Your search keyword '"Helmut Hirt"' showing total 25 results

1. Dynamics of plasmid-mediated niche invasion, immunity to invasion, and pheromone-inducible conjugation in the murine gastrointestinal tract

Author

Helmut Hirt, Kerryl E. Greenwood-Quaintance, Aaron M. T. Barnes, Melissa J. Karau, Lisa M. Till, Elise Palzer, Weihua Guan, Michael S. VanNieuwenhze, Purna C. Kashyap, Robin Patel, and Gary M. Dunny

Subjects

Science

Abstract

Microbial communities provide protection to their hosts by excluding colonizing pathogens. Here the authors study plasmid transfer and plasmid-mediated effects on host colonization and persistence of Enterococcus faecalis in the intestinal tract of mice.

Published

2022

2. Polymer Adhesin Domains in Gram-Positive Cell Surface Proteins

Author

Michael A. Järvå, Helmut Hirt, Gary M. Dunny, and Ronnie P.-A. Berntsson

Subjects

adhesin, Gram-positive, conjugation, biofilm, binding, Microbiology, QR1-502

Abstract

Surface proteins in Gram-positive bacteria are often involved in biofilm formation, host-cell interactions, and surface attachment. Here we review a protein module found in surface proteins that are often encoded on various mobile genetic elements like conjugative plasmids. This module binds to different types of polymers like DNA, lipoteichoic acid and glucans, and is here termed polymer adhesin domain. We analyze all proteins that contain a polymer adhesin domain and classify the proteins into distinct classes based on phylogenetic and protein domain analysis. Protein function and ligand binding show class specificity, information that will be useful in determining the function of the large number of so far uncharacterized proteins containing a polymer adhesin domain.

Published

2020

3. Enterococcus faecalis Sex Pheromone cCF10 Enhances Conjugative Plasmid Transfer In Vivo

Author

Helmut Hirt, Kerryl E. Greenwood-Quaintance, Melissa J. Karau, Lisa M. Till, Purna C. Kashyap, Robin Patel, and Gary M. Dunny

Subjects

antibiotic resistance transfer, cell-cell signaling, competitive fitness, gut microbiota, mobile genetic element, Microbiology, QR1-502

Abstract

ABSTRACT Cell-cell communication mediated by peptide pheromones (cCF10 [CF]) is essential for high-frequency plasmid transfer in vitro in Enterococcus faecalis. To examine the role of pheromone signaling in vivo, we established either a CF-producing (CF+) recipient or a recipient producing a biologically inactive variant of CF (CF− recipient) in a germfree mouse model 3 days before donor inoculation and determined transfer frequencies of the pheromone-inducible plasmid pCF10. Plasmid transfer was detected in the upper and middle sections of the intestinal tract 5 h after donor inoculation and was highly efficient in the absence of antibiotic selection. The transconjugant/donor ratio reached a maximum level approaching 1 on day 4 in the upper intestinal tract. Plasmid transfer was significantly lower with the CF− recipient. While rescue of the CF− mating defect by coculture with CF+ recipients is easily accomplished in vitro, no extracellular complementation occurred in vivo. This suggests that most pheromone signaling in the gut occurs between recipient and donor cells in very close proximity. Plasmid-bearing cells (donors plus transconjugants) steadily increased in the population from 0.1% after donor inoculation to about 10% at the conclusion of the experiments. This suggests a selective advantage of pCF10 carriage distinct from antibiotic resistance or bacteriocin production. Our results demonstrate that pheromone signaling is required for efficient pCF10 transfer in vivo. In the absence of CF+ recipients, a low level of transfer to CF− recipients occurred in the gut. This may result from low-level host-mediated induction of the donors in the gastrointestinal (GI) tract, similar to that previously observed in serum. IMPORTANCE Horizontal gene transfer is a major factor in the biology of Enterococcus faecalis, an important nosocomial pathogen. Previous studies showing efficient conjugative plasmid transfer in the gastrointestinal (GI) tracts of experimental animals did not examine how the enterococcal sex pheromone response impacts the efficiency of transfer. Our study demonstrates for the first time pheromone-enhanced, high-frequency plasmid transfer of E. faecalis plasmid pCF10 in a mouse model in the absence of antibiotic or bacteriocin selection. Pheromone production by recipients dramatically increased plasmid transfer in germfree mice colonized initially with recipients, followed by donors. The presence of a coresident community of common gut microbes did not significantly reduce in vivo plasmid transfer between enterococcal donors and recipients. In mice colonized with enterococcal recipients, we detected plasmid transfer in the intestinal tract within 5 h of addition of donors, before transconjugants could be cultured from feces. Surprisingly, pCF10 carriage provided a competitive fitness advantage unrelated to antibiotic resistance or bacteriocin production.

Published

2018

4. A D-enantiomer of the antimicrobial peptide GL13K evades antimicrobial resistance in the Gram positive bacteria Enterococcus faecalis and Streptococcus gordonii.

Author

Helmut Hirt, Jeffrey W Hall, Elliot Larson, and Sven-Ulrik Gorr

Subjects

Medicine, Science

Abstract

Antimicrobial peptides represent an alternative to traditional antibiotics that may be less susceptible to bacterial resistance mechanisms by directly attacking the bacterial cell membrane. However, bacteria have a variety of defense mechanisms that can prevent cationic antimicrobial peptides from reaching the cell membrane. The L- and D-enantiomers of the antimicrobial peptide GL13K were tested against the Gram-positive bacteria Enterococcus faecalis and Streptococcus gordonii to understand the role of bacterial proteases and cell wall modifications in bacterial resistance. GL13K was derived from the human salivary protein BPIFA2. Minimal inhibitory concentrations were determined by broth dilution and a serial assay used to determine bacterial resistance. Peptide degradation was determined in a bioassay utilizing a luminescent strain of Pseudomonas aeruginosa to detect peptide activity. Autolysis and D-alanylation-deficient strains of E. faecalis and S. gordonii were tested in autolysis assays and peptide activity assays. E. faecalis protease inactivated L-GL13K but not D-GL13K, whereas autolysis did not affect peptide activity. Indeed, the D-enantiomer appeared to kill the bacteria prior to initiation of autolysis. D-alanylation mutants were killed by L-GL13K whereas this modification did not affect killing by D-GL13K. The mutants regained resistance to L-GL13K whereas bacteria did not gain resistance to D-GL13K after repeated treatment with the peptides. D-alanylation affected the hydrophobicity of bacterial cells but hydrophobicity alone did not affect GL13K activity. D-GL13K evades two resistance mechanisms in Gram-positive bacteria without giving rise to substantial new resistance. D-GL13K exhibits attractive properties for further antibiotic development.

