Your search keyword '"G. Grandi"' showing total 21 results

1. nprR1 and nprR2 regulatory regions for neutral protease expression in Bacillus subtilis

Author

M. Del Bue, Salvatore Toma, A Pirola, and G. Grandi

Subjects

Base Sequence, Transcription, Genetic, biology, Nucleic acid sequence, Chromosome Mapping, Promoter, Bacillus subtilis, biology.organism_classification, Microbiology, Molecular biology, Gene Expression Regulation, Start codon, Transcription (biology), Regulatory sequence, Endopeptidases, Genes, Regulator, Gene expression, Neprilysin, RNA, Messenger, Cloning, Molecular, Promoter Regions, Genetic, Molecular Biology, Gene, Research Article

Abstract

The gene coding for the Bacillus subtilis extracellular neutral protease was isolated from strain BGSC 1A341, an overproducer carrying the nprR2 region, and from strain 168, a normal producer with the nprR1 sequence. The sequence of about 600 nucleotides upstream from the start codon of the protease gene was determined for both strains. The two regions are highly homologous except for a stretch of 66 base pairs close to the promoter region, which is absent in the BGSC 1A341 gene. Northern blot analysis of the in vivo RNAs indicated that the different levels of enzyme secreted by the two strains were due to different amounts of transcripts that accumulated in the cells. Furthermore, at the end of exponential growth, the amount of transcript increased dramatically in the overproducer strain but remained approximately constant in the normal producer strain. The start point(s) for transcription, however, as determined by S1 nuclease mapping of the in vivo transcripts, appeared to be the same for both genes.

Published

1986

2. Auto-Assembling Detoxified Staphylococcus aureus Alpha-Hemolysin Mimicking the Wild-Type Cytolytic Toxin.

Author

Fiaschi L, Di Palo B, Scarselli M, Pozzi C, Tomaszewski K, Galletti B, Nardi-Dei V, Arcidiacono L, Mishra RP, Mori E, Pallaoro M, Falugi F, Torre A, Fontana MR, Soriani M, Bubeck Wardenburg J, Grandi G, Rappuoli R, Ferlenghi I, and Bagnoli F

Subjects

ADAM10 Protein metabolism, Animals, Bacterial Toxins administration & dosage, Bacterial Toxins genetics, Cell Line, Cytotoxins, Epitopes immunology, Escherichia coli genetics, Hemolysin Proteins administration & dosage, Hemolysin Proteins genetics, Humans, Membrane Proteins metabolism, Mice, Microscopy, Electron, Transmission, Models, Molecular, Protein Engineering, Recombinant Proteins administration & dosage, Recombinant Proteins genetics, Recombinant Proteins immunology, Recombinant Proteins isolation & purification, Staphylococcal Vaccines immunology, Vaccination, Bacterial Toxins chemistry, Bacterial Toxins immunology, Hemolysin Proteins chemistry, Hemolysin Proteins immunology, Molecular Mimicry, Staphylococcal Infections prevention & control, Staphylococcus aureus chemistry, Staphylococcus aureus metabolism

Abstract

Staphylococcus aureus alpha-hemolysin (Hla) assembles into heptameric pores on the host cell membrane, causing lysis, apoptosis, and junction disruption. Herein, we present the design of a newly engineered S. aureus alpha-toxin, HlaPSGS, which lacks the predicted membrane-spanning stem domain. This protein is able to form heptamers in aqueous solution in the absence of lipophilic substrata, and its structure, obtained by transmission electron microscopy and single-particle reconstruction analysis, resembles the cap of the wild-type cytolytic Hla pore. HlaPSGS was found to be impaired in binding to host cells and to its receptor ADAM10 and to lack hemolytic and cytotoxic activity. Immunological studies using human sera as well as sera from mice convalescent from S. aureus infection suggested that the heptameric conformation of HlaPSGS mimics epitopes exposed by the cytolytic Hla pore during infection. Finally, immunization with this newly engineered Hla generated high protective immunity against staphylococcal infection in mice. Overall, this study provides unprecedented data on the natural immune response against Hla and suggests that the heptameric HlaPSGS is a highly valuable vaccine candidate against S. aureus., (Copyright © 2016 Fiaschi et al.)

Published

2016

3. Four-component Staphylococcus aureus vaccine 4C-staph enhances Fcγ receptor expression in neutrophils and monocytes and mitigates S. aureus infection in neutropenic mice.

Author

Torre A, Bacconi M, Sammicheli C, Galletti B, Laera D, Fontana MR, Grandi G, De Gregorio E, Bagnoli F, Nuti S, Bertholet S, and Bensi G

Subjects

Animals, Antibodies, Bacterial immunology, Disease Models, Animal, Female, Humans, Immunization, Mice, Mice, Inbred C57BL, Neutropenia genetics, Neutropenia microbiology, Receptors, IgG immunology, Staphylococcal Infections genetics, Staphylococcal Infections microbiology, Staphylococcal Vaccines administration & dosage, Staphylococcal Vaccines genetics, Staphylococcus aureus genetics, Monocytes immunology, Neutropenia immunology, Neutrophils immunology, Receptors, IgG genetics, Staphylococcal Infections immunology, Staphylococcal Vaccines immunology, Staphylococcus aureus immunology

Abstract

Staphylococcus aureus is a human bacterial pathogen causing a variety of diseases. The occurrence of multidrug-resistant strains of Staphylococcus aureus underlines the need for a vaccine. Defining immune correlates of protection may support the design of an effective vaccine. We used a murine Staphylococcus aureus infection model, in which bacteria were inoculated in an air pouch generated on the back of the animal. Analysis of the air-pouch content in mice immunized or not with an adjuvanted multiantigen vaccine formulation, four-component S. aureus vaccine (4C-Staph), prior to infection allowed us to measure bacteria, cytokines, and 4C-Staph-specific antibodies and to analyze host immune cells recruited to the infection site. Immunization with 4C-Staph resulted in accumulation of antigen-specific antibodies in the pouch and mitigated the infection. Neutrophils were the most abundant cells in the pouch, and they showed the upregulation of Fcγ receptor (FcγR) following immunization with 4C-Staph. Reduction of the infection was also obtained in mice immunized with 4C-Staph and depleted of neutrophils; these mice showed an increase in monocytes and macrophages. Upregulation of the FcγR and the presence of antigen-specific antibodies induced by immunization with 4C-Staph may contribute to increase bacterial opsonophagocytosis. Protection in neutropenic mice indicated that an effective vaccine could activate alternative protection mechanisms compensating for neutropenia, a condition often occurring in S. aureus-infected patients., (Copyright © 2015, American Society for Microbiology. All Rights Reserved.)

