechanism of the enzyme at 25 °C. Under equilibrium conditions, both chemical- and pressure-induced unfolding show two-state transitions, with average conformational stability (Δ G ° = 35 ± 5 kJ·mol -1 ) but exceptionally high resistance to pressure ( P m = 800 ± 7 MPa). Stopped-flow kinetic experiments revealed a very rapid (τ < 1 ms) hydrophobic collapse accompanied by the formation of an extended secondary structure but did not reveal stable tertiary contacts. This is followed by three distinct cooperative phases and the significant population of two intermediate species. The kinetics followed by intrinsic fluorescence shows a lag phase, strongly indicating that these intermediates are productive species on a sequential folding pathway, for which we propose a plausible model. These combined data demonstrate that even a large repeat protein can fold in a highly cooperative manner.

Published

2021

4. Determination of glycation levels in Erwinia chrysanthemi asparaginase drug product by liquid chromatography - mass spectrometry.

Author

Kanda P and Minshull TC

Subjects

Asparaginase analysis, Chromatography, Liquid methods, Dickeya chrysanthemi chemistry, Glycosylation, Humans, Isoelectric Focusing methods, Mass Spectrometry methods, Asparaginase metabolism, Chemistry, Pharmaceutical methods, Dickeya chrysanthemi metabolism

Abstract

Erwinase (Erwinia chrysanthemi L-asparaginase) Drug Product (DP) is a freeze-dried formulation with a three-year shelf life at 2-8  ° C, and an established safety, stability and efficacy profile over the more than three decades of clinical use. Seven Erwinase® DP batches, released over a 7-year period, were screened by reversed-phase liquid chromatography coupled to time-of-flight mass spectrometry for glycation levels. This modification is a known and natural consequence of exposure of Erwinase Drug Product to glucose excipients in stabilizing formulations. Although glycation is detected in current release and stability methods, glycation, including the conditions under which this reaction occurs, has not been previously characterised in detail. We have found that glycation levels of different DP lots generally correlated with age, when they were stored at low temperature. This suggests that the glycation reaction continues over time within the Drug Product formulation in the lyophilised state, even under low temperature (+2-8 °C) conditions. We were also able to examine glycation levels of one DP lot, Lot D, held under long term stability at 3 different temperatures over a 5-year period. The 2 samples held at -20 °C and -80 °C, were glycated to levels of 12% and 17%, respectively. However, the DP Lot D sample held at +2-8  o C in this time period was found to be glycated to a level of 35.6%, with multiple glycations of individual subunits observed. For analytical reference materials, it is important to keep parameters such as glycation levels as constant as possible, to avoid a 'moving target' with respect to comparisons with release and stability testing. These data suggest that storage of DP as reference standards at a lower temperature (e.g., -20 °C) can significantly reduce levels of glycation over the longer time periods required for analytical reference standards., (Copyright © 2020 Elsevier B.V. All rights reserved.)

Published

2020

5. Amino acid substitutions in the human homomeric β 3 GABA A receptor that enable activation by GABA.

Author

Gottschald Chiodi C, Baptista-Hon DT, Hunter WN, and Hales TG

Subjects

Amino Acid Substitution, Catalytic Domain, Dickeya chrysanthemi chemistry, Dickeya chrysanthemi genetics, Dickeya chrysanthemi metabolism, HEK293 Cells, Humans, Propofol pharmacology, gamma-Aminobutyric Acid chemistry, gamma-Aminobutyric Acid metabolism, Ion Channel Gating, Mutation, Missense, Protein Structure, Secondary, Receptors, GABA-B chemistry, Receptors, GABA-B genetics, Receptors, GABA-B metabolism

Abstract

GABA A receptors (GABA A Rs) are pentameric ligand-gated ion channels that mediate synaptic inhibition throughout the central nervous system. The α 1 β 2 γ 2 receptor is the major subtype in the brain; GABA binds at the β 2 (+)α 1 (-) interface. The structure of the homomeric β 3 GABA A R, which is not activated by GABA, has been solved. Recently, four additional heteromeric structures were reported, highlighting key residues required for agonist binding. Here, we used a protein engineering method, taking advantage of knowledge of the key binding residues, to create a β 3 (+)α 1 (-) heteromeric interface in the homomeric human β 3 GABA A R that enables GABA-mediated activation. Substitutions were made in the complementary side of the orthosteric binding site in loop D (Y87F and Q89R), loop E (G152T), and loop G (N66D and A70T). The Q89R and G152T combination enabled low-potency activation by GABA and potentiation by propofol but impaired direct activation by higher propofol concentrations. At higher concentrations, GABA inhibited gating of β 3 GABA A R variants containing Y87F, Q89R, and G152T. Reversion of Phe 87 to tyrosine abolished GABA's inhibitory effect and partially recovered direct activation by propofol. This tyrosine is conserved in homomeric GABA A Rs and in the Erwinia chrysanthemi ligand-gated ion channel and may be essential for the absence of an inhibitory effect of GABA on homomeric channels. This work demonstrated that only two substitutions, Q89R and G152T, in β 3 GABA A R are sufficient to reconstitute GABA-mediated activation and suggests that Tyr 87 prevents inhibitory effects of GABA., (© 2019 Gottschald Chiodi et al.)

Published

2019

6. In Vitro Formation of Dickeya zeae MS1 Biofilm.

Author

Huang N, Pu X, Zhang J, Shen H, Yang Q, Wang Z, and Lin B

Subjects

Dickeya chrysanthemi isolation & purification, Environment, Microscopy, Confocal, Plant Diseases microbiology, Sucrose metabolism, Biofilms growth & development, Dickeya chrysanthemi growth & development, Dickeya chrysanthemi metabolism, Musa microbiology, Polysaccharides, Bacterial metabolism

Abstract

Bacterial soft rot caused by Dickeya zeae MS1 (Erwinia chrysanthemi) is one of the most devastating banana diseases worldwide. However, knowledge of the development and ecological interactions of D. zeae MS1 biofilm is limited. Here, we visualized the development and architecture of D. zeae MS1 biofilm using confocal laser scanning microscopy, and we evaluated the ability of D. zeae MS1 to form biofilms under different environmental conditions (carbon sources, temperatures, pH levels and mineral elements) using a microtiter plate assay. We found that the development of D. zeae MS1 biofilm could be categorized into four phases and that mature biofilm consisted of a highly organized architecture of both bacterial cells and a self-produced matrix of extracellular polysaccharides. Furthermore, sucrose was the most suitable carbon source for supporting the growth of biofilm cells and that 32 °C and pH 7.0 were the most favorable of the temperatures and pH levels examined. Meanwhile, the addition of Ca 2+ , Fe 2+ , K + and Na + enhanced the formation of biofilm in minimal medium cultures, whereas 2.5 mM Cu 2+ and Mn 2+ was inhibitory. A better understanding of biofilm formation under different environmental parameters will improve our knowledge of the growth kinetics of D. zeae MS1 biofilm.

Published

2019

7. From hopanoids to cholesterol: Molecular clocks of pentameric ligand-gated ion channels.

Author

Barrantes FJ and Fantini J

Subjects

Bacterial Proteins chemistry, Cyanobacteria metabolism, Dickeya chrysanthemi metabolism, Ligand-Gated Ion Channels chemistry, Protein Binding, Protein Structure, Quaternary, Triterpenes chemistry, Bacterial Proteins metabolism, Biological Clocks physiology, Cholesterol metabolism, Ligand-Gated Ion Channels metabolism, Triterpenes metabolism

Abstract

Pentameric ligand-gated ion channels (pLGICs) and their lipid microenvironments appear to have acquired mutually adaptive traits along evolution: 1) the three-ring architecture of their transmembrane (TM) region; 2) the ability of the outermost TM ring to convey lipid signals to the middle ring, which passes them on to the central pore ring, and 3) consensus motifs for sterol recognition in all pLGICs. Hopanoids are triterpenoid fossil lipids that constitute invaluable biomarkers for tracing evolution at the molecular scale. The cyanobacterium Gloeobacter violaceus is the oldest known living organism in which the X-ray structure of its pLGIC, GLIC, reveals the presence of the above attributes and, as discussed in this review, the ability to bind hopanoids. ELIC, the pLGIC from the bacillus Erwinia chrysanthemi is the only other known case to date. Both prokaryotes lack cholesterol but their pLGICs exhibit the same sterol motifs as mammalian pLGIC. This remarkable conservation suggests that the association of sterols and hopanoid surrogate molecules arose from the early need in prokaryotes to stabilize pLGIC TM regions by means of relatively rigid lipid molecules. The conservation of these phenotypic traits along such a long phylogenetic span leads us to suggest the possible co-evolution of these sterols with pLGICs., (Copyright © 2016 Elsevier B.V. All rights reserved.)

Published

2016

8. Structural Insight into Substrate Selectivity of Erwinia chrysanthemi L-asparaginase.

Author

Nguyen HA, Su Y, and Lavie A

Subjects

Asparaginase chemistry, Aspartic Acid metabolism, Crystallography, X-Ray, Dickeya chrysanthemi chemistry, Dickeya chrysanthemi metabolism, Glutamic Acid metabolism, Humans, Models, Molecular, Protein Conformation, Substrate Specificity, Asparaginase metabolism, Dickeya chrysanthemi enzymology

Abstract

l-Asparaginases of bacterial origin are a mainstay of acute lymphoblastic leukemia treatment. The mechanism of action of these enzyme drugs is associated with their capacity to deplete the amino acid l-asparagine from the blood. However, clinical use of bacterial l-asparaginases is complicated by their dual l-asparaginase and l-glutaminase activities. The latter, even though representing only ∼10% of the overall activity, is partially responsible for the observed toxic side effects. Hence, l-asparaginases devoid of l-glutaminase activity hold potential as safer drugs. Understanding the key determinants of l-asparaginase substrate specificity is a prerequisite step toward the development of enzyme variants with reduced toxicity. Here we present crystal structures of the Erwinia chrysanthemi l-asparaginase in complex with l-aspartic acid and with l-glutamic acid. These structures reveal two enzyme conformations-open and closed-corresponding to the inactive and active states, respectively. The binding of ligands induces the positioning of the catalytic Thr15 into its active conformation, which in turn allows for the ordering and closure of the flexible N-terminal loop. Notably, l-aspartic acid is more efficient than l-glutamic acid in inducing the active positioning of Thr15. Structural elements explaining the preference of the enzyme for l-asparagine over l-glutamine are discussed with guidance to the future development of more specific l-asparaginases.

Published

2016

9. Consensus expert recommendations for identification and management of asparaginase hypersensitivity and silent inactivation.

Author

van der Sluis IM, Vrooman LM, Pieters R, Baruchel A, Escherich G, Goulden N, Mondelaers V, Sanchez de Toledo J, Rizzari C, Silverman LB, and Whitlock JA

Subjects

Antibodies, Neutralizing biosynthesis, Antibodies, Neutralizing blood, Antineoplastic Agents blood, Antineoplastic Agents pharmacokinetics, Asparaginase antagonists & inhibitors, Asparaginase blood, Asparaginase pharmacokinetics, Consensus, Dickeya chrysanthemi genetics, Dickeya chrysanthemi metabolism, Drug Hypersensitivity diagnosis, Drug Hypersensitivity etiology, Drug Monitoring, Drug Substitution, Escherichia coli genetics, Escherichia coli metabolism, Gene Expression, Humans, Precursor Cell Lymphoblastic Leukemia-Lymphoma blood, Precursor Cell Lymphoblastic Leukemia-Lymphoma pathology, Recombinant Proteins blood, Recombinant Proteins pharmacokinetics, Recombinant Proteins therapeutic use, Antineoplastic Agents therapeutic use, Asparaginase therapeutic use, Disease Management, Drug Hypersensitivity prevention & control, Precursor Cell Lymphoblastic Leukemia-Lymphoma drug therapy

Abstract

L-asparaginase is an integral component of therapy for acute lymphoblastic leukemia. However, asparaginase-related complications, including the development of hypersensitivity reactions, can limit its use in individual patients. Of considerable concern in the setting of clinical allergy is the development of neutralizing antibodies and associated asparaginase inactivity. Also problematic in the use of asparaginase is the potential for the development of silent inactivation, with the formation of neutralizing antibodies and reduced asparaginase activity in the absence of a clinically evident allergic reaction. Here we present guidelines for the identification and management of clinical hypersensitivity and silent inactivation with Escherichia coli- and Erwinia chrysanthemi- derived asparaginase preparations. These guidelines were developed by a consensus panel of experts following a review of the available published data. We provide a consensus of expert opinions on the role of serum asparaginase level assessment, indications for switching asparaginase preparation, and monitoring after change in asparaginase preparation., (Copyright© Ferrata Storti Foundation.)

