Your search keyword '"Federica Briani"' showing total 64 results

1. Integrative structural analysis of Pseudomonas phage DEV reveals a genome ejection motor

Author

Ravi K. Lokareddy, Chun-Feng David Hou, Francesca Forti, Stephano M. Iglesias, Fenglin Li, Mikhail Pavlenok, David S. Horner, Michael Niederweis, Federica Briani, and Gino Cingolani

Subjects

Science

Abstract

Abstract DEV is an obligatory lytic Pseudomonas phage of the N4-like genus, recently reclassified as Schitoviridae. The DEV genome encodes 91 ORFs, including a 3398 amino acid virion-associated RNA polymerase (vRNAP). Here, we describe the complete architecture of DEV, determined using a combination of cryo-electron microscopy localized reconstruction, biochemical methods, and genetic knockouts. We built de novo structures of all capsid factors and tail components involved in host attachment. We demonstrate that DEV long tail fibers are essential for infection of Pseudomonas aeruginosa but dispensable for infecting mutants with a truncated lipopolysaccharide devoid of the O-antigen. We determine that DEV vRNAP is part of a three-gene operon conserved in 191 Schitoviridae genomes. We propose these three proteins are ejected into the host to form a genome ejection motor spanning the cell envelope. We posit that the design principles of the DEV ejection apparatus are conserved in all Schitoviridae.

Published

2024

2. Human PNPase causes RNA stabilization and accumulation of R-loops in the Escherichia coli model system

Author

Federica A. Falchi, Francesca Forti, Cristina Carnelli, Aurelia Genco, Roberto Pizzoccheri, Caterina Manzari, Giulio Pavesi, and Federica Briani

Subjects

Medicine, Science

Abstract

Abstract Polyribonucleotide phosphorylase (PNPase) is a phosphorolytic RNA exonuclease highly conserved throughout evolution. In Escherichia coli, PNPase controls complex phenotypic traits like biofilm formation and growth at low temperature. In human cells, PNPase is located in mitochondria, where it is implicated in the RNA import from the cytoplasm, the mitochondrial RNA degradation and the processing of R-loops, namely stable RNA–DNA hybrids displacing a DNA strand. In this work, we show that the human PNPase (hPNPase) expressed in E. coli causes oxidative stress, SOS response activation and R-loops accumulation. Hundreds of E. coli RNAs are stabilized in presence of hPNPase, whereas only few transcripts are destabilized. Moreover, phenotypic traits typical of E. coli strains lacking PNPase are strengthened in presence of the human enzyme. We discuss the hypothesis that hPNPase expressed in E. coli may bind, but not degrade, the RNA, in agreement with previous in vitro data showing that phosphate concentrations in the range of those found in the bacterial cytoplasm and, more relevant, in the mitochondria, inhibit its activity.

Published

2023

3. High-resolution cryo-EM structure of the Pseudomonas bacteriophage E217

Author

Fenglin Li, Chun-Feng David Hou, Ravi K. Lokareddy, Ruoyu Yang, Francesca Forti, Federica Briani, and Gino Cingolani

Subjects

Science

Abstract

Abstract E217 is a Pseudomonas phage used in an experimental cocktail to eradicate cystic fibrosis-associated Pseudomonas aeruginosa. Here, we describe the structure of the whole E217 virion before and after DNA ejection at 3.1 Å and 4.5 Å resolution, respectively, determined using cryogenic electron microscopy (cryo-EM). We identify and build de novo structures for 19 unique E217 gene products, resolve the tail genome-ejection machine in both extended and contracted states, and decipher the complete architecture of the baseplate formed by 66 polypeptide chains. We also determine that E217 recognizes the host O-antigen as a receptor, and we resolve the N-terminal portion of the O-antigen-binding tail fiber. We propose that E217 design principles presented in this paper are conserved across PB1-like Myoviridae phages of the Pbunavirus genus that encode a ~1.4 MDa baseplate, dramatically smaller than the coliphage T4.