Published

2015

4. SpyAD, a moonlighting protein of group A Streptococcus contributing to bacterial division and host cell adhesion.

Author

Gallotta M, Gancitano G, Pietrocola G, Mora M, Pezzicoli A, Tuscano G, Chiarot E, Nardi-Dei V, Taddei AR, Rindi S, Speziale P, Soriani M, Grandi G, Margarit I, and Bensi G

Subjects

Antigens, Bacterial, Bacterial Proteins genetics, Cell Line, Cloning, Molecular, Cytoskeletal Proteins genetics, Cytoskeletal Proteins metabolism, Epithelial Cells microbiology, Gene Deletion, Humans, Lactococcus lactis metabolism, Protein Binding, Streptococcus pyogenes cytology, Streptococcus pyogenes genetics, Bacterial Adhesion physiology, Bacterial Proteins metabolism, Gene Expression Regulation, Bacterial immunology, Streptococcus pyogenes metabolism

Abstract

Group A streptococcus (GAS) is a human pathogen causing a wide repertoire of mild and severe diseases for which no vaccine is yet available. We recently reported the identification of three protein antigens that in combination conferred wide protection against GAS infection in mice. Here we focused our attention on the characterization of one of these three antigens, Spy0269, a highly conserved, surface-exposed, and immunogenic protein of unknown function. Deletion of the spy0269 gene in a GAS M1 isolate resulted in very long bacterial chains, which is indicative of an impaired capacity of the knockout mutant to properly divide. Confocal microscopy and immunoprecipitation experiments demonstrated that the protein was mainly localized at the cell septum and could interact in vitro with the cell division protein FtsZ, leading us to hypothesize that Spy0269 is a member of the GAS divisome machinery. Predicted structural domains and sequence homologies with known streptococcal adhesins suggested that this antigen could also play a role in mediating GAS interaction with host cells. This hypothesis was confirmed by showing that recombinant Spy0269 could bind to mammalian epithelial cells in vitro and that Lactococcus lactis expressing Spy0269 on its cell surface could adhere to mammalian cells in vitro and to mice nasal mucosa in vivo. On the basis of these data, we believe that Spy0269 is involved both in bacterial cell division and in adhesion to host cells and we propose to rename this multifunctional moonlighting protein as SpyAD (Streptococcus pyogenes Adhesion and Division protein)., (Copyright © 2014, American Society for Microbiology. All Rights Reserved.)

Published

2014

5. Analysis of two-component systems in group B Streptococcus shows that RgfAC and the novel FspSR modulate virulence and bacterial fitness.

Author

Faralla C, Metruccio MM, De Chiara M, Mu R, Patras KA, Muzzi A, Grandi G, Margarit I, Doran KS, and Janulczyk R

Subjects

Animals, Bacterial Proteins chemistry, Carbon metabolism, Cluster Analysis, Disease Models, Animal, Female, Gene Expression Profiling, Gene Expression Regulation, Bacterial, Genomics, Mice, Mutation, Phenotype, Protein Interaction Domains and Motifs, Streptococcal Infections microbiology, Streptococcus agalactiae pathogenicity, Transcription, Genetic, Vagina microbiology, Virulence genetics, Bacterial Proteins genetics, Bacterial Proteins metabolism, Genetic Fitness, Signal Transduction, Streptococcus agalactiae genetics, Streptococcus agalactiae metabolism

Abstract

Unlabelled: Group B Streptococcus (GBS), in the transition from commensal organisms to pathogens, will encounter diverse host environments and, thus, require coordinated control of the transcriptional responses to these changes. This work was aimed at better understanding the role of two-component signal transduction systems (TCS) in GBS pathophysiology through a systematic screening procedure. We first performed a complete inventory and sensory mechanism classification of all putative GBS TCS by genomic analysis. Five TCS were further investigated by the generation of knockout strains, and in vitro transcriptome analysis identified genes regulated by these systems, ranging from 0.1% to 3% of the genome. Interestingly, two sugar phosphotransferase systems appeared to be differentially regulated in the TCS-16 knockout strain (TCS loci were numbered in order of their appearance on the chromosome), suggesting an involvement in monitoring carbon source availability. High-throughput analysis of bacterial growth on different carbon sources showed that TCS-16 was necessary for the growth of GBS on fructose-6-phosphate. Additional transcriptional analysis provided further evidence for a stimulus-response circuit where extracellular fructose-6-phosphate leads to autoinduction of TCS-16, with concomitant dramatic upregulation of the adjacent operon, which encodes a phosphotransferase system. The TCS-16-deficient strain exhibited decreased persistence in a model of vaginal colonization. All mutant strains were also characterized in a murine model of systemic infection, and inactivation of TCS-17 (also known as RgfAC) resulted in hypervirulence. Our data suggest a role for the previously unknown TCS-16, here named FspSR, in bacterial fitness and carbon metabolism during host colonization, and the data also provide experimental evidence for TCS-17/RgfAC involvement in virulence., Importance: Two-component systems have been evolved by bacteria to detect environmental changes, and they play key roles in pathogenicity. A comprehensive analysis of TCS in GBS has not been performed previously. In this work, we classify 21 TCS and present evidence for the involvement of two specific TCS in GBS virulence and colonization in vivo. Although pinpointing specific TCS stimuli is notoriously difficult, we used a combination of techniques to identify two systems with different effects on GBS pathogenesis. For one of the systems, we propose that fructose-6-phosphate, a metabolite in glycolysis, is sufficient to induce a regulatory response involving a sugar transport system. Our catalogue and classification of TCS may guide further studies into the role of TCS in GBS pathogenicity and biology., (Copyright © 2014 Faralla et al.)