Published

2018

5. Antimicrobial GL13K peptide coatings killed and ruptured the wall of Streptococcus gordonii and prevented formation and growth of biofilms.

Author

Xi Chen, Helmut Hirt, Yuping Li, Sven-Ulrik Gorr, and Conrado Aparicio

Subjects

Medicine, Science

Abstract

Infection is one of the most prevalent causes for dental implant failure. We have developed a novel antimicrobial peptide coating on titanium by immobilizing the antimicrobial peptide GL13K. GL13K was developed from the human salivary protein BPIFA2. The peptide exhibited MIC of 8 µg/ml against planktonic Pseudonomas aeruginosa and their biofilms were reduced by three orders of magnitude with 100 µg/ml GL13K. This peptide concentration also killed 100% of Streptococcus gordonii. At 1 mg/ml, GL13K caused less than 10% lysis of human red blood cells, suggesting low toxicity to mammalian cells. Our GL13K coating has also previously showed bactericidal effect and inhibition of biofilm growth against peri-implantitis related pathogens, such as Porphyromonas gingivalis. The GL13K coating was cytocompatible with human fibroblasts and osteoblasts. However, the bioactivity of antimicrobial coatings has been commonly tested under (quasi)static culture conditions that are far from simulating conditions for biofilm formation and growth in the oral cavity. Oral salivary flow over a coating is persistent, applies continuous shear forces, and supplies sustained nutrition to bacteria. This accelerates bacteria metabolism and biofilm growth. In this work, the antimicrobial effect of the coating was tested against Streptococcus gordonii, a primary colonizer that provides attachment for the biofilm accretion by P. gingivalis, using a drip-flow biofilm bioreactor with media flow rates simulating salivary flow. The GL13K peptide coatings killed bacteria and prevented formation and growth of S. gordonii biofilms in the drip-flow bioreactor and under regular mild-agitation conditions. Surprisingly the interaction of the bacteria with the GL13K peptide coatings ruptured the cell wall at their septum or polar areas leaving empty shell-like structures or exposed protoplasts. The cell wall rupture was not detected under regular culture conditions, suggesting that cell wall rupture induced by GL13K peptides also requires media flow and possible attendant biological sequelae of the conditions in the bioreactor.

Published

2014

6. Dynamics of plasmid-mediated niche invasion, immunity to invasion, and pheromone-inducible conjugation in the murine gastrointestinal tract

Author

Helmut Hirt, Kerryl E. Greenwood-Quaintance, Aaron M. T. Barnes, Melissa J. Karau, Lisa M. Till, Elise Palzer, Weihua Guan, Michael S. VanNieuwenhze, Purna C. Kashyap, Robin Patel, and Gary M. Dunny

Subjects

Intestines, Mice, Multidisciplinary, Bacterial Proteins, Conjugation, Genetic, Enterococcus faecalis, General Physics and Astronomy, Animals, General Chemistry, General Biochemistry, Genetics and Molecular Biology, Pheromones, Plasmids

Abstract

Microbial communities provide protection to their hosts by resisting pathogenic invasion. Microbial residents of a host often exclude subsequent colonizers, but this protection is not well understood. The Enterococcus faecalis plasmid pCF10, whose conjugative transfer functions are induced by a peptide pheromone, efficiently transfers in the intestinal tract of mice. Here we show that an invading donor strain established in the gastrointestinal tract of mice harboring resident recipients, resulting in a stable, mixed population comprised of approximately 10% donors and 90% recipients. We also show that the plasmid-encoded surface protein PrgB (Aggregation Substance), enhanced donor invasion of resident recipients, and resistance of resident donors to invasion by recipients. Imaging of the gastrointestinal mucosa of mice infected with differentially labeled recipients and donors revealed pheromone induction within microcolonies harboring both strains in close proximity, suggesting that adherent microcolonies on the mucosal surface of the intestine comprise an important niche for cell-cell signaling and plasmid transfer.

Published

2021

7. A new flavor of entry exclusion in ICE elements provides a selective advantage for the element and its host

Author

Helmut Hirt and Gary M. Dunny

Subjects

0303 health sciences, Gene Transfer, Horizontal, 030306 microbiology, Extramural, Mechanism (biology), Bacterial conjugation, Gene transfer, Computational biology, Biology, Microbiology, Article, 03 medical and health sciences, Conjugation, Genetic, Selective advantage, Element (category theory), Molecular Biology, Host (network), Gene, Bacillus subtilis, 030304 developmental biology

Abstract

Entry exclusion mechanisms have been described in many bacterial conjugation systems, but their molecular mechanisms are not well understood. In the current issue, Avello et al. describe a new exclusion system in the conjugative element ICEBs1. They identify the yddJ gene as the functional exclusion gene and its target as the protein product of the conG gene. They provide evidence for a possible mechanism, and for contribution of the system to reducing fitness costs of ICE expression.