Published

2023

4. Identification and impact on Pseudomonas aeruginosa virulence of mutations conferring resistance to a phage cocktail for phage therapy

Author

Francesca Forti, Claudia Bertoli, Marco Cafora, Sara Gilardi, Anna Pistocchi, and Federica Briani

Subjects

bacteriophage therapy, phage receptors, Pseudomonas aeruginosa phages, zebrafish infection model, Microbiology, QR1-502

Abstract

ABSTRACT Phage therapy represents a promising strategy for curing bacterial infections refractory to antibiotics. However, the success rate of phage therapy may be lowered by the emergence of bacterial resistance to the phages used for therapy. In this work, we studied the resistance to the CK4 cocktail, which is a mixture composed of four phages able to cure Pseudomonas aeruginosa infections in animal models. CK4-resistant mutants were easily isolated from cultures grown in either a standard laboratory medium or an artificial sputum medium mimicking the composition of the airway fluid of cystic fibrosis (CF) patients, who are highly susceptible to P. aeruginosa chronic lung infections. In both cases, CK4-resistant mutants resulted in being defective in lipopolysaccharide (LPS) biosynthesis. Accordingly, all CK4 phages were unable to infect wzy mutants lacking the O-antigen polymerase. A survey of the other 15 P. aeruginosa phages isolated from different environmental sources showed that they all needed either wzy or the Type IV-pilus (T4P) biosynthetic gene pilQ for the infection. Overall, our data suggest that 16 out of the 19 analyzed Pseudomonas phages may use either the LPS or the T4P as a receptor. Interestingly, CK4-resistant mutants devoid of the O-antigen had strongly attenuated virulence in a zebrafish embryo infection model, and the lack of T4P also decreased virulence in zebrafish. With respect to isolates from patients with CF, phages not reproducing in the Δwzy mutant had a wider host range than those requiring pilQ, suggesting that phages dependent on PAO1-type T4P may have limited therapeutic value for treating CF-related infections. IMPORTANCE In this work, we identified the putative receptors of 16 Pseudomonas phages and evaluated how resistance to phages recognizing different bacterial receptors may affect the virulence. Our findings are relevant for the implementation of phage therapy of Pseudomonas aeruginosa infections, which are difficult to treat with antibiotics. Overall, our results highlight the need to modify natural phages to enlarge the repertoire of receptors exploited by therapeutic phages and suggest that phages using the PAO1-type T4P as receptor may have limited value for the therapy of the cystic fibrosis infection.

Published

2023

5. Evaluation of phages and liposomes as combination therapy to counteract Pseudomonas aeruginosa infection in wild-type and CFTR-null models

Author

Marco Cafora, Noemi Poerio, Francesca Forti, Nicoletta Loberto, Davide Pin, Rosaria Bassi, Massimo Aureli, Federica Briani, Anna Pistocchi, and Maurizio Fraziano

Subjects

bacteriophages, liposomes, zebrafish, cystic fibrosis, pseudomonas, Microbiology, QR1-502

Abstract

Multi drug resistant (MDR) bacteria are insensitive to the most common antibiotics currently in use. The spread of antibiotic-resistant bacteria, if not contained, will represent the main cause of death for humanity in 2050. The situation is even more worrying when considering patients with chronic bacterial infections, such as those with Cystic Fibrosis (CF). The development of alternative approaches is essential and novel therapies that combine exogenous and host-mediated antimicrobial action are promising. In this work, we demonstrate that asymmetric phosphatidylserine/phosphatidic acid (PS/PA) liposomes administrated both in prophylactic and therapeutic treatments, induced a reduction in the bacterial burden both in wild-type and cftr-loss-of-function (cftr-LOF) zebrafish embryos infected with Pseudomonas aeruginosa (Pa) PAO1 strain (PAO1). These effects are elicited through the enhancement of phagocytic activity of macrophages. Moreover, the combined use of liposomes and a phage-cocktail (CKΦ), already validated as a PAO1 “eater”, improves the antimicrobial effects of single treatments, and it is effective also against CKΦ-resistant bacteria. We also address the translational potential of the research, by evaluating the safety of CKΦ and PS/PA liposomes administrations in in vitro model of human bronchial epithelial cells, carrying the homozygous F508del-CFTR mutation, and in THP-1 cells differentiated into a macrophage-like phenotype with pharmacologically inhibited CFTR. Our results open the way to the development of novel pharmacological formulations composed of both phages and liposomes to counteract more efficiently the infections caused by Pa or other bacteria, especially in patients with chronic infections such those with CF.