Published

2014

6. Targeted amino acid substitutions impair streptolysin O toxicity and group A Streptococcus virulence.

Author

Chiarot E, Faralla C, Chiappini N, Tuscano G, Falugi F, Gambellini G, Taddei A, Capo S, Cartocci E, Veggi D, Corrado A, Mangiavacchi S, Tavarini S, Scarselli M, Janulczyk R, Grandi G, Margarit I, and Bensi G

Subjects

Animals, Antibodies, Bacterial blood, Antitoxins blood, Bacterial Proteins genetics, Bacterial Proteins immunology, Bacterial Proteins toxicity, Disease Models, Animal, Mice, Models, Molecular, Mutant Proteins genetics, Mutant Proteins immunology, Mutant Proteins toxicity, Streptococcal Infections immunology, Streptococcal Infections microbiology, Streptococcal Infections pathology, Streptococcal Infections prevention & control, Streptococcus pyogenes genetics, Streptococcus pyogenes immunology, Streptolysins immunology, Survival Analysis, Virulence, Virulence Factors immunology, Amino Acid Substitution, Streptococcus pyogenes pathogenicity, Streptolysins genetics, Streptolysins toxicity, Virulence Factors genetics, Virulence Factors toxicity

Abstract

Unlabelled: Streptolysin O is a potent pore-forming toxin produced by group A Streptococcus. The aims of the present study were to dissect the relative contributions of different structural domains of the protein to hemolytic activity, to obtain a detoxified form of streptolysin O amenable to human vaccine formulation, and to investigate the role of streptolysin O-specific antibodies in protection against group A Streptococcus infection. On the basis of in silico structural predictions, we introduced two amino acid substitutions, one in the proline-rich domain 1 and the other in the conserved undecapeptide loop in domain 4. The resulting streptolysin O derivative showed no toxicity, was highly impaired in binding to eukaryotic cells, and was unable to form organized oligomeric structures on the cell surface. However, it was fully capable of conferring consistent protection in a murine model of group A Streptococcus infection. When we engineered a streptococcal strain to express the double-mutated streptolysin O, a drastic reduction in virulence as well as a diminished capacity to kill immune cells recruited at the infection site was observed. Furthermore, when mice immunized with the toxoid were challenged with the wild-type and mutant strains, protection only against the wild-type strain, not against the strain expressing the double-mutated streptolysin O, was obtained. We conclude that protection occurs by antibody-mediated neutralization of active toxin., Importance: We present a novel example of structural design of a vaccine antigen optimized for human vaccine use. Having previously demonstrated that immunization of mice with streptolysin O elicits a protective immune response against infection with group A Streptococcus strains of different serotypes, we developed in this study a double-mutated nontoxic derivative that represents a novel tool for the development of protective vaccine formulations against this important human pathogen. Furthermore, the innovative construction of an isogenic strain expressing a functionally inactive toxin and its use in infection and opsonophagocytosis experiments allowed us to investigate the mechanism by which streptolysin O mediates protection against group A Streptococcus. Finally, the ability of this toxin to directly attack and kill host immune cells during infection was studied in an air pouch model, which allowed parallel quantification of cellular recruitment, vitality, and cytokine release at the infection site.

Published

2013

7. Simple sequence repeats and genome plasticity in Streptococcus agalactiae.

Author

Janulczyk R, Masignani V, Maione D, Tettelin H, Grandi G, and Telford JL

Subjects

Base Sequence, DNA, Bacterial genetics, Genetic Variation, Genome, Bacterial, Repetitive Sequences, Nucleic Acid genetics, Streptococcus agalactiae genetics

Abstract

Simple sequence repeats (SSRs) and their role in phase variation have been extensively studied in Gram-negative organisms, where they have been associated with antigenic variation and other adaptation strategies. In this study, we apply comparative genomics in order to find evidence of slipped-strand mispairing in the human Gram-positive pathogen Streptococcus agalactiae. In two consecutive screenings, 2,233 (650 + 1,583) SSRs were identified in our reference genome 2603V/R, and these loci were examined in seven other S. agalactiae genomes. A total of 56 SSR loci were found to exhibit variation, where gain or loss of repeat units was observed in at least one other genome, resulting in aberrant genotypes. Homopolymeric adenine tracts predominated among the repeats that varied. Positional analysis revealed that long polyadenine tracts were overrepresented in the 5' ends of open reading frames (ORFs) and underrepresented in the 3' ends. Repeat clustering in ORFs was also examined, and the highest degree of clustering was observed for a capsule biosynthesis gene and a pilus sortase. A statistical analysis of observed over expected ratios suggested a selective pressure against long homopolymeric tracts. Altered phenotypes were verified for three genes encoding surface-attached proteins, in which frameshifts or fusions led to truncation of proteins and/or affected surface localization through loss or gain of the cell wall sorting signal. The data suggest that SSRs contributes to genome plasticity in S. agalactiae but that the bet-hedging strategy is different from Gram-negative organisms.

Published

2010

8. CsrRS regulates group B Streptococcus virulence gene expression in response to environmental pH: a new perspective on vaccine development.