Published

2019

8. Enterococcal PrgA extends far outside the cell and provides surface exclusion to protect against unwanted conjugation

Author

Gary M. Dunny, Andreas Schmitt, Helmut Hirt, Ronnie P.-A. Berntsson, Wei Sheng Sun, Josy ter Beek, and Michael Järvå

Subjects

DNA, Bacterial, Gene Transfer, Horizontal, Virulence Factors, In silico, Virulence, Virulence factor, Microbiology in the medical area, Type IV Secretion Systems, 03 medical and health sciences, 0302 clinical medicine, Plasmid, Bacterial Proteins, Structural Biology, Enterococcus faecalis, Mikrobiologi inom det medicinska området, Secretion, Adhesins, Bacterial, Cell adhesion, Molecular Biology, 030304 developmental biology, 0303 health sciences, Chemistry, Biochemistry and Molecular Biology, Membrane Proteins, Gene Expression Regulation, Bacterial, Cell biology, Bacterial adhesin, Horizontal gene transfer, 030217 neurology & neurosurgery, Function (biology), Enterococcus, Biokemi och molekylärbiologi, Plasmids

Abstract

Horizontal gene transfer between Gram-positive bacteria leads to a rapid spread of virulence factors and antibiotic resistance. This transfer is often facilitated via Type 4 Secretion Systems (T4SS), which frequently are encoded on conjugative plasmids. However, donor cells that already contain a particular conjugative plasmid resist acquisition of a 2nd copy of said plasmid. They utilize different mechanisms, including surface exclusion for this purpose. Enterococcus faecalis PrgA, encoded by the conjugative plasmid pCF10, is a surface protein that has been implicated to play a role in both virulence and surface exclusion, but the mechanism by which this is achieved has not been fully explained. Here, we report the structure of full-length PrgA, which shows that PrgA protrudes far out from the cell wall (approximately 40 nm), where it presents a protease domain. In vivo experiments show that PrgA provides a physical barrier to cellular adhesion, thereby reducing cellular aggregation. This function of PrgA contributes to surface exclusion, reducing the uptake of its cognate plasmid by approximately one order of magnitude. Using variants of PrgA with mutations in the catalytic site we show that the surface exclusion effect is dependent on the activity of the protease domain of PrgA. In silico analysis suggest that PrgA can interact with another enterococcal adhesin, PrgB, and that these two proteins have co-evolved. PrgB is a strong virulence factor, and PrgA is involved in post-translational processing of PrgB. Finally, competition mating experiments show that PrgA provides a significant fitness advantage to plasmid-carrying cells.

Published

2020

9. Mechanistic Features of the Enterococcal pCF10 Sex Pheromone Response and the Biology of Enterococcus faecalis in Its Natural Habitat

Author

Gary M. Dunny, Rebecca J. Breuer, and Helmut Hirt

Subjects

0301 basic medicine, Genetics, Gene Transfer, Horizontal, biology, Ecology (disciplines), 030106 microbiology, Niche, Gene Expression Regulation, Bacterial, biology.organism_classification, Meeting Review, Microbiology, In vitro, Enterococcus faecalis, 03 medical and health sciences, Antibiotic resistance, Plasmid, Bacterial Proteins, Conjugation, Genetic, Sex pheromone, Horizontal gene transfer, Molecular Biology, Plasmids

Abstract

Conjugative transfer of plasmids in enterococci is promoted by intercellular communication using peptide pheromones. The regulatory mechanisms that control transfer have been extensively studied in vitro . However, the complicated systems that regulate the spread of these plasmids did not evolve in the laboratory test tube, and remarkably little is known about this form of signaling in the intestinal tract, the primary niche of these organisms. Because the evolution of Enterococcus faecalis strains and their coresident pheromone-inducible plasmids, such as pCF10, have occurred in the gastrointestinal (GI) tract, it is important to consider the functions controlled by pheromones in light of this ecology. This review summarizes our current understanding of the pCF10-encoded pheromone response. We consider how selective pressures in the natural environment may have selected for the complex and very tightly regulated systems controlling conjugation, and we pay special attention to the ecology of enterococci and the pCF10 plasmid as a gut commensal. We summarize the results of recent studies of the pheromone response at the single-cell level, as well as those of the first experiments demonstrating a role for pheromone signaling in plasmid transfer and in GI tract competitive fitness. These results will serve as a foundation for further in vivo studies that could lead to novel interventions to reduce opportunistic infections and the spread of antibiotic resistance.

Published

2018

10. Antimicrobial Peptide GL13K Is Effective in Reducing Biofilms of Pseudomonas aeruginosa

Author

Sven Ulrik Gorr and Helmut Hirt

Subjects

Pharmacology, Alanine, chemistry.chemical_classification, Pseudomonas aeruginosa, Antimicrobial peptides, Biofilm, Peptide, Biology, medicine.disease_cause, biology.organism_classification, Antimicrobial, Anti-Bacterial Agents, Microbiology, Infectious Diseases, Anti-Infective Agents, chemistry, Biochemistry, Biofilms, medicine, Pharmacology (medical), Peptides, Mechanisms of Action: Physiological Effects, Peptide sequence, Bacteria

Abstract

Human parotid secretory protein (PSP; BPIF2A) is predicted to be structurally similar to bactericidal/permeability-increasing protein and lipopolysaccharide (LPS)-binding protein. Based on the locations of known antimicrobial peptides in the latter two proteins, potential active peptides in the PSP sequence were identified. One such peptide, GL13NH 2 (PSP residues 141 to 153) was shown previously to interfere with LPS binding and agglutinate bacteria without bactericidal activity. By introducing three additional positively charged lysine residues, the peptide was converted to the novel bactericidal cationic peptide GL13K (MIC for Pseudomonas aeruginosa , 8 μg/ml [5.6 μM]). We investigated the antibiofilm activity of GL13K against static, monospecies biofilms of P. aeruginosa PAO1. Two-hour exposure of a 24-h biofilm to 64 μg/ml (44.8 μM) GL13K reduced biofilm bacteria by 10 2 , and 100 μg/ml (70 μM) GL13K reduced bacteria by 10 3 . Similar results could be achieved on 48-h-old biofilms. Lower concentrations of GL13K (32 μg/ml [22.4 μM]) were successful in reducing biofilm cell numbers in combination with tobramycin. This combination treatment also achieved total eradication of the biofilm in a majority (67.5%) of tested samples. An alanine scan of GL13K revealed the importance of the leucine residue in position six of the peptide sequence, where replacement led to a loss of antibiofilm activity, whereas the impact of replacing charged residues was less pronounced. Bacterial metalloproteases were found to partially inactivate GL13K but not a d amino acid version of the peptide.