Published

2022

6. Sanguinarine Inhibits the 2-Ketogluconate Pathway of Glucose Utilization in Pseudomonas aeruginosa

Author

Federica A. Falchi, Giorgia Borlotti, Francesco Ferretti, Gianvito Pellegrino, Matteo Raneri, Marco Schiavoni, Alessandro Caselli, and Federica Briani

Subjects

bacterial infections in hyperglycemic patients, Pseudomonas aeruginosa, glucose catabolism, antibacterial drug discovery, drug repurposing, Prestwick Chemical Library, Microbiology, QR1-502

Abstract

Interfering with the ability of pathogenic bacteria to import glucose may represent a new promising antibacterial strategy, especially for the treatment of infections occurring in diabetic and other hyperglycemic patients. Such patients are particularly susceptible to infections caused by a variety of bacteria, among which opportunistic pathogens like Pseudomonas aeruginosa. In P. aeruginosa, glucose can be directly imported into the cytoplasm or after its periplasmic oxidation into gluconate and 2-ketogluconate (2-KG). We recently demonstrated that a P. aeruginosa mutant lacking the 2-KG transporter KguT is less virulent than its kguT+ parental strain in an insect infection model, pointing to 2-KG branch of glucose utilization as a possible target for anti-Pseudomonas drugs. In this work, we devised an experimental protocol to find specific inhibitors of the 2-KG pathway of P. aeruginosa glucose utilization and applied it to the screening of the Prestwick Chemical Library. By exploiting mutants lacking genes involved in the transport of glucose derivatives in the primary screening and in the secondary assays, we could identify sanguinarine as an inhibitor of 2-KG utilization. We also demonstrated that sanguinarine does not prevent 2-KG formation by gluconate oxidation or its transport, suggesting that either KguD or KguK is the target of sanguinarine in P. Aeruginosa.

Published

2021

7. Activity and Function in Human Cells of the Evolutionary Conserved Exonuclease Polynucleotide Phosphorylase

Author

Federica A. Falchi, Roberto Pizzoccheri, and Federica Briani

Subjects

polyribonucleotide phosphorylase, PNPase, PNPT1, RNA decay, RNA stability, RNA binding protein, Biology (General), QH301-705.5, Chemistry, QD1-999

Abstract

Polynucleotide phosphorylase (PNPase) is a phosphorolytic RNA exonuclease highly conserved throughout evolution. Human PNPase (hPNPase) is located in mitochondria and is essential for mitochondrial function and homeostasis. Not surprisingly, mutations in the PNPT1 gene, encoding hPNPase, cause serious diseases. hPNPase has been implicated in a plethora of processes taking place in different cell compartments and involving other proteins, some of which physically interact with hPNPase. This paper reviews hPNPase RNA binding and catalytic activity in relation with the protein structure and in comparison, with the activity of bacterial PNPases. The functions ascribed to hPNPase in different cell compartments are discussed, highlighting the gaps that still need to be filled to understand the physiological role of this ancient protein in human cells.

Published

2022

8. Polynucleotide phosphorylase is implicated in homologous recombination and DNA repair in Escherichia coli

Author

Thomas Carzaniga, Giulia Sbarufatti, Federica Briani, and Gianni Dehò

Subjects

Polynucleotide phosphorylase, Genetic recombination, DNA repair, Mutagenesis, RNA metabolism, Microbiology, QR1-502