Author

Santi I, Grifantini R, Jiang SM, Brettoni C, Grandi G, Wessels MR, and Soriani M

Subjects

Acids pharmacology, Anti-Bacterial Agents pharmacology, Bacterial Proteins genetics, Gene Deletion, Gene Expression Profiling, Hydrogen-Ion Concentration, Protein Kinases genetics, Streptococcus agalactiae drug effects, Streptococcus agalactiae immunology, Stress, Physiological, Virulence Factors immunology, Bacterial Proteins physiology, Gene Expression Regulation, Bacterial, Protein Kinases physiology, Streptococcal Vaccines immunology, Streptococcus agalactiae physiology, Virulence Factors biosynthesis

Abstract

To identify factors involved in the response of group B streptococci (GBS) to environmental pH, we performed a comparative global gene expression analysis of GBS at acidic and neutral pHs. We found that the transcription of 317 genes was increased at pH 5.5 relative to that at pH 7.0, while 61 genes were downregulated. The global response to acid stress included the differential expression of genes involved in transport, metabolism, stress response, and virulence. Known vaccine candidates, such as BibA and pilus components, were also regulated by pH. We observed that many of the genes involved in the GBS response to pH are known to be controlled by the CsrRS two-component system. Comparison of the regulon of wild-type strain 2603 V/R with that of a csrRS deletion mutant strain revealed that the pH-dependent regulation of 90% of the downregulated genes and 59.3% of the up-regulated genes in strain 2603 V/R was CsrRS dependent and that many virulence factors were overexpressed at high pH. Beta-hemolysin regulation was abrogated by selective inactivation of csrS, suggesting the implication of the CsrS protein in pH sensing. These results imply that the translocation of GBS from the acidic milieu of the vagina to the neutral pH of the neonatal lung signals the up-regulation of GBS virulence factors and conversion from a colonizing to an invasive phenotype. In addition, the fact that increased exposure of BibA on the bacterial surface at pH 7.0 induced opsonophagocytic killing of GBS in immune serum highlights the importance of pH regulation in the protective efficacy of specific antibodies to surface-exposed GBS proteins.

Published

2009

9. CT043, a protective antigen that induces a CD4+ Th1 response during Chlamydia trachomatis infection in mice and humans.

Author

Meoni E, Faenzi E, Frigimelica E, Zedda L, Skibinski D, Giovinazzi S, Bonci A, Petracca R, Bartolini E, Galli G, Agnusdei M, Nardelli F, Buricchi F, Norais N, Ferlenghi I, Donati M, Cevenini R, Finco O, Grandi G, and Grifantini R

Subjects

Animals, Bacterial Vaccines immunology, Chlamydia muridarum immunology, Female, Genital Diseases, Female immunology, Humans, Immunization, Interferon-gamma biosynthesis, Mice, Mice, Inbred BALB C, Porins immunology, Antigens, Bacterial immunology, Chlamydia Infections immunology, Chlamydia trachomatis immunology, Th1 Cells immunology

Abstract

Despite several decades of intensive studies, no vaccines against Chlamydia trachomatis, an intracellular pathogen causing serious ocular and urogenital diseases, are available yet. Infection-induced immunity in both animal models and humans strongly supports the notion that for a vaccine to be effective a strong CD4(+) Th1 immune response should be induced. In the course of our vaccine screening program based on the selection of chlamydial proteins eliciting cell-mediated immunity, we have found that CT043, a protein annotated as hypothetical, induces CD4(+) Th1 cells both in chlamydia-infected mice and in human patients with diagnosed C. trachomatis genital infection. DNA priming/protein boost immunization with CT043 results in a 2.6-log inclusion-forming unit reduction in the murine lung infection model. Sequence analysis of CT043 from C. trachomatis human isolates belonging to the most representative genital serovars revealed a high degree of conservation, suggesting that this antigen could provide cross-serotype protection. Therefore, CT043 is a promising vaccine candidate against C. trachomatis infection.

Published

2009

10. Group B streptococcus pullulanase crystal structures in the context of a novel strategy for vaccine development.

Author

Gourlay LJ, Santi I, Pezzicoli A, Grandi G, Soriani M, and Bolognesi M

Subjects

Bacterial Vaccines, Calcium metabolism, Cell Line, Tumor, Chlorides metabolism, Epithelial Cells metabolism, Glycoside Hydrolases genetics, Humans, Hydrogen Bonding, Microscopy, Confocal, Microscopy, Fluorescence, Protein Binding physiology, Protein Structure, Tertiary, Streptococcal Infections prevention & control, Crystallography, X-Ray methods, Glycoside Hydrolases chemistry, Glycoside Hydrolases metabolism, Models, Molecular, Streptococcus agalactiae metabolism

Abstract

The group B streptococcus type I pullulanase (SAP) is a class 13 glycoside hydrolase that is anchored to the bacterial cell surface via a conserved C-terminal anchoring motif and involved in alpha-glucan degradation. Recent in vitro functional studies have shown that SAP is immunogenic in humans and that anti-SAP sera derived from immunized animals impair both group A and group B streptococcus pullulanase activities, suggesting that in vivo immunization with this antigen could prevent streptococcal colonization. To further investigate the putative role of SAP in bacterial pathogenesis, we carried out functional studies and found that recombinant SAP binds to human cervical epithelial cells. Furthermore, with a view of using SAP as a vaccine candidate, we present high-resolution crystal structure analyses of an N-terminally truncated form of SAP lacking the carbohydrate binding module but containing the catalytic domain and displaying glycosidase hydrolase activity, both in its apo form and in complex with maltotetraose, at resolutions of 2.1 and 2.4 A, respectively.

Published

2009

11. Sortase A utilizes an ancillary protein anchor for efficient cell wall anchoring of pili in Streptococcus agalactiae.