Published

2013

11. Antibiotic Resistance of Enterococci in American Bison ( Bison bison ) from a Nature Preserve Compared to That of Enterococci in Pastured Cattle

Author

Helmut Hirt, John F. Anderson, Ludek Zurek, Mastura Akhtar, and Torrey D. Parrish

Subjects

Enterococcus faecium, Population, Applied Microbiology and Biotechnology, Enterococcus faecalis, Microbiology, Bison bison, Feces, Hemolysin Proteins, Bacteriocins, Ciprofloxacin, Vancomycin, Enterococcus hirae, Drug Resistance, Bacterial, Environmental Microbiology, Enterococcus casseliflavus, Animals, symbols.heraldic_charge, education, visual_art.artwork, education.field_of_study, Bison, Ecology, biology, Biodiversity, Tetracycline, biochemical phenomena, metabolism, and nutrition, biology.organism_classification, Erythromycin, Chloramphenicol, Phenotype, Enterococcus, Gelatinases, American bison, visual_art, symbols, Ampicillin, Cattle, Food Science, Biotechnology

Abstract

Enterococci isolated from a bison population on a native tall-grass prairie preserve in Kansas were characterized and compared to enterococci isolated from pastured cattle. The species diversity was dominated by Enterococcus casseliflavus in bison (62.4%), while Enterococcus hirae was the most common isolate from cattle (39.7%). Enterococcus faecalis was the second most common species isolated from bison (16%). In cattle, E. faecalis and Enterococcus faecium were isolated at lower percentages (3.2% and 1.6%, respectively). No resistance to ampicillin, chloramphenicol, gentamicin, or high levels of vancomycin was detected from either source. Tetracycline and erythromycin resistance phenotypes, encoded by tetO and ermB , respectively, were common in cattle isolates (42.9% and 12.7%, respectively). A significant percentage of bison isolates (8% and 4%, respectively) were also resistant to these two antibiotics. The tetracycline resistance genes from both bison and cattle isolates resided on mobile genetic elements and showed a transfer frequency of 10 −6 per donor, whereas erythromycin resistance was not transferable. Resistance to ciprofloxacin was found to be higher in enterococci from bison (14.4%) than in enterococci isolated from cattle (9.5%). The bison population can serve as a sentinel population for studying the spread and origin of antibiotic resistance.

Published

2008

12. The Salivary Protein PSP/Bpifa2 Protects Against Intestinal Inflammation

Author

Helmut Hirt, Seshagiri Rao Nandula, and Sven Ulrik Gorr

Subjects

business.industry, digestive, oral, and skin physiology, Inflammatory Bowel Diseases, medicine.disease, digestive system, Biochemistry, digestive system diseases, Malnutrition, Diarrhea, Immune system, Weight loss, Intestinal inflammation, Immunology, Genetics, Salivary Proteins, Medicine, sense organs, medicine.symptom, business, Molecular Biology, Biotechnology

Abstract

Inflammatory bowel diseases are associated with intestinal inflammation, diarrhea, malnutrition and weight loss. IBD appears to result from immune system dysregulation, diet and changes to the gut ...

Published

2015

13. Transcriptional Response of Enterococcus faecalis V583 to Erythromycin

Author

Helmut Hirt, Vivek Kapur, Lars Snipen, Ågot Aakra, Ingolf F. Nes, Barbara E. Murray, Are H. Aastveit, Heidi Vebø, and Gary M. Dunny

Subjects

Transcription, Genetic, medicine.medical_treatment, Erythromycin, ATP-binding cassette transporter, Microbial Sensitivity Tests, Enterococcus faecalis, Microbiology, Bacterial Proteins, Gene expression, medicine, Humans, Pharmacology (medical), Mechanisms of Action: Physiological Effects, Gene, Oligonucleotide Array Sequence Analysis, Antibacterial agent, Pharmacology, Regulation of gene expression, Chemotherapy, Errata, biology, business.industry, Gene Expression Profiling, Gene Expression Regulation, Bacterial, Antimicrobial, biology.organism_classification, Anti-Bacterial Agents, Gene expression profiling, Infectious Diseases, Transcriptional response, business, Genome, Bacterial, medicine.drug

Abstract

A transcriptional profile of Enterococcus faecalis V583 (V583) treated with erythromycin is presented. This is the first study describing a complete transcriptional profile of Enterococcus. E. faecalis is a common and nonvirulent bacterium in many natural environments, but also an important cause of nosocomial infections. We have used a genome-wide microarray based on the genome sequence of V583 to study gene expression in cells exposed to erythromycin. V583 is resistant to relatively high concentrations of erythromycin, but growth is retarded by the treatment. The effect of erythromycin treatment on V583 was studied by a time course experiment; samples were extracted at five time points over a period of 90 min. A drastic change in gene transcription was seen with the erythromycin-treated cells compared to the untreated cells. Altogether, 260 genes were down-regulated at one or more time points, while 340 genes were up-regulated. Genes encoding hypothetical proteins and genes encoding transport and binding proteins were the two most dominating groups of differentially expressed genes. The gene encoding ermB (EFA0007) was expressed, but not differentially, which indicated that other genes are important for the survival and growth maintenance of V583 treated with erythromycin. One of these genes is a putative MsrC-like protein, which was up-regulated at all time points studied. Other specific genes that were found to be up-regulated were genes encoding ABC transporters and two-component regulatory systems, and these may be genes that are important for the specific response of V583 to erythromycin.