Abstract

Abstract Background Polynucleotide phosphorylase (PNPase, encoded by pnp) is generally thought of as an enzyme dedicated to RNA metabolism. The pleiotropic effects of PNPase deficiency is imputed to altered processing and turnover of mRNAs and small RNAs, which in turn leads to aberrant gene expression. However, it has long since been known that this enzyme may also catalyze template-independent polymerization of dNDPs into ssDNA and the reverse phosphorolytic reaction. Recently, PNPase has been implicated in DNA recombination, repair, mutagenesis and resistance to genotoxic agents in diverse bacterial species, raising the possibility that PNPase may directly, rather than through control of gene expression, participate in these processes. Results In this work we present evidence that in Escherichia coli PNPase enhances both homologous recombination upon P1 transduction and error prone DNA repair of double strand breaks induced by zeocin, a radiomimetic agent. Homologous recombination does not require PNPase phosphorolytic activity and is modulated by its RNA binding domains whereas error prone DNA repair of zeocin-induced DNA damage is dependent on PNPase catalytic activity and cannot be suppressed by overexpression of RNase II, the other major enzyme (encoded by rnb) implicated in exonucleolytic RNA degradation. Moreover, E. coli pnp mutants are more sensitive than the wild type to zeocin. This phenotype depends on PNPase phosphorolytic activity and is suppressed by rnb, thus suggesting that zeocin detoxification may largely depend on RNA turnover. Conclusions Our data suggest that PNPase may participate both directly and indirectly through regulation of gene expression to several aspects of DNA metabolism such as recombination, DNA repair and resistance to genotoxic agents.

Published

2017

9. Different csrA Expression Levels in C versus K-12 E. coli Strains Affect Biofilm Formation and Impact the Regulatory Mechanism Presided by the CsrB and CsrC Small RNAs

Author

Thomas Carzaniga, Federica A. Falchi, Francesca Forti, Davide Antoniani, Paolo Landini, and Federica Briani

Subjects

CsrA, PNPase, pgaABCD operon, auto-aggregation, biofilm, poly-β-1,6-N-acetylglucosamine, Biology (General), QH301-705.5

Abstract

Escherichia coli C is a strong biofilm producer in comparison to E. coli K-12 laboratory strains due to higher expression of the pgaABCD operon encoding the enzymes for the biosynthesis of the extracellular polysaccharide poly-β-1,6-N-acetylglucosamine (PNAG). The pgaABCD operon is negatively regulated at the post-transcriptional level by two factors, namely CsrA, a conserved RNA-binding protein controlling multiple pathways, and the RNA exonuclease polynucleotide phosphorylase (PNPase). In this work, we investigated the molecular bases of different PNAG production in C-1a and MG1655 strains taken as representative of E. coli C and K-12 strains, respectively. We found that pgaABCD operon expression is significantly lower in MG1655 than in C-1a; consistently, CsrA protein levels were much higher in MG1655. In contrast, we show that the negative effect exerted by PNPase on pgaABCD expression is much stronger in C-1a than in MG1655. The amount of CsrA and of the small RNAs CsrB, CsrC, and McaS sRNAs regulating CsrA activity is dramatically different in the two strains, whereas PNPase level is similar. Finally, the compensatory regulation acting between CsrB and CsrC in MG1655 does not occur in E. coli C. Our results suggest that PNPase preserves CsrA-dependent regulation by indirectly modulating csrA expression.

Published

2021

10. Overexpression of lpxT Gene in Escherichia coli Inhibits Cell Division and Causes Envelope Defects without Changing the Overall Phosphorylation Level of Lipid A

Author

Federica A. Falchi, Flaviana Di Lorenzo, Roberto Pizzoccheri, Gianluca Casino, Moira Paroni, Francesca Forti, Antonio Molinaro, and Federica Briani

Subjects

membrane proteins, outer membrane, peptidoglycan, lipopolysaccharide (LPS), lipid A phosphorylation, lipid A modification, Biology (General), QH301-705.5

Abstract

LpxT is an inner membrane protein that transfers a phosphate group from the essential lipid undecaprenyl pyrophosphate (C-55PP) to the lipid A moiety of lipopolysaccharide, generating a lipid A tris-phosphorylated species. The protein is encoded by the non-essential lpxT gene, which is conserved in distantly related Gram-negative bacteria. In this work, we investigated the phenotypic effect of lpxT ectopic expression from a plasmid in Escherichia coli. We found that lpxT induction inhibited cell division and led to the formation of elongated cells, mostly with absent or altered septa. Moreover, the cells became sensitive to detergents and to hypo-osmotic shock, indicating that they had cell envelope defects. These effects were not due to lipid A hyperphosphorylation or C-55PP sequestering, but most likely to defective lipopolysaccharide transport. Indeed, lpxT overexpression in mutants lacking the L,D-transpeptidase LdtD and LdtE, which protect cells with outer membrane defects from osmotic lysis, caused cell envelope defects. Moreover, we found that pyrophosphorylated lipid A was also produced in a lpxT deletion mutant, indicating that LpxT is not the only protein able to perform such lipid A modification in E. coli.