Author

Nobbs AH, Rosini R, Rinaudo CD, Maione D, Grandi G, and Telford JL

Subjects

Bacterial Proteins genetics, Gene Deletion, Gene Order, Multigene Family, Streptococcus agalactiae genetics, Aminoacyltransferases genetics, Aminoacyltransferases metabolism, Bacterial Proteins metabolism, Cell Wall metabolism, Cysteine Endopeptidases genetics, Cysteine Endopeptidases metabolism, Fimbriae, Bacterial metabolism, Streptococcus agalactiae physiology

Abstract

Pili are putative virulence factors and promising vaccine candidates in Streptococcus agalactiae (group B Streptococcus [GBS]) infection, a leading cause of neonatal sepsis and meningitis. The genes necessary for pilus synthesis and assembly are clustered in pilus islands (PI). Each gene encodes three structural subunits (a backbone and two ancillary proteins) bearing a C-terminal LPXTG motif and two subfamily C sortases (SrtC) involved in covalent polymerization of the subunits. GBS strains also possess the conserved "housekeeping" sortase A (SrtA), but its role in pilus assembly is unclear. To address this issue, pilus expression and cell wall anchoring were analyzed in srtA deletion mutants. Loss of SrtA did not affect pilus polymerization. However, pilus expression on the cell surface was reduced, and pili accumulated in the culture supernatant. Furthermore, cell-associated pili could be readily released by detergent treatment, indicating that SrtA is involved in covalent anchoring of pili to the cell wall. When each of the genes comprising PI-2a was systematically deleted, only the absence of ancillary subunit GBS150 or the SrtC required for incorporation of GBS150 into pili mimicked the srtA mutant phenotype. Thus, from these data a model for GBS pilus assembly can be proposed in which PI sortases are responsible for polymerization of the pilus structure, while SrtA is required to covalently attach it to the cell wall, utilizing ancillary pilus subunit GBS150 as the anchor protein.

Published

2008

12. A chemokine-degrading extracellular protease made by group A Streptococcus alters pathogenesis by enhancing evasion of the innate immune response.

Author

Sumby P, Zhang S, Whitney AR, Falugi F, Grandi G, Graviss EA, Deleo FR, and Musser JM

Subjects

Animals, Bacterial Proteins metabolism, Cell Wall chemistry, DNA, Bacterial metabolism, Female, Gene Deletion, Gene Expression Profiling, Gene Expression Regulation, Bacterial, Humans, Mice, Neutrophil Activation, Neutrophils immunology, Peptide Hydrolases genetics, Promoter Regions, Genetic, Protein Binding, Repressor Proteins metabolism, Streptococcal Infections microbiology, Streptococcus pyogenes genetics, Streptococcus pyogenes pathogenicity, Virulence, Virulence Factors genetics, Chemokine CXCL1 metabolism, Chemokine CXCL6 metabolism, Peptide Hydrolases metabolism, Streptococcus pyogenes enzymology, Streptococcus pyogenes immunology, Virulence Factors metabolism

Abstract

Circumvention of the host innate immune response is critical for bacterial pathogens to infect and cause disease. Here we demonstrate that the group A Streptococcus (GAS; Streptococcus pyogenes) protease SpyCEP (S. pyogenes cell envelope protease) cleaves granulocyte chemotactic protein 2 (GCP-2) and growth-related oncogene alpha (GROalpha), two potent chemokines made abundantly in human tonsils. Cleavage of GCP-2 and GROalpha by SpyCEP abrogated their abilities to prime neutrophils for activation, detrimentally altering the innate immune response. SpyCEP expression is negatively regulated by the signal transduction system CovR/S. Purified recombinant CovR bound the spyCEP gene promoter region in vitro, indicating direct regulation. Immunoreactive SpyCEP protein was present in the culture supernatants of covR/S mutant GAS strains but not in supernatants from wild-type strains. However, wild-type GAS strains do express SpyCEP, where it is localized to the cell wall. Strain MGAS2221, an organism representative of the highly virulent and globally disseminated M1T1 GAS clone, differed significantly from its isogenic spyCEP mutant derivative strain in a mouse soft tissue infection model. Interestingly, and in contrast to previous studies, the isogenic mutant strain generated lesions of larger size than those formed following infection with the parent strain. The data indicate that SpyCEP contributes to GAS virulence in a strain- and disease-dependent manner.

Published

2008

13. Transcriptional and proteomic profiles of group B Streptococcus type V reveal potential adherence proteins associated with high-level invasion.

Author

Johri AK, Margarit I, Broenstrup M, Brettoni C, Hua L, Gygi SP, Telford JL, Grandi G, and Paoletti LC

Subjects

Cell Line, Tumor, Female, Gene Expression Profiling, Humans, Proteome metabolism, Streptococcus pyogenes genetics, Streptococcus pyogenes metabolism, Bacterial Adhesion genetics, Bacterial Adhesion immunology, Gene Expression Regulation, Bacterial immunology, Proteome genetics, Streptococcus pyogenes classification, Streptococcus pyogenes pathogenicity

Abstract

Group B Streptococcus (GBS) is an opportunistic organism that can harmlessly colonize the human gut, vagina, and rectum but can also cause pneumonia, sepsis, and meningitis in neonates born to colonized mothers. We have shown previously that growth rate and oxygen level regulate the ability of GBS to invade eukaryotic cells in vitro. Herein we extend and expand on these observations to show that GBS type V, an emergent serotype, grown in a chemostat at a cell mass-doubling time (t(d)) of 1.8 h with oxygen invaded human ME-180 cervical epithelial cells in large numbers compared with those grown at the same t(d) without oxygen or at a slower t(d) of 11.0 h. The fact that several GBS type V cell wall-associated and membrane proteins were expressed exclusively under the invasive growth condition prompted an investigation, using genomics and proteomics, of all upregulated genes and proteins. Several proteins with potential roles in adherence were identified, including an undefined surface antigen (SAG1350), a lipoprotein (SAG0971), penicillin-binding protein 2b (SAG0765), glyceraldehyde-3-phosphate dehydrogenase (SAG0823), and an iron-binding protein (SAG1007). Mouse antisera to these five proteins inhibited binding of GBS type V to ME-180 cells by > or =85%. Recombinant undefined surface antigen (SAG1350), lipoprotein (SAG0971), and penicillin-binding protein 2b (SAG0765) each bound to ME-180 cells in a dose-dependent fashion, confirming their ability to act as ligands. Collectively, these data increase the number of potential GBS adherence factors and also suggest a role for these surface-associated proteins in initial pathogenic events.