Published

2005

14. Characterization of the Pheromone Response of the Enterococcus faecalis Conjugative Plasmid pCF10: Complete Sequence and Comparative Analysis of the Transcriptional and Phenotypic Responses of pCF10-Containing Cells to Pheromone Induction

Author

Vivek Kapur, Jack H. Staddon, Jesper K. Marklund, Dawn A. Manias, Edward M. Bryan, Joanna R. Klein, Michael L. Paustian, Gary M. Dunny, and Helmut Hirt

Subjects

DNA, Bacterial, Transcription, Genetic, Bacteriophages, Transposons, and Plasmids, Chromosome Mapping, Virulence, Biology, biology.organism_classification, Polymerase Chain Reaction, Microbiology, Molecular biology, Pheromones, Enterococcus faecalis, law.invention, Open reading frame, Complete sequence, Phenotype, Plasmid, law, Transcription (biology), Molecular Biology, Gene, Phylogeny, Polymerase chain reaction, Plasmids

Abstract

The sex pheromone plasmids in Enterococcus faecalis are one of the most efficient conjugative plasmid transfer systems known in bacteria. Plasmid transfer rates can reach or exceed 10 −1 transconjugants per donor in vivo and under laboratory conditions. We report the completion of the DNA sequence of plasmid pCF10 and the analysis of the transcription profile of plasmid genes, relative to conjugative transfer ability following pheromone induction. These experiments employed a mini-microarray containing all 57 open reading frames of pCF10 and a set of selected chromosomal genes. A clear peak of transcription activity was observed 30 to 60 min after pheromone addition, with transcription subsiding 2 h after pheromone induction. The transcript activity correlated with the ability of donor cells to transfer pCF10 to recipient cells. Remarkably, aggregation substance (Asc10, encoded by the prgB gene) was present on the cell surface for a long period of time after pheromone-induced transcription of prgB and plasmid transfer ability had ceased. This observation could have relevance for the virulence of E. faecalis .

Published

2005

15. An amino-terminal domain of Enterococcus faecalis aggregation substance is required for aggregation, bacterial internalization by epithelial cells and binding to lipoteichoic acid

Author

Helmut Hirt, Christopher M. Waters, Patrick M. Schlievert, Gary M. Dunny, Carol L. Wells, and John K. McCormick

Subjects

Lipopolysaccharides, Gene Transfer, Horizontal, media_common.quotation_subject, Microbiology, Bacterial Adhesion, Enterococcus faecalis, Cell Line, Cell wall, Plasmid, Bacterial Proteins, Mutant protein, Humans, Internalization, Molecular Biology, Sequence Deletion, media_common, chemistry.chemical_classification, Virulence, biology, Membrane Proteins, biology.organism_classification, Protein Structure, Tertiary, Amino acid, Teichoic Acids, Enterocytes, Biochemistry, chemistry, Mutation, Lipoteichoic acid, HT29 Cells, Bacteria, Plasmids, Protein Binding

Abstract

Aggregation substance (AS), a plasmid-encoded surface protein of Enterococcus faecalis, plays important roles in virulence and antibiotic resistance transfer. Previous studies have suggested that AS-mediated aggregation of enterococcal cells could involve the binding of this protein to cell wall lipoteichoic acid (LTA). Here, a method to purify an undegraded form of Asc10, the AS of the plasmid pCF10, is described. Using this purified protein, direct binding of Asc10 to purified E. faecalis LTA was demonstrated. Equivalent binding of Asc10 to LTA purified from INY3000, an E. faecalis strain that is incapable of aggregation, was also observed. Surprisingly, mutations in a previously identified aggregation domain from amino acids 473 to 683 that abolished aggregation had no effect on LTA binding. In frame deletion analysis of Asc10 was used to identify a second aggregation domain located in the N-terminus of the protein from amino acids 156 to 358. A purified Asc10 mutant protein lacking this domain showed reduced LTA binding, while a purified N-terminal fragment from amino acids 44-331 had high LTA binding. Like the previously described aggregation domain, the newly identified Asc10((156-358)) aggregation domain was also required for efficient internalization of E. faecalis into HT-29 enterocytes. Thus, Asc10 possess two distinct domains required for aggregation and eukaryotic cell internalization: an N-terminal domain that promotes binding to LTA and a second domain located near the middle of the protein.

Published

2004

16. Enterococcal Aggregation Substance and Binding Substance Are Not Major Contributors to Urinary Tract Colonization by Enterococcus faecalis in a Mouse Model of Ascending Unobstructed Urinary Tract Infection

Author

James R. Johnson, Gary M. Dunny, Christopher M. Waters, Helmut Hirt, and Connie Clabots

Subjects

Urinary system, Immunology, Receptors, Cell Surface, Urine, Biology, Microbiology, Enterococcus faecalis, law.invention, Mice, Plasmid, Bacterial Proteins, In vivo, law, Animals, Humans, Urinary Tract, Gram-Positive Bacterial Infections, Bacterial Infections, Streptococcaceae, biology.organism_classification, In vitro, Disease Models, Animal, Infectious Diseases, Urinary Tract Infections, Mice, Inbred CBA, Recombinant DNA, Female, Parasitology

Abstract

Isogenic Enterococcus faecalis strains that differ in their expression of aggregation substance (AS) and its cognate receptor, enterococcal binding substance (EBS), were compared for urovirulence in mice. Strain OG1SSp/pCF500 (inducible AS + , constitutive EBS + ) failed to outcompete isogenic derivative INY3000 (AS − EBS − ) in the urine, bladders, or kidneys of mice harvested at 48 h postinoculation. Neither mouse nor human urine induced AS expression by OG1SSp/pCF500. Recombinant strain OG1SSp/pINY1801 (constitutive AS + , EBS + ) exhibited plasmid segregation that was as extensive in vivo as in vitro. These data suggest that AS and EBS do not contribute to upper or lower urinary tract colonization by E. faecalis and that growth in urine does not induce AS expression by strains carrying plasmids in the pCF10 family.