Published

2016

10. Macroscopic kinetics of pentameric ligand gated ion channels: comparisons between two prokaryotic channels and one eukaryotic channel.

Author

Laha KT, Ghosh B, and Czajkowski C

Subjects

Animals, Crystallography, X-Ray methods, Dickeya chrysanthemi metabolism, HEK293 Cells, Humans, Kinetics, Rats, Receptors, GABA-A chemistry, Xenopus laevis metabolism, Eukaryotic Cells metabolism, Ligand-Gated Ion Channels chemistry, Ligand-Gated Ion Channels metabolism, Prokaryotic Cells metabolism

Abstract

Electrochemical signaling in the brain depends on pentameric ligand-gated ion channels (pLGICs). Recently, crystal structures of prokaryotic pLGIC homologues from Erwinia chrysanthemi (ELIC) and Gloeobacter violaceus (GLIC) in presumed closed and open channel states have been solved, which provide insight into the structural mechanisms underlying channel activation. Although structural studies involving both ELIC and GLIC have become numerous, thorough functional characterizations of these channels are still needed to establish a reliable foundation for comparing kinetic properties. Here, we examined the kinetics of ELIC and GLIC current activation, desensitization, and deactivation and compared them to the GABAA receptor, a prototypic eukaryotic pLGIC. Outside-out patch-clamp recordings were performed with HEK-293T cells expressing ELIC, GLIC, or α1β2γ2L GABAA receptors, and ultra-fast ligand application was used. In response to saturating agonist concentrations, we found both ELIC and GLIC current activation were two to three orders of magnitude slower than GABAA receptor current activation. The prokaryotic channels also had slower current desensitization on a timescale of seconds. ELIC and GLIC current deactivation following 25 s pulses of agonist (cysteamine and pH 4.0 buffer, respectively) were relatively fast with time constants of 24.9 ± 5.1 ms and 1.2 ± 0.2 ms, respectively. Surprisingly, ELIC currents evoked by GABA activated very slowly with a time constant of 1.3 ± 0.3 s and deactivated even slower with a time constant of 4.6 ± 1.2 s. We conclude that the prokaryotic pLGICs undergo similar agonist-mediated gating transitions to open and desensitized states as eukaryotic pLGICs, supporting their use as experimental models. Their uncharacteristic slow activation, slow desensitization and rapid deactivation time courses are likely due to differences in specific structural elements, whose future identification may help uncover mechanisms underlying pLGIC gating transitions.

Published

2013

11. Cysteine scanning mutagenesis and disulfide mapping analysis of arrangement of GspC and GspD protomers within the type 2 secretion system.

Author

Wang X, Pineau C, Gu S, Guschinskaya N, Pickersgill RW, and Shevchik VE

Subjects

Bacterial Proteins genetics, Cysteine genetics, Cysteine metabolism, Dickeya chrysanthemi genetics, Membrane Proteins genetics, Mutagenesis, Peptide Mapping methods, Protein Structure, Tertiary, Bacterial Proteins metabolism, Bacterial Secretion Systems physiology, Dickeya chrysanthemi metabolism, Disulfides metabolism, Membrane Proteins metabolism, Protein Multimerization

Abstract

The type II secretion system (T2SS) secretes enzymes and toxins across the outer membrane of Gram-negative bacteria. The precise assembly of T2SS, which consists of at least 12 core-components called Gsp, remains unclear. The outer membrane secretin, GspD, forms the channels, through which folded proteins are secreted, and interacts with the inner membrane component, GspC. The periplasmic regions of GspC and GspD consist of several structural domains, HR(GspC) and PDZ(GspC), and N0(GspD) to N3(GspD), respectively, and recent structural and functional studies have proposed several interaction sites between these domains. We used cysteine mutagenesis and disulfide bonding analysis to investigate the organization of GspC and GspD protomers and to map their interaction sites within the secretion machinery of the plant pathogen Dickeya dadantii. At least three distinct GspC-GspD interactions were detected, and they involve two sites in HR(GspC), two in N0(GspD), and one in N2(GspD). None of these interactions occurs through static interfaces because the same sites are also involved in self-interactions with equivalent neighboring domains. Disulfide self-bonding of critical interaction sites halts secretion, indicating the transient nature of these interactions. The secretion substrate diminishes certain interactions and provokes an important rearrangement of the HR(GspC) structure. The T2SS components OutE/L/M affect various interaction sites differently, reinforcing some but diminishing the others, suggesting a possible switching mechanism of these interactions during secretion. Disulfide mapping shows that the organization of GspD and GspC subunits within the T2SS could be compatible with a hexamer of dimers arrangement rather than an organization with 12-fold rotational symmetry.

Published

2012

12. Structure of the pentameric ligand-gated ion channel ELIC cocrystallized with its competitive antagonist acetylcholine.

Author

Pan J, Chen Q, Willenbring D, Yoshida K, Tillman T, Kashlan OB, Cohen A, Kong XP, Xu Y, and Tang P

Subjects

Acetylcholine metabolism, Crystallography, X-Ray, Cysteine Loop Ligand-Gated Ion Channel Receptors metabolism, Dickeya chrysanthemi cytology, Dickeya chrysanthemi metabolism, Ion Channel Gating, Ligand-Gated Ion Channels antagonists & inhibitors, Models, Molecular, Molecular Dynamics Simulation, Protein Structure, Quaternary, Protein Structure, Tertiary, Quaternary Ammonium Compounds chemistry, Quaternary Ammonium Compounds metabolism, Static Electricity, Acetylcholine chemistry, Cysteine Loop Ligand-Gated Ion Channel Receptors chemistry, Dickeya chrysanthemi chemistry, Ligand-Gated Ion Channels chemistry, Ligand-Gated Ion Channels metabolism

Abstract

ELIC, the pentameric ligand-gated ion channel from Erwinia chrysanthemi, is a prototype for Cys-loop receptors. Here we show that acetylcholine is a competitive antagonist for ELIC. We determine the acetylcholine-ELIC cocrystal structure to a 2.9-Å resolution and find that acetylcholine binding to an aromatic cage at the subunit interface induces a significant contraction of loop C and other structural rearrangements in the extracellular domain. The side chain of the pore-lining residue F247 reorients and the pore size consequently enlarges, but the channel remains closed. We attribute the inability of acetylcholine to activate ELIC primarily to weak cation-π and electrostatic interactions in the pocket, because an acetylcholine derivative with a simple quaternary-to-tertiary ammonium substitution activates the channel. This study presents a compelling case for understanding the structural underpinning of the functional relationship between agonism and competitive antagonism in the Cys-loop receptors, providing a new framework for developing novel therapeutic drugs.

Published

2012

13. Dickeya dadantii, a plant pathogenic bacterium producing Cyt-like entomotoxins, causes septicemia in the pea aphid Acyrthosiphon pisum.

Author

Costechareyre D, Balmand S, Condemine G, and Rahbé Y

Subjects

Animals, Animals, Genetically Modified, Aphids embryology, Aphids genetics, Aphids physiology, Bacillus thuringiensis Toxins, Bacterial Proteins genetics, Bacterial Proteins metabolism, Bacterial Toxins genetics, Dickeya chrysanthemi genetics, Dickeya chrysanthemi metabolism, Dickeya chrysanthemi pathogenicity, Disease Vectors, Embryo, Nonmammalian microbiology, Endotoxins genetics, Endotoxins metabolism, Enterobacteriaceae Infections genetics, Enterobacteriaceae Infections veterinary, Gene Expression Regulation, Hemolysin Proteins genetics, Hemolysin Proteins metabolism, Intestines embryology, Intestines microbiology, Pisum sativum parasitology, Plant Diseases microbiology, Sepsis genetics, Sepsis veterinary, Aphids microbiology, Bacterial Toxins metabolism, Dickeya chrysanthemi physiology, Enterobacteriaceae Infections microbiology, Sepsis microbiology

Abstract

Dickeya dadantii (syn. Erwinia chrysanthemi) is a plant pathogenic bacteria that harbours a cluster of four horizontally-transferred, insect-specific toxin genes. It was recently shown to be capable of causing an acute infection in the pea aphid Acyrthosiphon pisum (Insecta: Hemiptera). The infection route of the pathogen, and the role and in vivo expression pattern of these toxins, remain unknown. Using bacterial numeration and immunolocalization, we investigated the kinetics and the pattern of infection of this phytopathogenic bacterium within its insect host. We compared infection by the wild-type strain and by the Cyt toxin-deficient mutant. D. dadantii was found to form dense clusters in many luminal parts of the aphid intestinal tract, including the stomach, from which it invaded internal tissues as early as day 1 post-infection. Septicemia occurred soon after, with the fat body being the main infected tissue, together with numerous early infections of the embryonic chains showing embryonic gut and fat body as the target organs. Generalized septicemia led to insect death when the bacterial load reached about 10(8) cfu. Some individual aphids regularly escaped infection, indicating an effective partial immune response to this bacteria. Cyt-defective mutants killed insects more slowly but were capable of localisation in any type of tissue. Cyt toxin expression appeared to be restricted to the digestive tract where it probably assisted in crossing over the first cell barrier and, thus, accelerating bacterial diffusion into the aphid haemocel. Finally, the presence of bacteria on the surface of leaves hosting infected aphids indicated that the insects could be vectors of the bacteria.

Published

2012

14. A structure-based QSAR and docking study on imidazo[1,5-a][1,2,4]-triazolo[1,5-d][1,4,]benzodiazepines as Selective GABA(A) α5 inverse agonists.

Author

Gharaghani S, Khayamian T, and Keshavarz F

Subjects

Amino Acid Sequence, Bacterial Proteins chemistry, Bacterial Proteins metabolism, Binding Sites, Dickeya chrysanthemi chemistry, Dickeya chrysanthemi metabolism, Molecular Dynamics Simulation, Molecular Sequence Data, Protein Binding, Receptors, GABA-A chemistry, Receptors, GABA-A metabolism, Sequence Alignment, Benzodiazepines chemistry, Benzodiazepines pharmacology, Drug Design, GABA-A Receptor Agonists chemistry, GABA-A Receptor Agonists pharmacology, Quantitative Structure-Activity Relationship

Abstract

As three-dimensional (3D) structure of the GABA(A) α5 was not determined, the crystal structure of 2Vl0E at 3.3 Å resolution which is a ligand-gated K(+) channel was used as a template in homology modeling, and the result was used in molecular dynamic simulation for obtaining its conformation in a water sphere. The resulted conformation of the receptor was used for docking with the most potent of imidazo[1,5-a][1,2,4]-triazolo[1,5-d][1,4,] benzodiazepines drugs to find out binding sites and consequently the types of the interaction between the drugs and receptor. The results showed that π-π interaction of the drugs with three phenylalanine and tyrosine residues plays an important role in determining the potency of the inhibitors. The obtained information relating to the binding sites of the receptor was utilized for docking all the drugs into the receptor and find out optimized conformation for each drug, used in structure-based quantitative structure-activity relationship (QSAR) model for calculation of descriptors. Then, selected descriptors were related to the binding affinity and selectivity of the drugs using multiple linear regression and least squares-support vector regression. Finally, the results of target- and ligand-based QSAR models were compared, resulted the superiority of the structure-based QSAR to the ligand-based model., (© 2011 John Wiley & Sons A/S.)

