Your search keyword '"Riccardo Manetti"' showing total 4 results

1. Mutations in the linker region of BvgS abolish response to environmental signals for the regulation of the virulence factors in Bordetella pertussis

Author

Rino Rappuoli, Riccardo Manetti, Beatrice Aricò, Vincenzo Scarlato, Manetti R., Arico B., Rappuoli R., and Scarlato V.

Subjects

Bordetella pertussis, Transcription, Genetic, Molecular Sequence Data, Mutant, Virulence, Biology, Bacterial Proteins, Transcription (biology), bvg locu, Genetics, Amino Acid Sequence, Gene, Peptide sequence, Regulation of gene expression, Promoter, Gene Expression Regulation, Bacterial, General Medicine, biology.organism_classification, Molecular biology, two-component system, Pathogenic bacteria, Mutation, environmental transcription control, Transcription Factors

Abstract

Expression of virulence factors of Bordetella pertussis is coordinately regulated by the products of the bvg locus, which codes for a sensory protein (BvgS) and a positive regulator of transcription (BvgA), a pair in the family of bacterial 'two-component' regulators. Transcription of the bvg-regulated promoters is repressed by modulating environmental factors such as 50 mM MgSO4, 10 mM nicotinic acid (NA) or low temperature (25 degrees C). We have isolated a spontaneous mutant (SK170) which expresses virulence genes at either 25 degrees C, or in the presence of 1-5 mM NA, or 10-50 mM MgSO4. Virulence factors in strain SK170 are still repressed by higher concentrations of NA (10 mM), or by a combination of low temperature (25 degrees C) and one of the other modulating agents. From this strain, we have isolated a second mutant (SK180) that showed constitutive synthesis of the virulence factors under any growth regime. Nucleotide (nt) and deduced amino acid (aa) sequence analysis showed that SK170 contains a substitution at aa570 of BvgS and SK180 contains an additional substitution at aa680. These substitutions are confined to a 161-aa sequence that links the transmembrane (TM) and kinase domains of BvgS. These mutations also alter the transcriptional autoregulation of the P1 and P2 promoters of the bvg locus. P1, which in the wild-type (wt) strain is repressed by modulating agents, is constitutively active in the mutant strains. On the contrary, P2, which is normally induced by all three modulating agents, is active in strain SK170 only in the presence of MgSO4 or NA, while in strain SK180 this promoter is repressed by modulating agents. The mutants exhibit elevated levels of the BvgA regulatory protein and have a virulent phenotype also in the presence of modulating agents.

Published

1994

2. Differential binding of BvgA to two classes of virulence genes of Bordetella pertussis directs promoter selectivity by RNA polymerase

Author

Riccardo Manetti, Rino Rappuoli, Tao Zu, Vincenzo Scarlato, Zu T., Manetti R., Rappuoli R., and Scarlato V.

Subjects

Bordetella pertussis, DNA Footprinting, Microbiology, EMSA, chemistry.chemical_compound, Bacterial Proteins, Transcription (biology), RNA polymerase, Transcriptional regulation, Deoxyribonuclease I, Virulence Factors, Bordetella, Binding site, Adhesins, Bacterial, Promoter Regions, Genetic, Molecular Biology, Gene, biology, virulence gene, BvgAS protein, Escherichia coli Proteins, Promoter, DNA-Directed RNA Polymerases, biology.organism_classification, Molecular biology, DNA-Binding Proteins, Hemagglutinins, Pertussis Toxin, chemistry, DNA, Transcription Factors

Abstract

Transcription of virulence genes of Bordetella pertussis is co-ordinately regulated by the BvgA and BvgS proteins, which are members of the two-component family of bacterial signal-transduction proteins. BvgS is the transmembrane sensor and BvgA the transcriptional regulator. By gel mobility shift assays we demonstrate that phosphorylated BvgA (BvgA approximately P) forms distinct complexes with the filamentous haemagglutinin (PFHA) promoter DNA at different BvgA approximately P: DNA ratios. DNase I protection analyses show that phosphorylation of BvgA not only enhances affinity of the protein for the binding sites of the PFHA and bvgP1 promoters, but it extends significantly the bound region towards position -35 of these promoters. Conversely, a 10-fold higher amount of BvgA approximately P is required for binding to a large DNA region, from -168 to -60, of the pertussis toxin (Ptox) promoter sequence. These findings suggest that the molecular interaction of BvgA approximately P with the Ptox promoter is different from its interaction with the PFHA and bvgP1 promoters. The sigma 70 Escherichia coli RNA polymerase (RNP) does not bind to the bvg-regulated promoters. However, following the formation of a BvgA approximately P-promoter complex, the E. coli RNP specifically recognizes and binds to the bvg-regulated promoters. Thus, BvgA approximately P exerts its action at the level of promoter recognition by directing promoter selectivity by RNP.