Published

2004

17. In Vivo Induction of Virulence and Antibiotic Resistance Transfer in Enterococcus faecalis Mediated by the Sex Pheromone-Sensing System of pCF10

Author

Helmut Hirt, Gary M. Dunny, and Patrick M. Schlievert

Subjects

DNA, Bacterial, Tetracycline, Immunology, Population, Virulence, Biology, Microbiology, Virulence factor, Enterococcus faecalis, Plasmid, Bacterial Proteins, In vivo, medicine, Animals, Humans, education, Gram-Positive Bacterial Infections, education.field_of_study, Tetracycline Resistance, Endocarditis, Bacterial, biology.organism_classification, Molecular Pathogenesis, In vitro, Disease Models, Animal, Infectious Diseases, Parasitology, Rabbits, Carrier Proteins, Plasmids, medicine.drug

Abstract

Enterococcus faecalis has become one of the most notable nosocomial pathogens in the last decade. Aggregation substance (AS) on the sex pheromone plasmids of E. faecalis has been implicated as a virulence factor in several model systems. We investigated the AS-encoding plasmid pCF10 for its ability to increase virulence in a rabbit endocarditis model. Cells containing pCF10 increased the virulence in the model significantly, as assessed by an increase in aortic valve vegetation size. The results confirmed in vivo induction of the normally tightly controlled AS. In addition to the expression of AS when E. faecalis cells were in contact with plasma, plasmid transfer of the tetracycline resistance-carrying plasmid was also activated in vitro and in vivo. In vivo, plasmid transfer reached remarkable frequencies of 8 × 10 −2 to 9 × 10 −2 . These values are comparable to the highest frequencies ever observed in vitro. Cells harboring pCF10 had a significant survival advantage over plasmid-free cells indicated by pCF10 present in two-thirds of the recipient population. Plasma induction was dependent on the presence of the plasmid-encoded PrgZ protein, indicating the requirement of the pheromone-sensing system in the induction process. The data suggested that the mechanism of in vivo induction may involve interference of plasma with the normal function of the pheromone peptide and its inhibitor.

Published

2002

18. Antibodies to a Surface-Exposed, N-terminal Domain of Aggregation Substance Are Not Protective in the Rabbit Model of Enterococcus faecalis Infective Endocarditis

Author

Timothy J. Tripp, Gary M. Dunny, Helmut Hirt, John K. McCormick, Patrick M. Schlievert, and Christopher M. Waters

Subjects

Molecular Sequence Data, Immunology, Macrophage-1 Antigen, Microbiology, Enterococcus faecalis, Immune system, Bacterial Proteins, Phagocytosis, Western blot, medicine, Animals, Endocarditis, Amino Acid Sequence, Cloning, Molecular, Gram-Positive Bacterial Infections, Antiserum, Base Sequence, biology, medicine.diagnostic_test, Membrane Proteins, Endocarditis, Bacterial, medicine.disease, biology.organism_classification, Antibodies, Bacterial, Peptide Fragments, Infectious Diseases, Polyclonal antibodies, Infective endocarditis, Microbial Immunity and Vaccines, biology.protein, Immunization, Parasitology, Rabbits, Antibody

Abstract

The aggregation substance (AS) surface protein from Enterococcus faecalis has been implicated as an important virulence factor for the development of infective endocarditis. To evaluate the role of antibodies specific for Asc10 (the AS protein from the conjugative plasmid pCF10) in protective immunity to infective endocarditis, an N-terminal region of Asc10 lacking the signal peptide and predicted to be surface exposed (amino acids 44 to 331; AS 44–331 ) was cloned with a C-terminal histidine tag translational fusion and expressed from Escherichia coli . N-terminal amino acid sequencing of the purified protein revealed the correct sequence, and rabbit polyclonal antisera raised against AS 44–331 reacted specifically to Asc10 expressed from E. faecalis OG1SSp, but not to other proteins as judged by Western blot analysis. Using these antisera, flow cytometry analysis demonstrated that antibodies to AS 44–331 bound to a surface-exposed region of Asc10. Furthermore, antibodies specific for AS 44–331 were opsonic for E. faecalis expressing Asc10 in vitro but not for cells that did not express Asc10. New Zealand White rabbits immunized with AS 44–331 were challenged intravenously with E. faecalis cells constitutively expressing Asc10 in the rabbit model of experimental endocarditis. Highly immune animals did not show significant differences in clearance of organisms from the blood or spleen or in formation of vegetations on the aortic valve, in comparison with nonimmune animals. Although in vivo expression of Asc10 was demonstrated by immunohistochemistry, these experiments provide evidence that immunity to Asc10 does not play a role in protection from experimental infective endocarditis due to E. faecalis and may have important implications for the development of immunological approaches to combat enterococcal endocarditis.

Published

2001

19. Inducible Expression of Enterococcus faecalis Aggregation Substance Surface Protein Facilitates Bacterial Internalization by Cultured Enterocytes

Author

Gary M. Dunny, Stanley L. Erlandsen, Julie A. Hoag, Carol L. Wells, Helmut Hirt, and Elizabeth A. Moore

Subjects

Enterocyte, media_common.quotation_subject, Immunology, Heterologous, Virulence, Microbiology, Enterococcus faecalis, Bacterial Proteins, Intestinal mucosa, medicine, Humans, Intestinal Mucosa, Internalization, Nisin, media_common, Cellular Microbiology: Pathogen-Host Cell Molecular Interactions, biology, Lactococcus lactis, biology.organism_classification, Cell Hypoxia, Infectious Diseases, medicine.anatomical_structure, Caco-2, Parasitology, Caco-2 Cells, HT29 Cells

Abstract

Aggregation substance (AS) is an Enterococcus faecalis surface protein that may contribute to virulence. Using a recently described system for controlled expression of AS in E. faecalis and the heterologous host Lactococcus lactis , experiments were designed to assess the effect of AS on bacterial internalization by HT-29 and Caco-2 enterocytes. AS expression was associated with increased internalization of E. faecalis by HT-29 enterocytes and of L. lactis by HT-29 and Caco-2 enterocytes. Compared to enterocytes cultivated under standard conditions, either cultivation in hypoxia or 1-h pretreatment of enterocytes with calcium-free medium resulted in increased internalization of both E. faecalis and L. lactis (with and without AS expression). Also, AS expression augmented these increases when E. faecalis was incubated with pretreated HT-29 enterocytes and when L. lactis was incubated with pretreated Caco-2 and HT-29 enterocytes. These data indicated that AS might facilitate E. faecalis internalization by cultured enterocytes.