Published

2011

15. Addition of genes for cellobiase and pectinolytic activity in Escherichia coli for fuel ethanol production from pectin-rich lignocellulosic biomass.

Author

Edwards MC, Henriksen ED, Yomano LP, Gardner BC, Sharma LN, Ingram LO, and Doran Peterson J

Subjects

Bacterial Proteins genetics, Bacterial Proteins metabolism, Carboxylic Ester Hydrolases metabolism, Carboxylic Ester Hydrolases pharmacology, Cosmids genetics, Dickeya chrysanthemi genetics, Dickeya chrysanthemi metabolism, Escherichia coli genetics, Fermentation, Genetic Engineering, Klebsiella oxytoca genetics, Klebsiella oxytoca metabolism, Phosphoenolpyruvate Sugar Phosphotransferase System genetics, Phosphoenolpyruvate Sugar Phosphotransferase System metabolism, Polysaccharide-Lyases genetics, Polysaccharide-Lyases metabolism, Biofuels, Biomass, Escherichia coli metabolism, Ethanol metabolism, Lignin metabolism, Pectins metabolism, beta-Glucosidase metabolism

Abstract

Ethanologenic Escherichia coli strain KO11 was sequentially engineered to contain the Klebsiella oxytoca cellobiose phosphotransferase genes (casAB) as well as a pectate lyase (pelE) from Erwinia chrysanthemi, yielding strains LY40A (casAB) and JP07 (casAB pelE), respectively. To obtain an effective secretion of PelE, the Sec-dependent pathway out genes from E. chrysanthemi were provided on a cosmid to strain JP07 to construct strain JP07C. Finally, oligogalacturonide lyase (ogl) from E. chrysanthemi was added to produce strain JP08C. E. coli strains LY40A, JP07, JP07C, and JP08C possessed significant cellobiase activity in cell lysates, while only strains JP07C and JP08C demonstrated extracellular pectate lyase activity. Fermentations conducted by using a mixture of pure sugars representative of the composition of sugar beet pulp (SBP) showed that strains LY40A, JP07, JP07C, and JP08C were able to ferment cellobiose, resulting in increased ethanol production from 15 to 45% in comparison to that of KO11. Fermentations with SBP at very low fungal enzyme loads during saccharification revealed significantly higher levels of ethanol production for LY40A, JP07C, and JP08C than for KO11. JP07C ethanol yields were not considerably higher than those of LY40A; however, oligogalacturonide polymerization studies showed an increased breakdown of biomass to small-chain (degree of polymerization, ≤6) oligogalacturonides. JP08C achieved a further breakdown of polygalacturonate to monomeric sugars, resulting in a 164% increase in ethanol yields compared to those of KO11. The addition of commercial pectin methylesterase (PME) further increased JP08C ethanol production compared to that of LY40A by demethylating the pectin for enzymatic attack by pectin-degrading enzymes.

Published

2011

16. Ligand bound structures of a glycosyl hydrolase family 30 glucuronoxylan xylanohydrolase.

Author

St John FJ, Hurlbert JC, Rice JD, Preston JF, and Pozharski E

Subjects

Binding Sites, Crystallography, X-Ray, Dickeya chrysanthemi enzymology, Hydrolysis, Ligands, Models, Molecular, Protein Binding, Protein Conformation, Protein Structure, Tertiary, Substrate Specificity, Dickeya chrysanthemi metabolism, Glycoside Hydrolases chemistry, Glycoside Hydrolases metabolism, Xylans chemistry, Xylans metabolism, Xylosidases chemistry, Xylosidases metabolism

Abstract

Xylanases of glycosyl hydrolase family 30 (GH30) have been shown to cleave β-1,4 linkages of 4-O-methylglucuronoxylan (MeGX(n)) as directed by the position along the xylan chain of an α-1,2-linked 4-O-methylglucuronate (MeGA) moiety. Complete hydrolysis of MeGX(n) by these enzymes results in singly substituted aldouronates having a 4-O-methylglucuronate moiety linked to a xylose penultimate from the reducing terminal xylose and some number of xylose residues toward the nonreducing terminus. This novel mode of action distinguishes GH30 xylanases from the more common xylanase families that cleave MeGX(n) in accessible regions. To help understand this unique biochemical function, we have determined the structure of XynC in its native and ligand-bound forms. XynC structure models derived from diffraction data of XynC crystal soaks with the simple sugar glucuronate (GA) and the tetrameric sugar 4-O-methyl-aldotetrauronate resulted in models containing GA and 4-O-methyl-aldotriuronate, respectively. Each is observed in two locations within XynC surface openings. Ligand coordination occurs within the XynC catalytic substrate binding cleft and on the structurally fused side β-domain, demonstrating a substrate targeting role for this putative carbohydrate binding module. Structural data reveal that GA acts as a primary functional appendage for recognition and hydrolysis of the MeGX(n) polymer by the protein. This work compares the structure of XynC with a previously reported homologous enzyme, XynA, from Erwinia chrysanthemi and analyzes the ligand binding sites. Our results identify the molecular interactions that define the unique function of XynC and homologous GH30 enzymes., (Published by Elsevier Ltd.)

Published

2011

17. Regulatory mechanisms of exoribonuclease PNPase and regulatory small RNA on T3SS of Dickeya dadantii.

Author

Zeng Q, Ibekwe AM, Biddle E, and Yang CH

Subjects

Bacterial Proteins genetics, Dickeya chrysanthemi genetics, Dickeya chrysanthemi metabolism, Dickeya chrysanthemi pathogenicity, Exoribonucleases genetics, RNA, Bacterial genetics, Bacterial Proteins metabolism, Dickeya chrysanthemi enzymology, Exoribonucleases metabolism, Gene Expression Regulation, Bacterial physiology, RNA, Bacterial metabolism

Abstract

The type III secretion system (T3SS) is an essential virulence factor for many bacterial pathogens. Polynucleotide phosphorylase (PNPase) is one of the major exoribonucleases in bacteria and plays important roles in mRNA degradation, tRNA processing, and small RNA (sRNA) turnover. In this study, we showed that PNPase downregulates the transcription of T3SS structural and effector genes of the phytopathogenic bacterium Dickeya dadantii. This negative regulation of T3SS by PNPase occurs by repressing the expression of hrpL, encoding a master regulator of T3SS in D. dadantii. By reducing rpoN mRNA stability, PNPase downregulates the transcription of hrpL, which leads to a reduction in T3SS gene expression. Moreover, we have found that PNPase downregulates T3SS by decreasing hrpL mRNA stability. RsmB, a regulatory sRNA, enhances hrpL mRNA stability in D. dadantii. Our results suggest that PNPase decreases the amount of functional RsmB transcripts that could result in reduction of hrpL mRNA stability. In addition, bistable gene expression (differential expression of a single gene that creates two distinct subpopulations) of hrpA, hrpN, and dspE was observed in D. dadantii under in vitro conditions. Although PNPase regulates the proportion of cells in the high state and the low state of T3SS gene expression, it appears that PNPase is not the key switch that triggers the bistable expression patterns of T3SS genes.

Published

2010

18. Unique features of Erwinia chrysanthemi (Dickeya dadantii) RA3B genes involved in the blue indigoidine production.

Author

Chu MK, Lin LF, Twu CS, Lin RH, Lin YC, Hsu ST, Tzeng KC, and Huang HC

Subjects

Base Sequence, Dickeya chrysanthemi genetics, Molecular Sequence Data, Open Reading Frames, Promoter Regions, Genetic, Protein Binding, Bacterial Proteins genetics, Bacterial Proteins metabolism, Dickeya chrysanthemi metabolism, Gene Expression Regulation, Bacterial, Piperidones metabolism

Abstract

Erwinia chrysanthemi (Ech) RA3B produces a large amount of blue indigoidine. Using Tn5-induced mutagenesis, three indigoidine-deficient mutants were generated. Followed by library screening, a 5.8kb fragment complemented mutants for indigoidine synthesis was cloned. This fragment contains four complete open-reading frames (ORFs), pecS, pecM, idgA, and idgB, and two partial ORFs, argG, and idgC. These genes are nearly identical to those in strain Ech3937. Primer extension assays demonstrated a clear transcriptional start site prior to idgA, while no promoter preceding idgB and idgC was detected, suggesting that idgA, idgB, and idgC are organized as one transcription unit. In contrast, indAB is separated from indC in Ech3937. Interestingly, an ERIC sequence was present between idgB and idgC in place of the promoter region of the homolog indC, which may contribute to the loss of promoter activity in RA3B. Futhermore, idgB mutant displayed much lighter blue color, while indB mutant appeared white on media. Overexpression of pecS in RA3B resulted in significantly reduced indigoidine production and idgC transcript. Moreover, gel shift and luxAB reporter assays revealed that PecS specifically binds to the sequence preceding idgA and inhibits gene expression, which is consistent with the results observed in Ech3937., (Copyright 2009. Published by Elsevier GmbH.)

Published

2010

19. ClpXP protease regulates the type III secretion system of Dickeya dadantii 3937 and is essential for the bacterial virulence.

Author

Li Y, Yamazaki A, Zou L, Biddle E, Zeng Q, Wang Y, Lin H, Wang Q, and Yang CH

Subjects

Bacterial Proteins genetics, Bacterial Proteins metabolism, Brassica microbiology, Dickeya chrysanthemi metabolism, Dickeya chrysanthemi pathogenicity, Endopeptidase Clp genetics, Gene Expression Regulation, Bacterial physiology, Virulence, Dickeya chrysanthemi enzymology, Endopeptidase Clp metabolism

Abstract

The type III secretion system (T3SS) is considered one of the major virulence factors in many bacterial pathogens. This report demonstrates that RssB, ClpXP, and RpoS play a role in T3SS regulation of Dickeya dadantii 3937. ClpP is a serine-type protease which associates with the ClpX chaperone to form a functional Clp proteolytic complex for degradation of proteins. With the assistance of recognition factor RssB, ClpXP degrades the RpoS sigma factor. RpoS positively regulates the expression of the rsmA gene encoding an RNA-binding regulatory protein. By interacting with the hrpL mRNA, RsmA reduces HrpL production and downregulates the T3SS genes in the HrpL regulon. In addition, ClpXP, RssB, and RpoS affect pectinolytic enzyme production in D. dadantii 3937, probably through RsmA. The ClpXP and RssB proteins are essential for bacterial virulence.

Published

2010

20. A 20-residue peptide of the inner membrane protein OutC mediates interaction with two distinct sites of the outer membrane secretin OutD and is essential for the functional type II secretion system in Erwinia chrysanthemi.

Author

Login FH, Fries M, Wang X, Pickersgill RW, and Shevchik VE

Subjects

Amino Acid Substitution, Bacterial Outer Membrane Proteins genetics, Peptides genetics, Peptides metabolism, Protein Interaction Mapping, Protein Transport, Bacterial Outer Membrane Proteins metabolism, Dickeya chrysanthemi metabolism

Abstract

The type II secretion system (T2SS) is widely exploited by proteobacteria to secrete enzymes and toxins involved in bacterial survival and pathogenesis. The outer membrane pore formed by the secretin OutD and the inner membrane protein OutC are two key components of the secretion complex, involved in secretion specificity. Here, we show that the periplasmic regions of OutC and OutD interact directly and map the interaction site of OutC to a 20-residue peptide named OutCsip (secretin interacting peptide, residues 139-158). This peptide interacts in vitro with two distinct sites of the periplasmic region of OutD, one located on the N0 subdomain and another overlapping the N2-N3' subdomains. The two interaction sites of OutD have different modes of binding to OutCsip. A single substitution, V143S, located within OutCsip prevents its interaction with one of the two binding sites of OutD and fully inactivates the T2SS. We show that the N0 subdomain of OutD interacts also with a second binding site within OutC located in the region proximal to the transmembrane segment. We suggest that successive interactions between these distinct regions of OutC and OutD may have functional importance in switching the secretion machine.