Published

2020

11. Comparative profiling of Pseudomonas aeruginosa strains reveals differential expression of novel unique and conserved small RNAs.

Author

Silvia Ferrara, Margherita Brugnoli, Angela De Bonis, Francesco Righetti, Francesco Delvillani, Gianni Dehò, David Horner, Federica Briani, and Giovanni Bertoni

Subjects

Medicine, Science

Abstract

Pseudomonas aeruginosa is a highly adaptable bacterium that thrives in a broad range of ecological niches and can infect multiple hosts as diverse as plants, nematodes and mammals. In humans, it is an important opportunistic pathogen. This wide adaptability correlates with its broad genetic diversity. In this study, we used a deep-sequencing approach to explore the complement of small RNAs (sRNAs) in P. aeruginosa as the number of such regulatory molecules previously identified in this organism is relatively low, considering its genome size, phenotypic diversity and adaptability. We have performed a comparative analysis of PAO1 and PA14 strains which share the same host range but differ in virulence, PA14 being considerably more virulent in several model organisms. Altogether, we have identified more than 150 novel candidate sRNAs and validated a third of them by Northern blotting. Interestingly, a number of these novel sRNAs are strain-specific or showed strain-specific expression, strongly suggesting that they could be involved in determining specific phenotypic traits.

Published

2012

12. Phages as immunomodulators and their promising use as anti-inflammatory agents in a cftr loss-of-function zebrafish model

Author

Nicoletta Loberto, Alessia Brix, Anna Pistocchi, Federica Briani, Francesca Forti, Marco Cafora, and Massimo Aureli

Subjects

0301 basic medicine, Pulmonary and Respiratory Medicine, Cystic Fibrosis, Anti-Inflammatory Agents, Virulence, Inflammation, medicine.disease_cause, Cystic fibrosis, Microbiology, 03 medical and health sciences, 0302 clinical medicine, Loss of Function Mutation, Animals, Immunologic Factors, Medicine, Bacteriophages, Pseudomonas Infections, Receptor, Zebrafish, Loss function, biology, business.industry, Pseudomonas aeruginosa, medicine.disease, biology.organism_classification, Immunity, Innate, Chronic infection, 030104 developmental biology, 030228 respiratory system, Pediatrics, Perinatology and Child Health, medicine.symptom, business

Abstract

Cystic Fibrosis (CF), one of the most frequent hereditary diseases due to mutations in the CFTR gene, causes mortality in humans mainly due to infection in the respiratory system. However, besides the massive inflammatory response triggered by chronic bacterial infections, a constitutive pro-inflammatory state associated with the most common CFTR mutations has been reported in paediatric cases before the onset of bacterial colonization. In previous works we isolated and characterized a mix of virulent bacteriophages (phage cocktail) able to efficiently counteract Pseudomonas aeruginosa infection in a zebrafish model with cftr loss-of-function (LOF), but also showing anti-inflammatory effects in zebrafish embryos not infected by bacteria. On these premises, in this work we demonstrated the anti-inflammatory role of the phage cocktail both in the wild-type (WT) and hyper-inflamed cftr LOF zebrafish embryos in terms of reduction of pro-inflammatory markers. We also dissect that only the virion proteinaceous components, but not the phage DNA, are responsible for the immune-modulatory effect and that this action is elicited through the activation of the Toll-like Receptor (TLR) pathway. In the cftr LOF zebrafish embryos, we demonstrated that phages injection significantly reduces neutrophil migration following acute inflammatory induction. The elucidation of the molecular interaction between phages and the cells of vertebrate immune system might open new possibility in their manipulation for therapeutic benefits especially in diseases such as cystic fibrosis, characterized by chronic infection and inflammation.