Published

2007

14. Combined conjugate vaccines: enhanced immunogenicity with the N19 polyepitope as a carrier protein.

Author

Baraldo K, Mori E, Bartoloni A, Norelli F, Grandi G, Rappuoli R, Finco O, and Del Giudice G

Subjects

Adjuvants, Immunologic administration & dosage, Animals, Antibodies, Bacterial biosynthesis, Antibody Affinity, Bacterial Infections immunology, Bacterial Infections prevention & control, Bacterial Proteins administration & dosage, Bacterial Proteins immunology, Bacterial Proteins metabolism, Bacterial Vaccines administration & dosage, Bacterial Vaccines metabolism, Carrier Proteins administration & dosage, Epitopes, T-Lymphocyte administration & dosage, Epitopes, T-Lymphocyte metabolism, Glycoconjugates administration & dosage, Humans, Immunoglobulin G biosynthesis, Mice, Neisseria meningitidis immunology, Vaccines, Combined administration & dosage, Vaccines, Combined immunology, Vaccines, Conjugate administration & dosage, Vaccines, Conjugate immunology, Bacterial Vaccines immunology, Carrier Proteins immunology, Epitopes immunology, Epitopes, T-Lymphocyte immunology, Glycoconjugates immunology

Abstract

The N19 polyepitope, consisting of a sequential string of universal human CD4(+)-T-cell epitopes, was tested as a carrier protein in a formulation of combined glycoconjugate vaccines containing the capsular polysaccharides (PSs) of Neisseria meningitidis serogroups A, C, W-135, and Y. Good antibody responses to all four polysaccharides were induced by one single immunization of mice with N19-based conjugates. Two immunizations with N19 conjugates elicited anti-MenACWY antibody titers comparable to those induced after three doses of glycoconjugates containing CRM197 as carrier protein. Compared to cross-reacting material (CRM)-based constructs, lower amounts of N19-MenACWY conjugates still induced high bactericidal titers to all four PSs. Moreover, N19-MenACWY-conjugated constructs induced faster and higher antibody avidity maturation against meningococcal C PS than CRM-based conjugates. Very importantly, N19-specific antibodies did not cross-react with the parent protein from which N19 epitopes were derived, e.g., tetanus toxoid and influenza virus hemagglutinin. Finally, T helper epitopes of the N19 carrier protein were effectively generated both in vivo (after immunization with the N19 itself) and in vitro (after restimulation of epitope-specific spleen cells). Taken together, these data show that the N19 polyepitope represents a strong and valid option for the generation of improved or new combined glycoconjugate vaccines.

Published

2005

15. N19 polyepitope as a carrier for enhanced immunogenicity and protective efficacy of meningococcal conjugate vaccines.

Author

Baraldo K, Mori E, Bartoloni A, Petracca R, Giannozzi A, Norelli F, Rappuoli R, Grandi G, and Del Giudice G

Subjects

Amino Acid Sequence, Animals, Antibodies, Bacterial blood, Bacterial Proteins immunology, Diphtheria Toxin immunology, Drug Carriers, Epitopes, T-Lymphocyte chemistry, Epitopes, T-Lymphocyte genetics, Epitopes, T-Lymphocyte metabolism, Female, Humans, Meningitis, Meningococcal prevention & control, Meningococcal Vaccines administration & dosage, Mice, Molecular Sequence Data, Recombinant Proteins administration & dosage, Vaccines, Conjugate administration & dosage, CD4-Positive T-Lymphocytes immunology, Epitopes, T-Lymphocyte immunology, Meningococcal Vaccines immunology, Neisseria meningitidis, Serogroup C immunology, Recombinant Proteins immunology, Vaccines, Conjugate immunology

Abstract

N19, a string of human universal CD4 T-cell epitopes from various pathogen-derived antigens, was shown to exert a stronger carrier effect than CRM197 for the induction of anti-group C Neisseria meningitidis capsular polysaccharide (MenC), after immunization of mice with various dosages of N19-MenC or CRM-MenC conjugate vaccines. After two immunizations, the N19-based construct induced anti-MenC antibody and protective bactericidal antibody titers higher than those induced by three doses of the CRM-MenC conjugate and required lower amounts of conjugate. N19-based conjugates are superior to CRM-based conjugates to induce protective immune responses to MenC conjugates.

Published

2004

16. GNA33 of Neisseria meningitidis is a lipoprotein required for cell separation, membrane architecture, and virulence.

Author

Adu-Bobie J, Lupetti P, Brunelli B, Granoff D, Norais N, Ferrari G, Grandi G, Rappuoli R, and Pizza M

Subjects

Animals, Animals, Newborn, Animals, Outbred Strains, Bacteremia microbiology, Bacteremia physiopathology, Cell Membrane ultrastructure, Gene Deletion, Glycosyltransferases chemistry, Glycosyltransferases genetics, Humans, Lipoproteins chemistry, Lipoproteins genetics, Meningococcal Infections microbiology, Meningococcal Infections physiopathology, Microscopy, Electron, Neisseria meningitidis, Serogroup B chemistry, Neisseria meningitidis, Serogroup B metabolism, Rats, Rats, Wistar, Cell Membrane metabolism, Glycosyltransferases metabolism, Lipoproteins metabolism, Neisseria meningitidis, Serogroup B growth & development, Neisseria meningitidis, Serogroup B pathogenicity