Published

2010

21. Catabolism of raffinose, sucrose, and melibiose in Erwinia chrysanthemi 3937.

Author

Hugouvieux-Cotte-Pattat N and Charaoui-Boukerzaza S

Subjects

Bacterial Proteins, Cichorium intybus microbiology, Dickeya chrysanthemi genetics, Dickeya chrysanthemi pathogenicity, Melibiose genetics, Models, Biological, Models, Genetic, Multigene Family genetics, Multigene Family physiology, Raffinose genetics, Dickeya chrysanthemi metabolism, Melibiose metabolism, Raffinose metabolism, Sucrose metabolism

Abstract

Erwinia chrysanthemi (Dickeya dadantii) is a plant pathogenic bacterium that has a large capacity to degrade the plant cell wall polysaccharides. The present study reports the metabolic pathways used by E. chrysanthemi to assimilate the oligosaccharides sucrose and raffinose, which are particularly abundant plant sugars. E. chrysanthemi is able to use sucrose, raffinose, or melibiose as a sole carbon source for growth. The two gene clusters scrKYABR and rafRBA are necessary for their catabolism. The phenotypic analysis of scr and raf mutants revealed cross-links between the assimilation pathways of these oligosaccharides. Sucrose catabolism is mediated by the genes scrKYAB. While the raf cluster is sufficient to catabolize melibiose, it is incomplete for raffinose catabolism, which needs two additional steps that are provided by scrY and scrB. The scr and raf clusters are controlled by specific repressors, ScrR and RafR, respectively. Both clusters are controlled by the global activator of carbohydrate catabolism, the cyclic AMP receptor protein (CRP). E. chrysanthemi growth with lactose is possible only for mutants with a derepressed nonspecific lactose transport system, which was identified as RafB. RafR inactivation allows the bacteria to the assimilate the novel substrates lactose, lactulose, stachyose, and melibionic acid. The raf genes also are involved in the assimilation of alpha- and beta-methyl-D-galactosides. Mutations in the raf or scr genes did not significantly affect E. chrysanthemi virulence. This could be explained by the large variety of carbon sources available in the plant tissue macerated by E. chrysanthemi.

Published

2009

22. Microbial siderophores exert a subtle role in Arabidopsis during infection by manipulating the immune response and the iron status.

Author

Dellagi A, Segond D, Rigault M, Fagard M, Simon C, Saindrenan P, and Expert D

Subjects

Arabidopsis drug effects, Arabidopsis genetics, Arabidopsis Proteins genetics, Arabidopsis Proteins metabolism, Cation Transport Proteins genetics, Cation Transport Proteins metabolism, Dickeya chrysanthemi drug effects, Dickeya chrysanthemi growth & development, Dipeptides pharmacology, Ethylenes metabolism, FMN Reductase genetics, FMN Reductase metabolism, Gene Expression Regulation, Plant drug effects, Genes, Plant, Iron Chelating Agents pharmacology, Models, Biological, Plant Roots drug effects, Plant Roots microbiology, Salicylic Acid metabolism, Signal Transduction drug effects, Signal Transduction genetics, Up-Regulation drug effects, Arabidopsis immunology, Arabidopsis microbiology, Dickeya chrysanthemi metabolism, Immune System Phenomena drug effects, Iron metabolism, Siderophores pharmacology

Abstract

Siderophores (ferric ion chelators) are secreted by organisms in response to iron deficiency. The pathogenic enterobacterium Erwinia chrysanthemi produces two siderophores, achromobactin and chrysobactin (CB), which are required for systemic dissemination in host plants. Previous studies have shown that CB is produced in planta and can trigger the up-regulation of the plant ferritin gene AtFER1. To further investigate the function of CB during pathogenesis, we analyzed its effect in Arabidopsis (Arabidopsis thaliana) plants following leaf infiltration. CB activates the salicylic acid (SA)-mediated signaling pathway, while the CB ferric complex is ineffective, suggesting that the elicitor activity of this siderophore is due to its iron-binding property. We confirmed this hypothesis by testing the effect of siderophores structurally unrelated to CB, including deferrioxamine. There was no activation of SA-dependent defense in plants grown under iron deficiency before CB treatment. Transcriptional analysis of the genes encoding the root ferrous ion transporter and ferric chelate reductase, and determination of the activity of this enzyme in response to CB or deferrioxamine, showed that these compounds induce a leaf-to-root iron deficiency signal. This root response as well as ferritin gene up-regulation in the leaf were not compromised in a SA-deficient mutant line. Using the Arabidopsis-E. chrysanthemi pathosystem, we have shown that CB promotes bacterial growth in planta and can modulate plant defenses through an antagonistic mechanism between SA and jasmonic acid signaling cascades. Collectively, these data reveal a new link between two processes mediated by SA and iron in response to microbial siderophores.

Published

2009

23. High-throughput screening of Erwinia chrysanthemi pectin methylesterase variants using carbohydrate microarrays.

Author

Øbro J, Sørensen I, Derkx P, Madsen CT, Drews M, Willer M, Mikkelsen JD, and Willats WG

Subjects

Data Interpretation, Statistical, Dickeya chrysanthemi genetics, Dickeya chrysanthemi metabolism, Pectins metabolism, Peptide Library, Reproducibility of Results, Sequence Analysis, Protein, Amino Acid Substitution physiology, Carboxylic Ester Hydrolases genetics, Carboxylic Ester Hydrolases metabolism, Dickeya chrysanthemi enzymology, Microarray Analysis methods

Abstract

Pectin methylesterases (PMEs) catalyse the removal of methyl esters from the homogalacturonan (HG) backbone domain of pectin, a ubiquitous polysaccharide in plant cell walls. The degree of methyl esterification (DE) impacts upon the functional properties of HG within cell walls and plants produce numerous PMEs that act upon HG in muro. Many microbial plant pathogens also produce PMEs, the activity of which renders HG more susceptible to cleavage by pectin lyase and polygalacturonase enzymes and hence aids cell wall degradation. We have developed a novel microarray-based approach to investigate the activity of a series of variant enzymes based on the PME from the important pathogen Erwinia chrysanthemi. A library of 99 E. chrysanthemi PME mutants was created in which seven amino acids were altered by various different substitutions. Each mutant PME was incubated with a highly methyl esterified lime pectin substrate and, after digestion the enzyme/substrate mixtures were printed as microarrays. The loss of activity that resulted from certain mutations was detected by probing arrays with a mAb (JIM7) that preferentially binds to HG with a relatively high DE. Active PMEs therefore resulted in diminished JIM7 binding to the lime pectin substrate, whereas inactive PMEs did not. Our findings demonstrate the feasibility of our approach for rapidly testing the effects on PME activity of substituting a wide variety of amino acids at different positions.

Published

2009

24. Ironing out a new siderophore synthesis strategy.

Author

Gulick AM

Subjects

Dickeya chrysanthemi enzymology, Molecular Structure, Siderophores chemistry, Dickeya chrysanthemi metabolism, Siderophores biosynthesis

Published

2009

25. AcsD catalyzes enantioselective citrate desymmetrization in siderophore biosynthesis.

Author

Schmelz S, Kadi N, McMahon SA, Song L, Oves-Costales D, Oke M, Liu H, Johnson KA, Carter LG, Botting CH, White MF, Challis GL, and Naismith JH

Subjects

Bacterial Proteins chemistry, Bacterial Proteins genetics, Base Sequence, Biocatalysis, Chromatography, High Pressure Liquid, Citric Acid chemistry, DNA Primers, Magnetic Resonance Spectroscopy, Models, Molecular, Mutagenesis, Site-Directed, Protein Conformation, Spectrometry, Mass, Electrospray Ionization, Stereoisomerism, Bacterial Proteins metabolism, Citric Acid metabolism, Dickeya chrysanthemi metabolism, Siderophores biosynthesis

Abstract

Bacterial pathogens need to scavenge iron from their host for growth and proliferation during infection. They have evolved several strategies to do this, one being the biosynthesis and excretion of small, high-affinity iron chelators known as siderophores. The biosynthesis of siderophores is an important area of study, not only for potential therapeutic intervention but also to illuminate new enzyme chemistries. Two general pathways for siderophore biosynthesis exist: the well-characterized nonribosomal peptide synthetase (NRPS)-dependent pathway and the NRPS-independent siderophore (NIS) pathway, which relies on a different family of sparsely investigated synthetases. Here we report structural and biochemical studies of AcsD from Pectobacterium (formerly Erwinia) chrysanthemi, an NIS synthetase involved in achromobactin biosynthesis. The structures of ATP and citrate complexes provide a mechanistic rationale for stereospecific formation of an enzyme-bound (3R)-citryladenylate, which reacts with L-serine to form a likely achromobactin precursor. AcsD is a unique acyladenylate-forming enzyme with a new fold and chemical catalysis strategy.

Published

2009

26. Erwinia chrysanthemi iron metabolism: the unexpected implication of the inner membrane platform within the type II secretion system.

Author

Douet V, Expert D, Barras F, and Py B

Subjects

Bacterial Outer Membrane Proteins chemistry, Bacterial Outer Membrane Proteins genetics, Bacterial Outer Membrane Proteins metabolism, Bacterial Proteins chemistry, Bacterial Proteins genetics, Carrier Proteins chemistry, Carrier Proteins genetics, Carrier Proteins metabolism, Chromatography, Affinity, Citrates metabolism, Dickeya chrysanthemi genetics, Dipeptides metabolism, Electrophoresis, Polyacrylamide Gel, Genotype, Ketoglutaric Acids metabolism, Mutation, Oxidative Stress, Phosphate-Binding Proteins, Protein Binding, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Streptonigrin pharmacology, Two-Hybrid System Techniques, Bacterial Proteins metabolism, Dickeya chrysanthemi metabolism, Iron metabolism

Abstract

The type II secretion (T2S) system is an essential device for Erwinia chrysanthemi virulence. Previously, we reported the key role of the OutF protein in forming, along with OutELM, an inner membrane platform in the Out T2S system. Here, we report that OutF copurified with five proteins identified by matrix-assisted laser desorption ionization-time of flight analysis as AcsD, TogA, SecA, Tsp, and DegP. The AcsD protein was known to be involved in the biosynthesis of achromobactin, which is a siderophore important for E. chrysanthemi virulence. The yeast two-hybrid system allowed us to gain further evidence for the OutF-AcsD interaction. Moreover, we showed that lack of OutF produced a pleiotropic phenotype: (i) altered production of the two siderophores of E. chrysanthemi, achromobactin and chrysobactin; (ii) hypersensitivity to streptonigrin, an iron-activated antibiotic; (iii) increased sensitivity to oxidative stress; and (iv) absence of the FbpA-like iron-binding protein in the periplasmic fraction. Interestingly, outE and outL mutants also exhibited similar phenotypes, but, outD and outJ mutants did not. Moreover, using the yeast two-hybrid system, several interactions were shown to occur between components of the T2S system inner membrane platform (OutEFL) and proteins involved in achromobactin production (AcsABCDE). The OutL-AcsD interaction was also demonstrated by Ni(2+) affinity chromatography. These results fully confirm our previous view that the T2S machinery is made up of three discrete blocks. The OutEFLM-forming platform is proposed to be instrumental in two different processes essential for virulence, protein secretion and iron homeostasis.

Published

2009

27. Siderophore-controlled iron assimilation in the enterobacterium Erwinia chrysanthemi: evidence for the involvement of bacterioferritin and the Suf iron-sulfur cluster assembly machinery.