Published

2021

13. Cell-Based Fluorescent Screen Amenable to HTS to Identify Inhibitors of Bacterial Translation Initiation

Author

Matteo Raneri, Emilio Alvarez-Ruiz, Danuta Mossakovska, and Federica Briani

Subjects

Settore BIO/18 - Genetica, Antibacterial compounds, Gram-negative bacteria, Leaderless mRNA, Ribosome, S1 ribosomal protein, Translation initiation, Whole-cell assay, Settore BIO/19 - Microbiologia Generale

Published

2022

14. Cell-Based Fluorescent Screen Amenable to HTS to Identify Inhibitors of Bacterial Translation Initiation

Author

Matteo, Raneri, Emilio, Alvarez-Ruiz, Danuta, Mossakovska, and Federica, Briani

Subjects

Mammals, Eukaryotic Cells, Bacteria, Escherichia coli, Animals, Biological Assay, Coloring Agents, Anti-Bacterial Agents

Abstract

A strategy that can be applied to the research of new molecules with antibacterial activity is to look for inhibitors of essential bacterial processes within large collections of chemically heterogeneous compounds. The implementation of this approach requires the development of assays aimed at the identification of molecules interfering with specific cell pathways that can also be used in high-throughput analysis of large chemical libraries. Here, we describe a fluorescence-based whole-cell assay in Escherichia coli devised to find inhibitors of the translation initiation pathway. Translation is a complex and essential mechanism. It involves numerous sub-steps performed by factors that are in many cases sufficiently dissimilar in bacterial and eukaryotic cells to be targetable with domain-specific drugs. As a matter of fact, translation has been proven as one of the few bacterial mechanisms pharmacologically tractable with specific antibiotics. The assay described in this updated chapter is tailored to the identification of molecules affecting the first stage of translation initiation, which is the most dissimilar step in bacteria versus mammals. The effect of the compounds under analysis is measured in living cells, thus allowing evaluation of their in vivo performance as inhibitors of translation initiation. Compared with other assays for antibacterials, the major advantages of this screen are its simplicity, high mechanism specificity, and amenability to scaling up to high-throughput analyses.

Published

2022

15. Perturbation of protein homeostasis brings plastids at the crossroad between repair and dismantling

Author

Luca Tadini, Nicolaj Jeran, Guido Domingo, Federico Zambelli, Simona Masiero, Anna Calabritto, Elena Costantini, Sara Forlani, Milena Marsoni, Federica Briani, Candida Vannini, and Paolo Pesaresi

Abstract

The chloroplast proteome is a dynamic mosaic of plastid- and nuclear-encoded proteins. Plastid protein homeostasis is maintained through the balance between de novo synthesis and proteolysis. Intracellular communication pathways, including the plastid-to-nucleus signalling and the protein homeostasis machinery, made of stromal chaperones and proteases, shape chloroplast proteome based on developmental and physiological needs. However, the maintenance of fully functional chloroplasts is costly and under specific stress conditions the degradation of damaged chloroplasts is essential to the maintenance of a healthy population of photosynthesising organelles while promoting nutrient redistribution to sink tissues. In this work, we have addressed this complex regulatory chloroplast- quality-control pathway by modulating the expression of two nuclear genes encoding plastid ribosomal proteins PRPS1 and PRPL4. By transcriptomics, proteomics and transmission electron microscopy analyses, we show that the increased expression of PRPS1 gene leads to chloroplast degradation and early flowering, as an escape strategy from stress. On the contrary, the overaccumulation of PRPL4 protein is kept under control by increasing the amount of plastid chaperones and components of the unfolded protein response (cpUPR) regulatory mechanism. This study advances our understanding of molecular mechanisms underlying chloroplast retrograde communication and provides new insight into cellular responses to impaired plastid protein homeostasis.

Published

2022

16. Terminase Subunits from the Pseudomonas-Phage E217

Author

Ravi K. Lokareddy, Chun-Feng David Hou, Steven G. Doll, Fenglin Li, Richard E. Gillilan, Francesca Forti, David S. Horner, Federica Briani, and Gino Cingolani

Subjects

Adenosine Triphosphatases, History, Endodeoxyribonucleases, Polymers and Plastics, Ribonuclease H, Pseudomonas-phages, bacteriophage E217, large terminase, small terminase, viral genome-packaging motor, Settore BIO/19 - Microbiologia Generale, Industrial and Manufacturing Engineering, Article, Settore BIO/18 - Genetica, Viral Proteins, Structural Biology, Settore BIO/10 - Biochimica, Myoviridae, DNA, Viral, Pseudomonas aeruginosa, Magnesium, Business and International Management, Pseudomonas Phages, Molecular Biology