Published

2000

20. Heterologous Inducible Expression of Enterococcus faecalis pCF10 Aggregation Substance Asc10 in Lactococcus lactis and Streptococcus gordonii Contributes to Cell Hydrophobicity and Adhesion to Fibrin

Author

Helmut Hirt, Gary M. Dunny, and Stanley L. Erlandsen

Subjects

biology, Lactococcus lactis, Streptococcus gordonii, Virulence, Heterologous, biology.organism_classification, Microbiology, Virulence factor, Enterococcus faecalis, Plasmid, Biochemistry, Heterologous expression, Molecular Biology

Abstract

Aggregation substance proteins encoded by the sex pheromone plasmid family of Enterococcus faecalis have been shown previously to contribute to the formation of a stable mating complex between donor and recipient cells and have been implicated in the virulence of this increasingly important nosocomial pathogen. In an effort to characterize the protein further, prgB , the gene encoding the aggregation substance Asc10 on pCF10, was cloned in a vector containing the nisin-inducible nisA promoter and its two-component regulatory system. Expression of aggregation substance after nisin addition to cultures of E. faecalis and the heterologous bacteria Lactococcus lactis and Streptococcus gordonii was demonstrated. Electron microscopy revealed that Asc10 was presented on the cell surfaces of E. faecalis and L. lactis but not on that of S. gordonii . The protein was also found in the cell culture supernatants of all three species. Characterization of Asc10 on the cell surfaces of E. faecalis and L. lactis revealed a significant increase in cell surface hydrophobicity upon expression of the protein. Heterologous expression of Asc10 on L. lactis also allowed the recognition of its binding ligand (EBS) on the enterococcal cell surface, as indicated by increased transfer of a conjugative transposon. We also found that adhesion of Asc10-expressing bacterial cells to fibrin was elevated, consistent with a role for the protein in the pathogenesis of enterococcal endocarditis. The data demonstrate that Asc10 expressed under the control of the nisA promoter in heterologous species will be an useful tool in the detailed characterization of this important enterococcal conjugation protein and virulence factor.

Published

2000

21. Lysine substitutions convert a bacterial-agglutinating peptide into a bactericidal peptide that retains anti-lipopolysaccharide activity and low hemolytic activity

Author

Seshagiri Rao Nandula, Sven Ulrik Gorr, Mahsa Abdolhosseini, Jonathan Song, and Helmut Hirt

Subjects

Lipopolysaccharides, Male, Agglutination, Physiology, Gram-positive bacteria, Peptide, medicine.disease_cause, Biochemistry, Hemolysis, Article, Microbiology, Cellular and Molecular Neuroscience, Mice, Endocrinology, Anti-Infective Agents, medicine, Escherichia coli, Animals, chemistry.chemical_classification, Alanine, biology, Lysine, Streptococcus gordonii, medicine.disease, biology.organism_classification, Peptide Fragments, Amino acid, Anti-Bacterial Agents, Mice, Inbred C57BL, chemistry, Amino Acid Substitution, Pseudomonas aeruginosa, Porphyromonas gingivalis, Bacteria, Antimicrobial Cationic Peptides

Abstract

GL13NH2 is a bacteria-agglutinating peptide derived from the sequence of the salivary protein parotid secretory protein (PSP, BPIFA2, SPLUNC2, C20orf70). The peptide agglutinates both Gram negative and Gram positive bacteria, and shows anti-lipopolysaccharide activity in vitro and in vivo. However, GL13NH2 does not exhibit bactericidal activity. To generate a more cationic peptide with potential bactericidal activity, three amino acid residues were replaced with lysine residues to generate the peptide GL13K. In this report, the antibacterial and anti-inflammatory activities of GL13K were characterized. GL13K had lost the ability to agglutinate bacteria but gained bactericidal activity. Substitution of individual amino acids in GL13K with alanine did not restore bacterial agglutination. GL13K was bactericidal against Pseudomonas aeruginosa, Streptococcus gordonii and Escherichia coli but not Porphyromonas gingivalis. Unlike the agglutinating activity of GL13NH2, the bactericidal activity of GL13K against Pseudomonas aeruginosa was retained in the presence of saliva. Both GL13NH2 and GL13K exhibited anti-lipopolysaccharide activity. In GL13K, this activity appeared to depend on a serine hydroxyl group. GL13K protected mice from lipopolysaccharide- induced sepsis and the peptide exhibited a low level of hemolysis, suggesting that it may be suitable for in vivo application.

Published

2012

22. Antimicrobial GL13K-peptide coatings

Author

Xi, Chen, primary, Helmut, Hirt, additional, Sven, Gorr, additional, and Conrado, Aparicio, additional

Published

2016

23. A paracrine peptide sex pheromone also acts as an autocrine signal to induce plasmid transfer and virulence factor expression in vivo

Author

Josephine R. Chandler, Helmut Hirt, and Gary M. Dunny

Subjects

Multidisciplinary, Gene Transfer, Horizontal, Virulence Factors, Molecular Sequence Data, Endogeny, Biology, Biological Sciences, Molecular biology, Virulence factor, Pheromones, Paracrine signalling, Plasmid, Conjugation, Genetic, Pheromone activity, Enterococcus faecalis, Humans, Amino Acid Sequence, Signal transduction, Cell-cell signaling, Autocrine signalling, Oligopeptides, Serum Albumin, Plasmids, Signal Transduction

Abstract

The peptide pheromone cCF10 of Enterococcus faecalis is an intercellular signal for induction of conjugative transfer of plasmid pCF10 from donor cells to recipient cells. When a donor cell is exposed to recipient-produced cCF10, expression of the pCF10-encoded aggregation substance of pCF10 (Asc10) and other conjugation gene products is activated. Asc10 also increases enterococcal virulence in several models, and when donor cells are grown in animals or in plasma, Asc10 expression is induced by means of the cCF10-sensing machinery. Plasmid pCF10 carries two genes that function to prevent self-induction by endogenous cCF10 in donor cells. The membrane protein PrgY reduces endogenous pheromone activity in donor cells, and the inhibitor peptide iCF10 neutralizes the residual endogenous cCF10 that escapes PrgY. In the current study, we found that E. faecalis strains with allelic replacements abolishing active cCF10 production showed reduced ability to acquire pCF10 by conjugation; prgY -null mutations had no phenotype in the cCF10-negative strains. We observed that expression of the mRNA for iCF10 was reduced in this background and that these mutations also blocked plasma induction of Asc10 expression. These findings support a model in which plasma induction in wild-type donors results from iCF10 inactivation by a plasma component, causing disruption of a precisely maintained balance of iCF10 to cCF10 activity and allowing subsequent induction by endogenous cCF10. Although cCF10 has traditionally been viewed as an intercellular signal, these results show that pCF10 has also adapted cCF10 as an autocrine signal that activates expression of virulence and conjugation functions.