Author

Expert D, Boughammoura A, and Franza T

Subjects

Bacterial Proteins physiology, Biological Transport, Cytochrome b Group physiology, Dipeptides chemistry, Electrophoresis, Polyacrylamide Gel, Ferritins physiology, Iron chemistry, Metalloproteins chemistry, Models, Biological, Mutation, Oxidation-Reduction, Plasmids metabolism, Bacterial Proteins chemistry, Cytochrome b Group chemistry, Dickeya chrysanthemi metabolism, Ferritins chemistry, Gene Expression Regulation, Bacterial, Iron metabolism, Iron-Sulfur Proteins chemistry, Siderophores metabolism

Abstract

The intracellular fate of iron acquired by bacteria during siderophore-mediated assimilation is poorly understood. We investigated this question in the pathogenic enterobacterium Erwinia chrysanthemi. This bacterium produces two siderophores, chrysobactin and achromobactin, during plant infection. We analyzed the distribution of iron into cytosolic proteins in bacterial cells supplied with 59Fe-chrysobactin using native gel electrophoresis. A parental strain and mutants deficient in bacterioferritin (bfr), miniferritin (dps), ferritin (ftnA), bacterioferredoxin (bfd), or iron-sulfur cluster assembly machinery (sufABCDSE) were studied. In the parental strain, we observed two rapidly 59Fe-labeled protein signals identified as bacterioferritin and an iron pool associated to the protein chain-elongation process. In the presence of increased 59Fe-chrysobactin concentrations, we detected mini-ferritin-bound iron. Iron incorporation into bacterioferritin was severely reduced in nonpolar sufA, sufB, sufD, sufS, and sufE mutants but not in a sufC background. Iron recycling from bacterioferritin did not occur in bfd and sufC mutants. Iron depletion caused a loss of aconitase activity, whereas ferric chrysobactin supplementation stimulated the production of active aconitase in parental cells and in bfr and bfd mutants. Aconitase activity in sufA, sufB, sufD, sufS, and sufE mutant strains was 10 times lower than that in parental cells. In the sufC mutant, it was twice as low as that in the parental strain. Defects observed in the mutants were not caused by altered ferric chrysobactin transport. Our data demonstrate a functional link between bacterioferritin, bacterioferredoxin, and the Suf protein machinery resulting in optimal bacterial growth and a balanced distribution of iron between essential metalloproteins.

Published

2008

28. Analysis of the LacI family regulators of Erwinia chrysanthemi 3937, involvement in the bacterial phytopathogenicity.

Author

Van Gijsegem F, Wlodarczyk A, Cornu A, Reverchon S, and Hugouvieux-Cotte-Pattat N

Subjects

Bacterial Proteins metabolism, Bacterial Proteins physiology, Cichorium intybus microbiology, Dickeya chrysanthemi metabolism, Dickeya chrysanthemi pathogenicity, Lac Repressors, Multigene Family genetics, Mutation, Repressor Proteins metabolism, Repressor Proteins physiology, Virulence genetics, Bacterial Proteins genetics, Dickeya chrysanthemi genetics, Repressor Proteins genetics

Abstract

Analysis of the regulators of the LacI family was performed in order to identify those potentially involved in pathogenicity of Erwinia chrysanthemi (Dickeya dadantii). Among the 18 members of the LacI family, the function of 11 members is either known or predicted and only 7 members have, as yet, no proposed function. Inactivation of these seven genes, called lfaR, lfbR, lfcR, lfdR, lfeR, lffR, and lfgR, demonstrated that four of them are important for plant infection. The lfaR and lfcR mutants showed a reduced virulence on chicory, Saintpaulia sp., and Arabidopsis. The lfeR mutant showed a reduced virulence on Arabidopsis. The lfdR mutant was more efficient than the wild-type strain in initiating maceration on Saintpaulia sp. The genetic environment of each regulator was examined to detect adjacent genes potentially involved in a common function. Construction of transcriptional fusions in these neighboring genes demonstrated that five regulators, LfaR, LfcR, LfeR, LffR, and LfgR, act as repressors of adjacent genes. Analysis of these fusions also indicated that the genes controlled by LfaR, LfcR, LfgR, and LffR are expressed during plant infection. Moreover, addition of crude plant extracts to culture medium demonstrated that the expression of the LfaR- and LfgR-controlled genes is specifically induced by plant components.

Published

2008

29. [Separation, characters and biological functions of Erwinia chrysanthemi pv. zeae toxin].

Author

Liu Q, Luo J, He X, and Wang Z

Subjects

1-Butanol chemistry, Bacterial Toxins toxicity, Biological Phenomena, Dickeya chrysanthemi metabolism, Formates chemistry, Methanol chemistry, Plant Diseases microbiology, Bacterial Toxins isolation & purification, Dickeya chrysanthemi chemistry

Abstract

Objective: The toxin produced by Erwinia chrysanthemi pv. zeae has not been reported so far. Toxin is one of the important pathogenic factors for plant pathogenic bacteria. The separation and purification of toxin are the key and basal work for toxin functional study., Methods: We used several chromatography columns, chemical and biochemical methods for Erwinia chrysanthemi pv. zeae toxin separation and its characterization., Results: We obtained a pure ingredient T3 of Erwinia chrysanthemi pv. zeae toxin . It was a yellow solid and dissolved in methanol, N-butyl alcohol(NBA), water and formic acid. It dissolved weakly in acetone but did not dissolve in trichloromethane and ethyl acetate. The results showed that T3 toxin ingredient was neither carbohydrate nor protein, and was sensitive to ultraviolet ray. Biological assays of the toxin showed that it could inhibit rice growth, cause rice seedlings to wilt and make tobacco cells necrosis. Toxin with high content could inhibit buds and roots of rice, corn, tomato and tobacco to grow, whereas toxin with low content could promote their growth. In addition, the toxin inhibited 10 plant pathogenic bacteria with 5 genera. Furthermore, toxin T3 induced the activities of phenylalanine ammonia-lysae(PAL) and peroxidase(POD) in rice., Conclusions: It is the first report about the separation and purification of E. chrysanthemi pv.zeae toxin. The T3 toxin of E. chrysanthemi pv.zeae had the biological characters with inhibiting plant seeds germination, causing rice seedlings wilt, inhibiting some plant pathogenic bacteria and inducing defense enzyme activities in rice.

Published

2008

30. PecS is a global regulator of the symptomatic phase in the phytopathogenic bacterium Erwinia chrysanthemi 3937.

Author

Hommais F, Oger-Desfeux C, Van Gijsegem F, Castang S, Ligori S, Expert D, Nasser W, and Reverchon S

Subjects

Bacterial Proteins genetics, Bacterial Proteins metabolism, DNA Footprinting, Dickeya chrysanthemi genetics, Dickeya chrysanthemi metabolism, Electrophoretic Mobility Shift Assay, Gene Expression Regulation, Bacterial, Host-Pathogen Interactions, Mutation, Oligonucleotide Array Sequence Analysis, Oxidative Stress, Promoter Regions, Genetic genetics, Protein Binding, Repressor Proteins genetics, Repressor Proteins metabolism, Reverse Transcriptase Polymerase Chain Reaction, Sequence Analysis, DNA, Bacterial Proteins physiology, Dickeya chrysanthemi physiology, Magnoliopsida microbiology, Repressor Proteins physiology

Abstract

Pathogenicity of the enterobacterium Erwinia chrysanthemi (Dickeya dadantii), the causative agent of soft-rot disease in many plants, is a complex process involving several factors whose production is subject to temporal regulation during infection. PecS is a transcriptional regulator that controls production of various virulence factors. Here, we used microarray analysis to define the PecS regulon and demonstrated that PecS notably regulates a wide range of genes that could be linked to pathogenicity and to a group of genes concerned with evading host defenses. Among the targets are the genes encoding plant cell wall-degrading enzymes and secretion systems and the genes involved in flagellar biosynthesis, biosurfactant production, and the oxidative stress response, as well as genes encoding toxin-like factors such as NipE and hemolysin-coregulated proteins. In vitro experiments demonstrated that PecS interacts with the regulatory regions of five new targets: an oxidative stress response gene (ahpC), a biosurfactant synthesis gene (rhlA), and genes encoding exported proteins related to other plant-associated bacterial proteins (nipE, virK, and avrL). The pecS mutant provokes symptoms more rapidly and with more efficiency than the wild-type strain, indicating that PecS plays a critical role in the switch from the asymptomatic phase to the symptomatic phase. Based on this, we propose that the temporal regulation of the different groups of genes required for the asymptomatic phase and the symptomatic phase is, in part, the result of a gradual modulation of PecS activity triggered during infection in response to changes in environmental conditions emerging from the interaction between both partners.

Published

2008

31. Iron(III) uptake and release by chrysobactin, a siderophore of the phytophatogenic bacterium Erwinia chrysanthemi.

Author

Tomisić V, Blanc S, Elhabiri M, Expert D, and Albrecht-Gary AM

Subjects

Ferric Compounds chemistry, Kinetics, Ligands, Potentiometry, Protein Binding, Spectrophotometry, Dickeya chrysanthemi metabolism, Dipeptides metabolism, Iron metabolism, Siderophores metabolism

Abstract

The plant pathogenic enterobacterium Erwinia chrysanthemi causes important soft-rot disease on a wide range of plants including vegetables and ornamentals of economic importance. It produces a major mono(catecholate) siderophore, chrysobactin (alpha-N-(2,3-dihydroxybenzoyl)-D-lysyl-L-serine). To unravel the role of chrysobactin in the virulence of E. chrysanthemi, its iron(III) coordination properties were thus investigated in aqueous solutions using electrospray ionization mass spectrometric, potentiometric, and spectrophotometric methods. Moreover, kinetic experiments allowed us to determine the uptake and release mechanisms. The formation mechanism of the 1:1 complex reveals a key role of the terminal carboxylic group of chrysobactin in the binding of either FeOH(2+) or Fe2(OH)2(4+). The proton-driven dissociation of the ferric tris-, bis-, and mono(chrysobactin) complexes was also studied. For these three ferric complexes, a single protonation triggers the release of the bound chrysobactin molecule. Interestingly, the dissociation of the last ligand proceeded via the formation of an intermediate for which a salicylate-type mode of bonding was proposed.

Published

2008

32. The crystal structure of pectate lyase peli from soft rot pathogen Erwinia chrysanthemi in complex with its substrate.

Author

Creze C, Castang S, Derivery E, Haser R, Hugouvieux-Cotte-Pattat N, Shevchik VE, and Gouet P

Subjects

Amino Acid Sequence, Arginine chemistry, Binding Sites, Catalysis, Catalytic Domain, Kinetics, Lysine chemistry, Models, Molecular, Molecular Sequence Data, Protein Folding, Protein Structure, Tertiary, Crystallography, X-Ray methods, Dickeya chrysanthemi metabolism, Gene Expression Regulation, Polysaccharide-Lyases chemistry

Abstract

The crystallographic structure of the family 3 polysaccharide lyase (PL-3) PelI from Erwinia chrysanthemi has been solved to 1.45 A resolution. It consists of an N-terminal domain harboring a fibronectin type III fold linked to a catalytic domain displaying a parallel beta-helix topology. The N-terminal domain is located away from the active site and is not involved in the catalytic process. After secretion in planta, the two domains are separated by E. chrysanthemi proteases. This event turns on the hypersensitive response of the host. The structure of the single catalytic domain determined to 2.1 A resolution shows that the domain separation unveils a "Velcro"-like motif of asparagines, which might be recognized by a plant receptor. The structure of PelI in complex with its substrate, a tetragalacturonate, has been solved to 2.3 A resolution. The sugar binds from subsites -2 to +2 in one monomer of the asymmetric unit, although it lies on subsites -1 to +3 in the other. These two "Michaelis complexes" have never been observed simultaneously before and are consistent with the dual mode of bond cleavage in this substrate. The bound sugar adopts a mixed 2(1) and 3(1) helical conformation similar to that reported in inactive mutants from families PL-1 and PL-10. However, our study suggests that the catalytic base in PelI is not a conventional arginine but a lysine as proposed in family PL-9.