Abstract

GNA33 is a membrane-bound lipoprotein with murein hydrolase activity that is present in all Neisseria species and well conserved in different meningococcal isolates. The protein shows 33% identity to a lytic transglycolase (MltA) from Escherichia coli and has been shown to be involved in the degradation of both insoluble murein sacculi and unsubstituted glycan strands. To study the function of the gene and its role in pathogenesis and virulence, a knockout mutant of a Neisseria meningitidis serogroup B strain was generated. The mutant exhibited retarded growth in vitro. Transmission electron microscopy revealed that the mutant grows in clusters which are connected by a continuous outer membrane, suggesting a failure in the separation of daughter cells. Moreover, sodium dodecyl sulfate-polyacrylamide gel electrophoresis analysis of culture supernatant revealed that the mutant releases several proteins in the medium. The five most abundant proteins, identified by matrix-assisted laser desorption ionization-time-of-flight mass spectrometry analysis, belong to the outer membrane protein family. Finally, the mutant showed an attenuated phenotype, since it was not able to cause bacteremia in the infant rat model. We conclude that GNA33 is a highly conserved lipoprotein which plays an important role in peptidoglycan metabolism, cell separation, membrane architecture, and virulence.

Published

2004

17. Genomic approach for analysis of surface proteins in Chlamydia pneumoniae.

Author

Montigiani S, Falugi F, Scarselli M, Finco O, Petracca R, Galli G, Mariani M, Manetti R, Agnusdei M, Cevenini R, Donati M, Nogarotto R, Norais N, Garaguso I, Nuti S, Saletti G, Rosa D, Ratti G, and Grandi G

Subjects

Animals, Antigens, Bacterial genetics, Antigens, Bacterial metabolism, Bacterial Outer Membrane Proteins metabolism, Blotting, Western methods, Female, Flow Cytometry methods, Gene Expression, Humans, Mice, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization methods, Bacterial Outer Membrane Proteins genetics, Chlamydophila pneumoniae genetics, Genome, Bacterial

Abstract

Chlamydia pneumoniae, a human pathogen causing respiratory infections and probably contributing to the development of atherosclerosis and heart disease, is an obligate intracellular parasite which for replication needs to productively interact with and enter human cells. Because of the intrinsic difficulty in working with C. pneumoniae and in the absence of reliable tools for its genetic manipulation, the molecular definition of the chlamydial cell surface is still limited, thus leaving the mechanisms of chlamydial entry largely unknown. In an effort to define the surface protein organization of C. pneumoniae, we have adopted a combined genomic-proteomic approach based on (i) in silico prediction from the available genome sequences of peripherally located proteins, (ii) heterologous expression and purification of selected proteins, (iii) production of mouse immune sera against the recombinant proteins to be used in Western blotting and fluorescence-activated cell sorter (FACS) analyses for the identification of surface antigens, and (iv) mass spectrometry analysis of two-dimensional electrophoresis (2DE) maps of chlamydial protein extracts to confirm the presence of the FACS-positive antigens in the chlamydial cell. Of the 53 FACS-positive sera, 41 recognized a protein species with the expected size on Western blots, and 28 of the 53 antigens shown to be surface-exposed by FACS were identified on 2DE maps of elementary-body extracts. This work represents the first systematic attempt to define surface protein organization in C. pneumoniae.

Published

2002

18. Evaluation of hepatitis C virus glycoprotein E2 for vaccine design: an endoplasmic reticulum-retained recombinant protein is superior to secreted recombinant protein and DNA-based vaccine candidates.

Author

Heile JM, Fong YL, Rosa D, Berger K, Saletti G, Campagnoli S, Bensi G, Capo S, Coates S, Crawford K, Dong C, Wininger M, Baker G, Cousens L, Chien D, Ng P, Archangel P, Grandi G, Houghton M, and Abrignani S

Subjects

Animals, Antigens, CD metabolism, Drug Design, Endoplasmic Reticulum metabolism, Evaluation Studies as Topic, Female, Glycosylation, Guinea Pigs, Hepatitis C Antibodies blood, Humans, Immunization, Mice, Mice, Inbred C57BL, Recombinant Proteins immunology, Recombinant Proteins metabolism, Tetraspanin 28, Viral Envelope Proteins chemistry, Viral Envelope Proteins metabolism, Hepacivirus immunology, Hepatitis C prevention & control, Membrane Proteins, Vaccines, DNA immunology, Viral Envelope Proteins genetics, Viral Envelope Proteins immunology, Viral Hepatitis Vaccines immunology

Abstract

Hepatitis C virus (HCV) is the leading causative agent of blood-borne chronic hepatitis and is the target of intensive vaccine research. The virus genome encodes a number of structural and nonstructural antigens which could be used in a subunit vaccine. The HCV envelope glycoprotein E2 has recently been shown to bind CD81 on human cells and therefore is a prime candidate for inclusion in any such vaccine. The experiments presented here assessed the optimal form of HCV E2 antigen from the perspective of antibody generation. The quality of recombinant E2 protein was evaluated by both the capacity to bind its putative receptor CD81 on human cells and the ability to elicit antibodies that inhibited this binding (NOB antibodies). We show that truncated E2 proteins expressed in mammalian cells bind with high efficiency to human cells and elicit NOB antibodies in guinea pigs only when purified from the core-glycosylated intracellular fraction, whereas the complex-glycosylated secreted fraction does not bind and elicits no NOB antibodies. We also show that carbohydrate moieties are not necessary for E2 binding to human cells and that only the monomeric nonaggregated fraction can bind to CD81. Moreover, comparing recombinant intracellular E2 protein to several E2-encoding DNA vaccines in mice, we found that protein immunization is superior to DNA in both the quantity and quality of the antibody response elicited. Together, our data suggest that to elicit antibodies aimed at blocking HCV binding to CD81 on human cells, the antigen of choice is a mammalian cell-expressed, monomeric E2 protein purified from the intracellular fraction.