Published

2005

24. Aggregation and Binding Substances Enhance Pathogenicity in Rabbit Models of Enterococcus faecalis Endocarditis

Author

Helmut Hirt, Aris P. Assimacopoulos, Gary M. Dunny, Jennifer Stoehr, Pamala J. Gahr, Martin M. Dinges, Patrick M. Schlievert, and John Harmala

Subjects

Cell Extracts, Pathology, medicine.medical_specialty, Immunology, Cell, Lymphocyte proliferation, Biology, Lymphocyte Activation, Microbiology, Enterococcus faecalis, Bacterial Adhesion, Catheterization, Interferon-gamma, Bacterial Proteins, medicine, Superantigen, Endocarditis, Animals, Humans, Interferon gamma, Lymphocytes, Sex Attractants, Adhesins, Bacterial, Lung, Lymphotoxin-alpha, Cells, Cultured, Inflammation, Superantigens, Tumor Necrosis Factor-alpha, Endocarditis, Bacterial, Macrophage Activation, medicine.disease, biology.organism_classification, In vitro, Infectious Diseases, medicine.anatomical_structure, Culture Media, Conditioned, Splenomegaly, Molecular and Cellular Pathogenesis, Leukocytes, Mononuclear, Parasitology, Tumor necrosis factor alpha, Rabbits, Cell Division, medicine.drug

Abstract

We investigated the importance of enterococcal aggregation substance (AS) and enterococcal binding substance (EBS) in rabbit models of Enterococcus faecalis cardiac infections. First, American Dutch belted rabbits were injected intraventricularly with 10 8 CFU and observed for 2 days. No clinical signs of illness developed in animals given AS − EBS − organisms, and all survived. All rabbits given AS − EBS + organisms developed signs of illness, including significant pericardial inflammation, but only one of six died. All animals given AS + EBS − organisms developed signs of illness, including pericardial inflammation, and survived. All rabbits given AS + EBS + organisms developed signs of illness and died. None of the rabbits receiving AS + EBS + organisms showed gross pericardial inflammation. The lethality and lack of inflammation are consistent with the presence of a superantigen. Rabbit and human lymphocytes were highly stimulated in vitro by cell extracts, but not cell-free culture fluids, of AS + EBS + organisms. In contrast, cell extracts from AS − EBS − organisms weakly stimulated lymphocyte proliferation. Culture fluids from human lymphocytes stimulated with AS + /EBS + enterococci contained high levels of gamma interferon and tumor necrosis factor alpha (TNF-α) and TNF-β, which is consistent with functional stimulation of T-lymphocyte proliferation and macrophage activation. Subsequent experiments examined the abilities of the same strains to cause endocarditis in a catheterization model. New Zealand White rabbits underwent transaortic catheterization for 2 h, at which time catheters were removed and animals were injected with 2 × 10 9 CFU of test organisms. None of the animals given AS − EBS − organisms developed vegetations or showed autopsy evidence of tissue damage. Rabbits given AS − EBS + or AS + EBS − organisms developed small vegetations and had splenomegaly at autopsy. All rabbits given AS + EBS + organisms developed large vegetations and had splenomegaly and lung congestion at autopsy. Similar experiments that left catheters in place for 3 days revealed that all rabbits given AS − EBS − or AS + EBS + organisms developed vegetations, but animals given AS + EBS + organisms had larger vegetations and autopsy evidence of lung congestion. These experiments provide direct evidence that these two cell wall components play an important role in the pathogenesis of endocarditis as well as in conjugative plasmid transfer.

Published

1998

25. Biochemical, immunological and ultrastructural characterization of aggregation substances encoded by Enterococcus faecalis sex-pheromone plasmids

Author

Dominique Galli, Reinhard Wirth, Gerhard Wanner, and Helmut Hirt

Subjects

chemistry.chemical_classification, biology, Blotting, Western, biology.organism_classification, Biochemistry, Enterococcus faecalis, Bacterial cell structure, Antibodies, Peptide Fragments, Bacterial adhesin, Microscopy, Electron, Plasmid, chemistry, Bacterial Proteins, Ultrastructure, biology.protein, Electrophoresis, Polyacrylamide Gel, Antibody, Antigens, Sex Attractants, Glycoprotein, Bacteria, Plasmids

Abstract

The sex-pheromone system of Enterococcus faecalis can be viewed as a unique and highly efficient plasmid-collection mechanism. The contact needed for transfer of the conjugative sex-pheromone plasmids is mediated by an adhesin, called aggregation substance, which is encoded by these plasmids. We show here that for 17 of the 18 sex-pheromone plasmids (pAM373 being the exception) described to date, their adhesins are immunologically related to each other. In each case, we observed the presence of an N-terminal fragment of about 78 kDa in addition to the 137-kDa form of mature aggregation substance. The cross-reactions were different for the various plasmids. In the case of pPD1 the 78-kDa fragment reacted only weakly. The aggregation substance encoded by sex-pheromone plasmid pAD1 (Asa1) was characterized in detail. The conditions used for SDS/PAGE had a drastic influence on the migration behavior of mature aggregation substance and differently migrating, interconvertible forms were identified. Preliminary data indicate that Asa1 might be a glycoprotein. Antibodies were isolated which are directed against the N- and C-terminal parts of aggregation substance. They showed about the same reactivity on Western blots; however, only antibodies directed against the N-terminal part of the aggregation substance could inhibit the bacterial cell/cell contact. The reactions of the two antibody preparations with induced cells of E. faecalis was analyzed by transmission electron microscopy. The results indicated that especially the N-terminal part of aggregation substance is exposed on the cell surface of E. faecalis; the C-terminal part seems to be much less exposed.

Published

1993