Published

2008

33. A pentameric, ligand-gated ion channel from a bacterium.

Author

Braun AP

Subjects

Bacterial Physiological Phenomena, Binding Sites, Crystallography, X-Ray methods, Cysteine chemistry, Dickeya chrysanthemi metabolism, Ion Channel Gating, Ligands, Protein Structure, Tertiary, Receptors, Nicotinic metabolism, Bacteria metabolism, Ion Channels chemistry

Published

2008

34. [Genetic and molecular characters of toxin producing Erwinia chrysanthemi pv. zeae].

Author

Liu Q, Zhang J, Wang Y, and Wang Z

Subjects

Cell Death, DNA Mutational Analysis, Genetic Markers genetics, Mutation, Open Reading Frames, Oryza microbiology, Plasmids genetics, Seedlings microbiology, Nicotiana microbiology, Bacterial Toxins biosynthesis, Dickeya chrysanthemi genetics, Dickeya chrysanthemi metabolism

Abstract

Objective: Bacterial foot rot, caused by Erwinia chrysanthemi pv. zeae, is one of the most important diseases in rice. Genetic and molecular characters of toxin producting for Erwinia chrysanthemi pv. zeae were conducted in this paper., Methods: A plasmid-deficient strain, Ech7-mul, was obtained by chemical mutation,and the relative specific molecular mark with toxin was screened from Random Amplified Polymorphic DNA (RAPD) by PCR., Results: The wild strain Ech7 and the plasmid-deficient strain Ech7-mul could both produce toxin.We screened 260 random primers in PCR, and found that a specific fragment (2139bp) could be amplified with K10 primer from theminus-toxin strain Ech7-4 DNA, but could not from the wild strain Ech7 DNA. The amplified fragment DNA was cloned and sequenced, and specific primers were designed to amplify it. The 2139bp fragment DNA could be a specific molecular mark with 100% SCAR identity between wild strain and the toxin mutant strain. Sequence analysis showed that there were five open reading frame (ORF), two of them were NADH-flavin reductase and N-acetyltransferase,respectively. Another ORF, located in the end region of 2139bp fragment, had 66% and 46% homologies with permeases of the drug/metabolite transporter (DMT) from Pseudomonas aerginosa (ZP00136947) and Yersinia Pestis (ZP01177873)., Conclusion: Toxin biosynthesis in E. chrysanthemi pv. zeae might be coded by chromosome, but not by the bacterial plasmid.The position of gene mutation in the mutant Ech7-4 might be at the 3' region of toxin-relation SCAR DNA fragment.

Published

2008

35. Biogenesis of Fe/S proteins and pathogenicity: IscR plays a key role in allowing Erwinia chrysanthemi to adapt to hostile conditions.

Author

Rincon-Enriquez G, Crété P, Barras F, and Py B

Subjects

Adaptation, Physiological genetics, Arabidopsis microbiology, Bacterial Proteins genetics, Carbon-Sulfur Lyases genetics, Carbon-Sulfur Lyases metabolism, Cichorium intybus microbiology, Chromosomes, Bacterial genetics, Dickeya chrysanthemi genetics, Dickeya chrysanthemi pathogenicity, Gene Expression Regulation, Bacterial drug effects, Genome, Bacterial, Iron-Sulfur Proteins genetics, Models, Genetic, Mutation, Operon genetics, Paraquat pharmacology, Phenotype, Plant Leaves microbiology, Virulence genetics, Adaptation, Physiological physiology, Bacterial Proteins metabolism, Dickeya chrysanthemi metabolism, Iron-Sulfur Proteins metabolism

Abstract

The Erwinia chrysanthemi genome is predicted to encode three systems, Nif, Isc and Suf, known to assist Fe/S cluster biogenesis and the CsdAE cysteine desulphurase. Single iscU, hscA and fdx mutants were found sensitive to paraquat and exhibited reduced virulence on both chicory leaves and Arabidopsis thaliana. Depletion of the whole Isc system led to a pleiotropic phenotype, including sensitivity to both paraquat and 2,2'-dipyridyl, auxotrophies for branched-chain amino acids, thiamine, nicotinic acid, and drastic alteration in virulence. IscR was able to suppress all of the phenotypes listed above in a sufC-dependent manner while depletion of the Isc system led to IscR-dependent activation of the suf operon. No virulence defects were found associated with csdA or nifS mutations. Surprisingly, we found that the sufC mutant was virulent against A. thaliana, whereas its virulence had been found altered in Saintpaulia. Collectively, these results lead us to propose that E. chrysanthemi possess the Fe/S biogenesis strategy suited to the physico-chemical conditions encountered in its host upon infection. In this view, the IscR regulator, which controls both Isc and Suf, is predicted to play a major role in the ability of E. chrysanthemi to colonize a wide array of different plants.

Published

2008

36. Differential role of ferritins in iron metabolism and virulence of the plant-pathogenic bacterium Erwinia chrysanthemi 3937.

Author

Boughammoura A, Matzanke BF, Böttger L, Reverchon S, Lesuisse E, Expert D, and Franza T

Subjects

Bacterial Proteins metabolism, Bacterial Proteins physiology, Base Sequence, Biological Transport, Blotting, Northern, Cichorium intybus microbiology, Chlorides, Cytochrome b Group metabolism, Cytochrome b Group physiology, Dickeya chrysanthemi metabolism, Dickeya chrysanthemi pathogenicity, Ferric Compounds metabolism, Ferritins metabolism, Ferritins physiology, Ferrous Compounds metabolism, Gene Expression Regulation, Bacterial, Iron Radioisotopes metabolism, Molecular Sequence Data, Mutation, Oxidative Stress, Plant Leaves microbiology, Spectroscopy, Mossbauer, Virulence genetics, Bacterial Proteins genetics, Cytochrome b Group genetics, Dickeya chrysanthemi genetics, Ferritins genetics, Iron metabolism

Abstract

During infection, the phytopathogenic enterobacterium Erwinia chrysanthemi has to cope with iron-limiting conditions and the production of reactive oxygen species by plant cells. Previous studies have shown that a tight control of the bacterial intracellular iron content is necessary for full virulence. The E. chrysanthemi genome possesses two loci that could be devoted to iron storage: the bfr gene, encoding a heme-containing bacterioferritin, and the ftnA gene, coding for a paradigmatic ferritin. To assess the role of these proteins in the physiology of this pathogen, we constructed ferritin-deficient mutants by reverse genetics. Unlike the bfr mutant, the ftnA mutant had increased sensitivity to iron deficiency and to redox stress conditions. Interestingly, the bfr ftnA mutant displayed an intermediate phenotype for sensitivity to these stresses. Whole-cell analysis by Mössbauer spectroscopy showed that the main iron storage protein is FtnA and that there is an increase in the ferrous iron/ferric iron ratio in the ftnA and bfr ftnA mutants. We found that ftnA gene expression is positively controlled by iron and the transcriptional repressor Fur via the small antisense RNA RyhB. bfr gene expression is induced at the stationary phase of growth. The sigmaS transcriptional factor is necessary for this control. Pathogenicity tests showed that FtnA and the Bfr contribute differentially to the virulence of E. chrysanthemi depending on the host, indicating the importance of a perfect control of iron homeostasis in this bacterial species during infection.

Published

2008

37. The acyl-homoserine lactone-type quorum-sensing system modulates cell motility and virulence of Erwinia chrysanthemi pv. zeae.

Author

Hussain MB, Zhang HB, Xu JL, Liu Q, Jiang Z, and Zhang LH

Subjects

Amino Acid Sequence, Bacterial Adhesion, Bacterial Proteins genetics, Base Sequence, Cell Movement, Dickeya chrysanthemi genetics, Dickeya chrysanthemi metabolism, Molecular Sequence Data, Oryza microbiology, Seeds microbiology, Sequence Analysis, DNA, Solanum tuberosum microbiology, Trans-Activators genetics, Trans-Activators metabolism, Virulence, Acyl-Butyrolactones metabolism, Bacterial Proteins metabolism, Dickeya chrysanthemi pathogenicity, Dickeya chrysanthemi physiology, Gene Expression Regulation, Bacterial, Quorum Sensing

Abstract

Erwinia chrysanthemi pv. zeae is one of the Erwinia chrysanthemi pathovars that infects on both dicotyledons and monocotyledons. However, little is known about the molecular basis and regulatory mechanisms of its virulence. By using a transposon mutagenesis approach, we cloned the genes coding for an E. chrysanthemi pv. zeae synthase of acyl-homoserine lactone (AHL) quorum-sensing signals (expI(Ecz)) and a cognate response regulator (expR(Ecz)). Chromatography analysis showed that expI(Ecz) encoded production of the AHL signal N-(3-oxo-hexanoyl)-homoserine lactone (OHHL). Null mutation of expI(Ecz) in the E. chrysanthemi pv. zeae strain EC1 abolished AHL production, increased bacterial swimming and swarming motility, disabled formation of multicell aggregates, and attenuated virulence of the pathogen on potato tubers. The mutation also marginally reduced the inhibitory activity of E. chrysanthemi pv. zeae on rice seed germination. The mutant phenotypes were rescued by either exogenous addition of AHL signal or in trans expression of expI(Ecz). These data demonstrate that the AHL-type QS signal plays an essential role in modulation of E. chrysanthemi pv. zeae cell motility and the ability to form multicell aggregates and is involved in regulation of bacterial virulence.

Published

2008

38. The DNA nucleoid-associated protein Fis co-ordinates the expression of the main virulence genes in the phytopathogenic bacterium Erwinia chrysanthemi.

Author

Lautier T and Nasser W

Subjects

Bacterial Proteins genetics, Base Sequence, Dickeya chrysanthemi genetics, Dickeya chrysanthemi pathogenicity, Gene Expression Regulation, Bacterial, Membrane Glycoproteins genetics, Membrane Glycoproteins metabolism, Molecular Sequence Data, Mutation, Phenotype, Polymerase Chain Reaction, Polysaccharide-Lyases genetics, Polysaccharide-Lyases metabolism, Promoter Regions, Genetic genetics, Transcription, Genetic, Virulence genetics, Bacterial Proteins metabolism, DNA, Bacterial metabolism, Dickeya chrysanthemi metabolism

Abstract

Erwinia chrysanthemi strain 3937 is a necrotrophic bacterial plant pathogen. Pectinolytic enzymes and, in particular, pectate lyases (Pels) play a key role in soft rot symptoms but the efficient colonization of plants by E. chrysanthemi requires additional factors. These factors include the harpin HrpN, the cellulase Cel5, proteases (Prts), flagellar proteins and the Sap system, involved in the detoxification of plant antimicrobial peptides. HrpN and flagellum are mostly involved in the early steps of infection whereas the degradative enzymes (Pels, Cel5, Prts) are mainly required in the advanced stages. Production of these virulence factors is tightly regulated by environmental conditions. This report shows that the nucleoid-associated protein Fis plays a pivotal role in the expression of the main virulence genes. Its production is regulated in a growth phase-dependent manner and is under negative autoregulation. An E. chrysanthemi fis mutant displays a reduced motility and expression of hrpN, prtC and the sap operon. In contrast, the expression of the cel5 gene is increased in this mutant. Furthermore, the induction of the Pel activity is delayed and increased during the stationary growth phase in the fis mutant. Most of these controls occur through a direct effect because purified Fis binds to the promoter regions of fis, hrpN, sapA, cel5 and fliC. Moreover, potassium permanganate footprinting and in vitro transcription assays have revealed that Fis prevents transcription initiation at the fis promoter and also transcript elongation from the cel5 promoter. Finally, the fis mutant has a decreased virulence. These results suggest a co-ordinated regulation by Fis of virulence factors involved in certain key steps of infection, early (asymptomatic) and advanced (symptomatic) phases.