Published

2000

19. Structure-function analysis of hepatitis C virus envelope-CD81 binding.

Author

Petracca R, Falugi F, Galli G, Norais N, Rosa D, Campagnoli S, Burgio V, Di Stasio E, Giardina B, Houghton M, Abrignani S, and Grandi G

Subjects

Amino Acid Sequence, Antibody Affinity, Antigens, CD genetics, Cysteine, Disulfides chemistry, Hepacivirus genetics, Humans, Liver cytology, Liver metabolism, Molecular Sequence Data, Recombinant Proteins metabolism, Structure-Activity Relationship, Tetraspanin 28, Tumor Cells, Cultured, Viral Envelope Proteins genetics, Antigens, CD chemistry, Antigens, CD metabolism, Hepacivirus metabolism, Membrane Proteins, Viral Envelope Proteins chemistry, Viral Envelope Proteins metabolism

Abstract

Hepatitis C virus (HCV) is a major human pathogen causing chronic liver disease. We have recently found that the large extracellular loop (LEL) of human CD81 binds HCV. This finding prompted us to assess the structure-function features of HCV-CD81 interaction by using recombinant E2 protein and a recombinant soluble form of CD81 LEL. We have found that HCV-E2 binds CD81 LEL with a K(d) of 1.8 nM; CD81 can mediate attachment of E2 on hepatocytes; engagement of CD81 mediates internalization of only 30% of CD81 molecules even after 12 h; and the four cysteines of CD81 LEL form two disulfide bridges, the integrity of which is necessary for CD81-HCV interaction. Altogether our data suggest that neutralizing antibodies aimed at interfering with HCV binding to human cells should have an affinity higher than 10(-9) M, that HCV binding to hepatocytes may not entirely depend on CD81, that CD81 is an attachment receptor with poor capacity to mediate virus entry, and that reducing environments do not favor CD81-HCV interaction. These studies provide a better understanding of the CD81-HCV interaction and should thus help to elucidate the viral life cycle and to develop new strategies aimed at interfering with HCV binding to human cells.

Published

2000

20. Introduction of unmarked mutations in the Helicobacter pylori vacA gene with a sucrose sensitivity marker.

Author

Copass M, Grandi G, and Rappuoli R

Subjects

Alleles, Bacillus subtilis genetics, Blotting, Western, Chromosome Mapping, Cloning, Molecular, Flagellin genetics, Histidine genetics, Kanamycin Resistance genetics, Mutagenesis, Site-Directed, Polymerase Chain Reaction, Promoter Regions, Genetic, Recombination, Genetic, Sucrose pharmacology, Transformation, Genetic, Cytotoxins genetics, Helicobacter pylori genetics, Mutagenesis, Insertional

Abstract

Research on Helicobacter pylori has been hindered by the lack of useful genetic tools. Using the sacB gene of Bacillus subtilis, we developed a sucrose-based counterselection system that allows introduction of unmarked mutations in H. pylori. A kan-sacB cassette, consisting of the sacB gene expressed from the H. pylori flagellin promoter and the kanamycin resistance module, was introduced by homologous recombination into a target H. pylori gene. The resultant strains were sucrose sensitive and kanamycin resistant. Following transformation with a mutated allele, growth in sucrose-containing medium allowed the selection of strains that had lost the kan-sacB module and had integrated the unmarked allele. We have used this cassette to perform a site-directed modification of two histidine residues encoded by the vacA gene in a two-step procedure. This system should prove useful in the site-directed mutagenesis of H. pylori genes.

Published

1997

21. Naturally occurring macrolide-lincosamide-streptogramin B resistance in Bacillus licheniformis.

Author

Docherty A, Grandi G, Grandi R, Gryczan TJ, Shivakumar AG, and Dubnau D

Subjects

Bacillus genetics, Bacterial Proteins biosynthesis, Cloning, Molecular, Drug Resistance, Microbial, Erythromycin pharmacology, Nucleic Acid Hybridization, Plasmids, Virginiamycin pharmacology, Anti-Bacterial Agents pharmacology, Bacillus drug effects, Genes

Abstract

Resistance to the macrolide-lincosamide-streptogramin B (MLS) group of antibiotics is widespread and of clinical importance. B. Weisblum and his coworkers have demonstrated that this resistance is associated with methylation of the 23S ribosomal ribonucleic acid of the large ribosomal subunit which results in a diminished affinity of this organelle for these antibiotics (Lai et al, J. Mol. Biol. 74:67-72, 1973). We report that 10 of 15 natural isolates of Bacillus licheniformis, a common soil organism, are resistant to the MLS antibiotics. The properties of this resistance (high level of tolerance for erythromycin, broad cross-resistance spectrum, and inducibility) suggest that resistance is conferred as described above. The resistance determinant from one of these strains was cloned onto a B. subtilis plasmid vector, and the resulting hybrid plasmid (pBD90) was used to prepare radioactive probe deoxyribonucleic acid for hybridization studies. All of the resistance B. licheniformis strains studied exhibited homology with the pBD90 insert. Plasmid pBD90 showed no homology to the following staphylococcal and streptococcal MLS-resistance plasmids: pE194, pE5, pAM77, pI258. Plasmids pE194 and pE5, on the other hand, carry homologous MLS genes but showed no detectable homology to one another in their replication genes. pBD90 specified a 35,000-dalton erythromycin-inducible protein, detectable in minicells, which therefore appears different from the 29,000-dalton inducible resistance protein specified by pE194. We conclude that there are at least three distinct MLS resistance determinants to be found among gram-positive bacteria.

Published

1981