Published

1996

3. A novel chromatin‐forming histone H1 homologue is encoded by a dispensable and growth‐regulated gene in Bordetella pertussis

Author

Riccardo Manetti, Anna Prugnola, Sophie Goyard, Stefano Ricci, Agnes Ullmann, Patrizia Polverino-De-Laureto, Rino Rappuoli, Vincenzo Scarlato, Beatrice Aricò, Roberto Manetti, Scarlato V., Arico B., Goyard S., Ricci S., Manetti R., Prugnola A., Polverino-De-Laureto P., Ullmann A., and Rappuoli R.

Subjects

DNA, Bacterial, Transcription, Genetic, Molecular Sequence Data, Regulatory Sequences, Nucleic Acid, SAP30, Microbiology, Bordetella pertussis, Histones, DNA replication factor CDT1, Bacterial Proteins, Histone H1, Kanamycin, histone-like protein, Consensus Sequence, Histone H2A, Deoxyribonuclease I, Amino Acid Sequence, supercoil DNA, Molecular Biology, Base Sequence, Sequence Homology, Amino Acid, biology, DNA, Superhelical, Single-Strand Specific DNA and RNA Endonucleases, DNA replication, Nuclear Proteins, Gene Expression Regulation, Bacterial, Biological Evolution, Molecular biology, Chromatin, Histone, biology.protein, DNA supercoil, Sequence Analysis

Abstract

We report the Identification of a protein homologous to a histone H1 in Bordetella pertussis. The B. pertussis histone homologue, BpH1, varies in size in different strains from 182 to 206 amino acids. The variability of the size of the protein is due to gene variability by insertion or deletion of DNA modules. Insertion of a kanamycin cassette into the bpH1 gene generates a BpH1 null mutant with phenotypic properties and growth rate similar to those of the wild‐type strain, showing that this gene is dispensable. In vitro, the BpH1 protein prevents chromosomal DNA degradation from DNase I and constrains supercoiled DNA. Transcription of the bpH1 gene is activated during exponential growth of the bacteria, whereas It is repressed during the stationary phase of growth, It is proposed that BpH1 plays a role in chromatin formation and condensation during DNA replication and that repression of transcription depends upon a reduced rate of DNA replication. Copyright © 1995, Wiley Blackwell. All rights reserved

Published

1995

4. Response of the bvg regulon of Bordetella pertussis to different temperatures and short-term temperature shifts

Author

Anna Prugnola, Rino Rappuoli, Vincenzo Scarlato, Riccardo Manetti, Beatrice Aricò, Prugnola A., Ario B., Manetti R., Rappuoli R., and Scarlato V.

Subjects

Bordetella pertussis, Bordetella pertussi, Environmental regulation, Hot Temperature, Time Factors, Blotting, Western, DNA Footprinting, Virulence, Biology, Regulon, Microbiology, Thermoregulation, Bacterial Proteins, Transcription (biology), Gene expression, bvg locu, Promoter, Gene Expression Regulation, Bacterial, Haemolysis, biology.organism_classification, Molecular biology, Adenylate Cyclase Toxin, Virulence genes, Cell Division, Transcription Factors

Abstract

Summary: Bordetella pertussis produces a number of virulence factors whose expression is coordinately regulated by the bvgAS locus. Transcription of virulence genes is repressed by environmental factors such as low temperature (25°C) and chemical stimuli. Temperature shift of bacterial cultures from 25°C to 37°C activates two classes of bvg-regulated virulence genes: the early genes, which are activated within 10 min, and late genes, which require 2-4 h for activation. During the interval between the activation of the early and late genes, the intracellular concentration of BvgA increases 50-fold. It has been proposed that this increased concentration may be required for the activation of the late genes. Here we have analysed the response of the bvg locus to intermediate temperatures and to repeated temperature shifts. Temperature shifts of B. pertussis cultures from 22°C to 28°C, 32°C or 35°C resulted in the synthesis of low, intermediate, and high amounts of BvgA. This implied that the intracellular concentration of BvgA is temperature-dependent. We have also observed that the amount of virulence factors produced correlates with the BvgA concentration. When bacteria grown at 37°C were shifted to 22 °C, transcription from the adenylate cyclase toxin haemolysis promoter (PAC) was repressed after 30 min, while transcription from the bvg (P1) and filamentous haemagglutinin (PFHA) promoters was repressed after 2 h. During this time, the amount of BvgA did not decrease. A subsequent temperature shift from 22°C to 37°C induced transcription from the P, and PFHA promoters after 10 min and transcription from the PAC promoter after 20 min. This result shows that in the presence of a high concentration of BvgA, the time lag between temperature shift and late promoter transcription is reduced from 2-4 h to 20 min. The above data support the proposal that the concentration of BvgA plays a role in activating expression of the late genes.

Published

1995