Published

2007

39. Integration of two essential virulence modulating signals at the Erwinia chrysanthemi pel gene promoters: a role for Fis in the growth-phase regulation.

Author

Lautier T, Blot N, Muskhelishvili G, and Nasser W

Subjects

Base Sequence, DNA metabolism, Dickeya chrysanthemi metabolism, Dickeya chrysanthemi pathogenicity, Electrophoretic Mobility Shift Assay, Molecular Sequence Data, Operator Regions, Genetic genetics, Polymerase Chain Reaction, Protein Binding, Repressor Proteins genetics, Transcription Factors genetics, Transcription, Genetic, Virulence genetics, Bacterial Proteins genetics, Dickeya chrysanthemi genetics, Polysaccharide-Lyases genetics, Promoter Regions, Genetic genetics

Abstract

Production of the essential virulence factors, called pectate lyases (Pels), in the phytopathogenic bacterium Erwinia chrysanthemi is controlled by a complex regulation system and responds to various stimuli, such as the presence of pectin or plant extracts, growth phase, temperature and iron concentration. The presence of pectin and growth phase are the most important signals identified. Eight regulators modulating the expression of the pel genes (encoding Pels) have been characterized. These regulators are organized in a network allowing a sequential functioning of the regulators during infection. Although many studies have been carried out, the mechanisms of control of Pel production by growth phase have not yet been elucidated. Here we report that a fis mutant of E. chrysanthemi showed a strong increase in transcription of the pel genes during exponential growth whereas induction of expression in the parental strain occurred at the end of exponential growth. This reveals that Fis acts to prevent an efficient transcription of pel genes at the beginning of exponential growth and also provides evidence of the involvement of Fis in the growth-phase regulation of the pel genes. By using in vitro DNA-protein interactions and transcription experiments, we find that Fis directly represses the pel gene expression at the transcription initiation step. In addition, we show that Fis acts in concert with KdgR, the main repressor responding to the presence of pectin compounds, to shut down the pel gene transcription. Finally, we find that active Fis is required for the efficient translocation of the Pels in growth medium. Together, these data indicate that Fis tightly controls the availability of Pels during pathogenesis by acting on both their production and their translocation in the external medium.

Published

2007

40. Characterization of the Erwinia chrysanthemi Gan locus, involved in galactan catabolism.

Author

Delangle A, Prouvost AF, Cogez V, Bohin JP, Lacroix JM, and Cotte-Pattat NH

Subjects

ATP-Binding Cassette Transporters genetics, ATP-Binding Cassette Transporters metabolism, Bacterial Proteins chemistry, Bacterial Proteins genetics, Bacterial Proteins metabolism, Cichorium intybus microbiology, Electrophoresis, Polyacrylamide Gel, Gene Expression Regulation, Bacterial drug effects, Genes, Bacterial, Genome, Bacterial, Glucose pharmacology, Multigene Family, Mutation, Protons, Solanum tuberosum microbiology, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Sucrose pharmacology, Temperature, Dickeya chrysanthemi genetics, Dickeya chrysanthemi metabolism, Galactans metabolism

Abstract

beta-1,4-Galactan is a major component of the ramified regions of pectin. Analysis of the genome of the plant pathogenic bacteria Erwinia chrysanthemi revealed the presence of a cluster of eight genes encoding proteins potentially involved in galactan utilization. The predicted transport system would comprise a specific porin GanL and an ABC transporter made of four proteins, GanFGK(2). Degradation of galactans would be catalyzed by the periplasmic 1,4-beta-endogalactanase GanA, which released oligogalactans from trimer to hexamer. After their transport through the inner membrane, oligogalactans would be degraded into galactose by the cytoplasmic 1,4-beta-exogalactanase GanB. Mutants affected for the porin or endogalactanase were unable to grow on galactans, but they grew on galactose and on a mixture of galactotriose, galactotetraose, galactopentaose, and galactohexaose. Mutants affected for the periplasmic galactan binding protein, the transporter ATPase, or the exogalactanase were only able to grow on galactose. Thus, the phenotypes of these mutants confirmed the functionality of the gan locus in transport and catabolism of galactans. These mutations did not affect the virulence of E. chrysanthemi on chicory leaves, potato tubers, or Saintpaulia ionantha, suggesting an accessory role of galactan utilization in the bacterial pathogeny.

Published

2007

41. Differential regulation of two oligogalacturonate outer membrane channels, KdgN and KdgM, of Dickeya dadantii (Erwinia chrysanthemi).

Author

Condemine G and Ghazi A

Subjects

Bacterial Outer Membrane Proteins genetics, Dickeya chrysanthemi genetics, Multigene Family, Bacterial Outer Membrane Proteins physiology, Dickeya chrysanthemi metabolism, Gene Expression Regulation, Bacterial physiology, Porins physiology

Abstract

The entry of oligogalacturonates into Dickeya dadantii occurs through the specific channel KdgM. The genome of the bacterium encodes a second member of this family of outer membrane proteins, KdgN. We showed that this protein is also involved in the uptake of oligogalacturonates. When KdgN was reconstituted in proteoliposomes, it formed channels with a conductance of about 450 pS at a positive potential. These channels had weak anionic selectivity. The regulation of kdgN is complex, and five genes controlling the expression of kdgN have been identified: kdgR, pecS, ompR, hns, and crp. Moreover, kdgN was regulated by growth phase but only when bacteria were grown in rich medium. Most of these regulators of kdgN also control kdgM expression, but some of them regulate kdgM in the opposite manner: while PecS and OmpR are repressors of kdgM, they are activators of kdgN. This pattern resembles the regulation of the Escherichia coli general porins OmpF and OmpC, but such opposite regulation of two specific outer membrane channels has never been described before. KdgN may allow the bacteria to collect oligogalacturonates under saprophytic conditions, when virulence genes, including kdgM, are not expressed.

Published

2007

42. Proteomic analysis of a non-virulent mutant of the phytopathogenic bacterium Erwinia chrysanthemi deficient in osmoregulated periplasmic glucans: change in protein expression is not restricted to the envelope, but affects general metabolism.

Author

Bouchart F, Delangle A, Lemoine J, Bohin JP, and Lacroix JM

Subjects

Bacterial Proteins isolation & purification, Dickeya chrysanthemi genetics, Dickeya chrysanthemi metabolism, Dickeya chrysanthemi pathogenicity, Electrophoresis, Gel, Two-Dimensional, Gene Expression Regulation, Bacterial, Glucans genetics, Mass Spectrometry, Metabolic Networks and Pathways, Molecular Chaperones biosynthesis, Peptide Hydrolases biosynthesis, Proteome isolation & purification, Proteomics, Virulence genetics, Bacterial Proteins analysis, Dickeya chrysanthemi chemistry, Glucans biosynthesis, Mutation, Proteome analysis

Abstract

Osmoregulated periplasmic glucans (OPGs) are general constituents of the envelope of Gram-negative bacteria. They are required for full virulence of bacterial phytopathogens such as Pseudomonas syringae, Xanthomonas campestris and Erwinia chrysanthemi. E. chrysanthemi is a pectinolytic gamma-proteobacterium that causes soft rot disease on a wide range of plant species. In addition to the loss of virulence, opg mutants exhibit a pleiotropic phenotype that affects motility, bile-salt resistance, exoenzyme secretion, exopolysaccharide synthesis and membrane lipid composition. This is believed to be the first proteomic analysis of an OPG-defective mutant of E. chrysanthemi and it revealed that, in addition to the effects described, catabolic enzyme synthesis was enhanced and there was a greater abundance of some proteins catalysing the folding and degradation of proteins needed for various stress responses. Thus, in the opg mutant strain, loss of virulence was the result of a combination of envelope structure changes and cellular metabolism modifications.

Published

2007

43. Efflux pump gene expression in Erwinia chrysanthemi is induced by exposure to phenolic acids.

Author

Ravirala RS, Barabote RD, Wheeler DM, Reverchon S, Tatum O, Malouf J, Liu H, Pritchard L, Hedley PE, Birch PR, Toth IK, Payton P, and San Francisco MJ

Subjects

Bacterial Proteins metabolism, Benzoic Acid pharmacology, Biological Transport drug effects, Cichorium intybus microbiology, Cinnamates pharmacology, Dickeya chrysanthemi growth & development, Dickeya chrysanthemi metabolism, Drug Resistance, Microbial genetics, Drug Resistance, Multiple genetics, Gene Expression Regulation, Bacterial drug effects, Immunoblotting, Membrane Proteins genetics, Membrane Proteins metabolism, Oligonucleotide Array Sequence Analysis, Plant Leaves microbiology, Reverse Transcriptase Polymerase Chain Reaction, Salicylic Acid pharmacology, Bacterial Proteins genetics, Dickeya chrysanthemi genetics, Genes, Bacterial

Abstract

Salicylic acid (SA) is an important signaling molecule in local and systemic plant resistance. Following infection by microbial pathogens and the initial oxidative burst in plants, SA accumulation functions in the amplification of defense gene expression. Production of pathogenesis-related proteins and toxic antimicrobial chemicals serves to protect the plant from infection. Successful microbial pathogens utilize a variety of mechanisms to rid themselves of toxic antimicrobial compounds. Important among these mechanisms are multidrug-resistance pumps that bring about the active efflux of toxic compounds from microbial cells. Here, we show that a combination SA and its precursors, t-cinnamic acid and benzoic acid, can activate expression of specific multidrug efflux pump-encoding genes in the plant pathogen Erwinia chrysanthemi and enhance survival of the bacterium in the presence of model as well as plant-derived antimicrobial chemicals. This ability of plant-pathogenic bacteria to co-opt plant defense-signaling molecules to activate multidrug efflux pumps may have evolved to ensure bacterial survival in susceptible host plants.

Published

2007

44. Global effect of indole-3-acetic acid biosynthesis on multiple virulence factors of Erwinia chrysanthemi 3937.

Author

Yang S, Zhang Q, Guo J, Charkowski AO, Glick BR, Ibekwe AM, Cooksey DA, and Yang CH

Subjects

Bacterial Proteins metabolism, Dickeya chrysanthemi enzymology, Molecular Sequence Data, Polysaccharide-Lyases metabolism, Dickeya chrysanthemi metabolism, Gene Expression Regulation, Bacterial physiology, Indoleacetic Acids metabolism, Virulence Factors biosynthesis

Abstract

Production of the plant hormone indole-3-acetic acid (IAA) is widespread among plant-associated microorganisms. The non-gall-forming phytopathogen Erwinia chrysanthemi 3937 (strain Ech3937) possesses iaaM (ASAP16562) and iaaH (ASAP16563) gene homologues. In this work, the null knockout iaaM mutant strain Ech138 was constructed. The IAA production by Ech138 was reduced in M9 minimal medium supplemented with l-tryptophan. Compared with wild-type Ech3937, Ech138 exhibited reduced ability to produce local maceration, but its multiplication in Saintpaulia ionantha was unaffected. The pectate lyase production of Ech138 was diminished. Compared with wild-type Ech3937, the expression levels of an oligogalacturonate lyase gene, ogl, and three endopectate lyase genes, pelD, pelI, and pelL, were reduced in Ech138 as determined by a green fluorescent protein-based fluorescence-activated cell sorting promoter activity assay. In addition, the transcription of type III secretion system (T3SS) genes, dspE (a putative T3SS effector) and hrpN (T3SS harpin), was found to be diminished in the iaaM mutant Ech138. Compared with Ech3937, reduced expression of hrpL (a T3SS alternative sigma factor) and gacA but increased expression of rsmA in Ech138 was also observed, suggesting that the regulation of T3SS and pectate lyase genes by IAA biosynthesis might be partially due to the posttranscriptional regulation of the Gac-Rsm regulatory pathway.

Published

2007

45. Proteomic analysis of the carbonate insoluble outer membrane fraction of the soft-rot pathogen Dickeya dadantii (syn. Erwinia chrysanthemi) strain 3937.

Author

Babujee L, Venkatesh B, Yamazaki A, and Tsuyumu S

Subjects

Electrophoresis, Gel, Two-Dimensional, Glycoproteins chemistry, Hydrogen-Ion Concentration, Lipoproteins chemistry, Phosphorylation, Protein Processing, Post-Translational, Proteome, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Virulence, Bacterial Outer Membrane Proteins metabolism, Carbonates chemistry, Computational Biology methods, Dickeya chrysanthemi metabolism, Plants microbiology, Proteomics methods

Abstract

We present results of the first comprehensive proteomic analysis of the outer membrane of the bacterial phytopathogen Dickeya dadantii strain 3937 and its response to virulence-contributing factors such as host plant extract, acidic stress, and iron starvation. We analyzed the carbonate-insoluble membrane fractions, which are highly enriched for outer membrane proteins, using two-dimensional electrophoresis and identified the proteins by MALDI-TOF MS. Forty unique proteins were identified, some of which were differentially expressed under the above conditions.

Published

2007

46. The single transmembrane segment drives self-assembly of OutC and the formation of a functional type II secretion system in Erwinia chrysanthemi.

Author

Login FH and Shevchik VE

Subjects

Amino Acid Sequence, Bacterial Outer Membrane Proteins chemistry, Bacterial Outer Membrane Proteins genetics, Cross-Linking Reagents chemistry, Cysteine metabolism, Dickeya chrysanthemi chemistry, Dickeya chrysanthemi genetics, Dimerization, Disulfides metabolism, Molecular Sequence Data, Oxidation-Reduction, Peptide Hydrolases metabolism, Substrate Specificity, Two-Hybrid System Techniques, Bacterial Outer Membrane Proteins metabolism, Cell Membrane metabolism, Dickeya chrysanthemi metabolism

Abstract

Many pathogenic Gram-negative bacteria secrete toxins and lytic enzymes via a multiprotein complex called the type II secretion system. This system, named Out in Erwinia chrysanthemi, consists of 14 proteins integrated or associated with the two bacterial membranes. OutC, a key player in this process, is probably implicated in the recognition of secreted proteins and signal transduction. OutC possesses a short cytoplasmic sequence, a single transmembrane segment (TMS), and a large periplasmic region carrying a putative PDZ domain. A hydrodynamic study revealed that OutC forms stable dimers of an elongated shape, whereas the PDZ domain adopts a globular shape. Bacterial two-hybrid, cross-linking, and pulldown assays revealed that the self-association of OutC is driven by the TMS, whereas the periplasmic region is dispensable for self-association. Site-directed mutagenesis of the TMS revealed that cooperative interactions between three polar residues located at the same helical face provide adequate stability for OutC self-assembly. An interhelical H-bonding mediated by Gln(29) appears to be the main driving force, and two Arg residues located at the TMS boundaries are essential for the stabilization of OutC oligomers. Stepwise mutagenesis of these residues gradually diminished OutC functionality and self-association ability. The triple OutC mutant R15V/Q29L/R36A became monomeric and nonfunctional. Self-association and functionality of the triple mutant were partially restored by the introduction of a polar residue at an alternative position in the interhelical interface. Thus, the OutC TMS is more than just a membrane anchor; it drives the protein self-association that is essential for formation of a functional secretion system.

Published

2006

47. Direct evidence for the modulation of the activity of the Erwinia chrysanthemi quorum-sensing regulator ExpR by acylhomoserine lactone pheromone.

Author

Castang S, Reverchon S, Gouet P, and Nasser W

Subjects

4-Butyrolactone physiology, Amino Acid Sequence, Bacterial Proteins genetics, Base Sequence, Dickeya chrysanthemi genetics, Molecular Sequence Data, Trans-Activators genetics, 4-Butyrolactone analogs & derivatives, Bacterial Proteins metabolism, Dickeya chrysanthemi metabolism, Pheromones physiology, Trans-Activators metabolism

Abstract

In Erwinia chrysanthemi production of pectic enzymes is controlled by a complex network involving several regulators. Among them is ExpR, the quorum-sensing regulatory protein. ExpR is a member of the LuxR family of transcriptional regulators, the activity of which is modulated by the binding of diffusible N-acylhomoserine lactone pheromones to the N-terminal receptor site of the proteins. Previous in vitro DNA-ExpR binding studies suggested that ExpR might activate pectic enzyme production and repress its cognate gene expression. This report presents genetic evidence that ExpR represses its own gene expression in the absence of pheromone and that the addition of pheromone promotes concentration-dependent de-repression. In vitro experiments show that (i) ExpR binds target DNA in the absence of pheromone and that the pheromone dissociates ExpR-DNA complexes, (ii) ExpR binds target DNA in a non-cooperative fashion, and (iii) two molecules of pheromone are bound per molecule of ExpR dimer. In the absence of N-(3-oxo-hexanoyl)-homoserine lactone, ExpR prevents RNA polymerase access to the expR promoter, thereby directly repressing transcription initiation. The presence of pheromone renders the expR promoter accessible to RNA polymerase and results in the de-repression of transcription initiation. Overall we have established that there is a direct modulation of the repressive activity of a LuxR family regulator by a pheromone. Furthermore, site-directed mutagenesis experiments strongly suggest that the ExpR residues Leu-19, Tyr-31, and Ser-125 are involved in the transduction of conformational changes induced by ligand binding, and this provides new insights into the structure-function relationship of this bacterial regulator family.

Published

2006

48. Regulation of virulence by members of the MarR/SlyA family.

Author

Ellison DW and Miller VL

Subjects

Amino Acid Sequence, Bacterial Proteins chemistry, Bacterial Proteins metabolism, Cyclic AMP Receptor Protein metabolism, DNA-Binding Proteins metabolism, DNA-Directed RNA Polymerases metabolism, Dickeya chrysanthemi metabolism, Dickeya chrysanthemi pathogenicity, Gene Expression Regulation, Bacterial, Molecular Sequence Data, Regulon, Repressor Proteins metabolism, Salmonella metabolism, Salmonella pathogenicity, Sequence Alignment, Transcription Factors chemistry, Transcription Factors metabolism, Virulence, Yersinia metabolism, Yersinia pathogenicity, Bacterial Proteins genetics, Dickeya chrysanthemi genetics, Repressor Proteins genetics, Salmonella genetics, Transcription Factors genetics, Yersinia genetics

Abstract

Virulence gene regulators RovA, SlyA and PecS comprise a subset of the MarR/SlyA family of transcriptional regulators, which has been shown to be involved in the regulation of virulence genes. These regulators have all been shown to both positively and negatively regulate the expression of multiple genes, involving several different mechanisms. One of the conserved mechanisms of regulatory control among these proteins appears to be competition for binding sites with other proteins. SlyA negatively regulates its own expression by interfering with the binding of RNA polymerase, whereas RovA appears to interfere with the progression of RNA polymerase from its promoter and to compete for binding with the heat-stable nucleoid-structural protein (H-NS), a global transcriptional silencer. PecS represses transcription by competing for binding with cAMP receptor protein, a global activator. RovA, SlyA and PecS have all been shown to act as derepressors by competing for binding sites with repressors. Recently, RovA also was found to enhance transcription through interaction with RNA polymerase.

Published

2006

49. Conserved role of the linker alpha-helix of the bacterial disulfide isomerase DsbC in the avoidance of misoxidation by DsbB.

Author

Segatori L, Murphy L, Arredondo S, Kadokura H, Gilbert H, Beckwith J, and Georgiou G

Subjects

Amino Acid Sequence, Bacterial Proteins chemistry, Catalysis, Conserved Sequence, Cysteine chemistry, Dickeya chrysanthemi metabolism, Dimerization, Disulfides chemistry, Electrophoresis, Polyacrylamide Gel, Escherichia coli Proteins chemistry, Gene Deletion, Haemophilus influenzae metabolism, Insulin metabolism, Kinetics, Membrane Proteins chemistry, Models, Biological, Molecular Sequence Data, Mutation, Oxidoreductases chemistry, Oxygen metabolism, Periplasmic Proteins chemistry, Phenotype, Phylogeny, Plasmids metabolism, Protein Binding, Protein Structure, Secondary, Protein Structure, Tertiary, Pseudomonas aeruginosa metabolism, Recombinant Proteins chemistry, Sequence Homology, Amino Acid, Species Specificity, Substrate Specificity, Thioredoxins chemistry, Vibrio cholerae metabolism, Yersinia pseudotuberculosis metabolism, Bacterial Proteins physiology, Escherichia coli Proteins physiology, Membrane Proteins physiology, Oxidoreductases physiology, Oxygen chemistry, Periplasmic Proteins physiology

Abstract

In the bacterial periplasm the co-existence of a catalyst of disulfide bond formation (DsbA) that is maintained in an oxidized state and of a reduced enzyme that catalyzes the rearrangement of mispaired cysteine residues (DsbC) is important for the folding of proteins containing multiple disulfide bonds. The kinetic partitioning of the DsbA/DsbB and DsbC/DsbD pathways partly depends on the ability of DsbB to oxidize DsbA at rates >1000 times greater than DsbC. We show that the resistance of DsbC to oxidation by DsbB is abolished by deletions of one or more amino acids within the alpha-helix that connects the N-terminal dimerization domain with the C-terminal thioredoxin domain. As a result, mutant DsbC carrying alpha-helix deletions could catalyze disulfide bond formation and complemented the phenotypes of dsbA cells. Examination of DsbC homologues from Haemophilus influenzae, Pseudomonas aeruginosa, Erwinia chrysanthemi, Yersinia pseudotuberculosis, Vibrio cholerae (30-70% sequence identity with the Escherichia coli enzyme) revealed that the mechanism responsible for avoiding oxidation by DsbB is a general property of DsbC family enzymes. In addition we found that deletions in the linker region reduced, but did not abolish, the ability of DsbC to assist the formation of active vtPA and phytase in vivo, in a DsbD-dependent manner, revealing that interactions between DsbD and DsbC are also conserved.

Published

2006

50. A differential medium for the isolation and rapid identification of a plant soft rot pathogen, Erwinia chrysanthemi.

Author

Lee YA and Yu CP

Subjects

Culture Media chemistry, Culture Media metabolism, Dickeya chrysanthemi classification, Dickeya chrysanthemi metabolism, Glycerol, Piperidones metabolism, Sensitivity and Specificity, Species Specificity, Taiwan, Dickeya chrysanthemi isolation & purification, Orchidaceae microbiology, Plant Diseases microbiology

Abstract

A medium was developed for the isolation and differentiation of Erwinia chrysanthemi from other Erwinia spp. based on the production of blue-pigmented indigoidine. The medium, named NGM, consists of nutrient agar supplemented with 1% glycerol, that induces pigment production, and 2 mM MnCl2*4H2O, that further enhances color development. More than fifty E. chrysanthemi strains from six different plant hosts were tested. All tested strains of E. chrysanthemi grew well on the NGM medium, developing dark brownish to blue colonies easily distinguishable from other Erwinia spp. The results indicate that pigment production on the NGM medium is a very stable property and can be used as a phenotypic property to differentiate E. chrysanthemi from other Erwinia spp. In addition, a specific oligonucleotide primer set was designed for the detection of indC, which is involved in indigoidine biosynthesis. All E. chrysanthemi strains tested contained indC as determined by PCR amplification. No amplification was observed with other Erwinia spp. Thus, pigment production of E. chrysanthemi on the NGM medium is consistent with the existence of indC. The NGM medium was used to isolate and identify the causal agent of soft rot lesions of diseased Phalaenopsis orchids from three orchid cultivation areas in Taiwan. The causal agents of Phalaenopsis soft rot were all identified as E. chrysanthemi. The results indicate that the NGM medium is efficient in isolation and identification of E. chrysanthemi from plants with soft rot symptoms and can also be used for epidemiological studies.

Published

2006