Abstract

Pseudomonas phages are increasingly important biomedicines for phage therapy, but little is known about how these viruses package DNA. This paper explores the terminase subunits from the Myoviridae E217, a Pseudomonas-phage used in an experimental cocktail to eradicate P. aeruginosa in vitro and in animal models. We identified the large (TerL) and small (TerS) terminase subunits in two genes ~58 kbs away from each other in the E217 genome. TerL presents a classical two-domain architecture, consisting of an N-terminal ATPase and C-terminal nuclease domain arranged into a bean-shaped tertiary structure. A 2.05 Å crystal structure of the C-terminal domain revealed an RNase H-like fold with two magnesium ions in the nuclease active site. Mutations in TerL residues involved in magnesium coordination had a dominant-negative effect on phage growth. However, the two ions identified in the active site were too far from each other to promote two-metal-ion catalysis, suggesting a conformational change is required for nuclease activity. We also determined a 3.38 Å cryo-EM reconstruction of E217 TerS that revealed a ring-like decamer, departing from the most common nonameric quaternary structure observed thus far. E217 TerS contains both N-terminal helix-turn-helix motifs enriched in basic residues and a central channel lined with basic residues large enough to accommodate double-stranded DNA. Overexpression of TerS caused a more than a four-fold reduction of E217 burst size, suggesting a catalytic amount of the protein is required for packaging. Together, these data expand the molecular repertoire of viral terminase subunits to Pseudomonas-phages used for phage therapy.

Published

2022

17. Phage therapy against Pseudomonas aeruginosa infections in a cystic fibrosis zebrafish model

Author

Daniela Ghisotti, Marco Cafora, Federica Briani, Laura Ferrari, Gianluca Deflorian, Anna Pistocchi, Giorgio Binelli, and Francesca Forti

Subjects

0301 basic medicine, Embryo, Nonmammalian, Phage therapy, Cystic Fibrosis, medicine.drug_class, medicine.medical_treatment, Antibiotics, lcsh:Medicine, Disease, medicine.disease_cause, Cystic fibrosis, Article, Microbiology, 03 medical and health sciences, Mice, 0302 clinical medicine, medicine, Animals, Pseudomonas Infections, lcsh:Science, Zebrafish, Respiratory Tract Infections, Multidisciplinary, biology, Pseudomonas aeruginosa, lcsh:R, biology.organism_classification, medicine.disease, Phenotype, Anti-Bacterial Agents, Galleria mellonella, Disease Models, Animal, 030104 developmental biology, lcsh:Q, Pseudomonas Phages, 030217 neurology & neurosurgery

Abstract

Cystic fibrosis (CF) is a hereditary disease due to mutations in the CFTR gene and causes mortality in humans mainly due to respiratory infections caused by Pseudomonas aeruginosa. In a previous work we used phage therapy, which is a treatment with a mix of phages, to actively counteract acute P. aeruginosa infections in mice and Galleria mellonella larvae. In this work we apply phage therapy to the treatment of P. aeruginosa PAO1 infections in a CF zebrafish model. The structure of the CFTR channel is evolutionary conserved between fish and mammals and cftr-loss-of-function zebrafish embryos show a phenotype that recapitulates the human disease, in particular with destruction of the pancreas. We show that phage therapy is able to decrease lethality, bacterial burden, and the pro-inflammatory response caused by PAO1 infection. In addition, phage administration relieves the constitutive inflammatory state of CF embryos. To our knowledge, this is the first time that phage therapy is used to cure P. aeruginosa infections in a CF animal model. We also find that the curative effect against PAO1 infections is improved by combining phages and antibiotic treatments, opening a useful therapeutic approach that could reduce antibiotic doses and time of administration.

Published

2019

18. Different csrA Expression Levels in C versus K-12 E. coli Strains Affect Biofilm Formation and Impact the Regulatory Mechanism Presided by the CsrB and CsrC Small RNAs

Author

Francesca Forti, Federica A. Falchi, Davide Antoniani, Paolo Landini, Federica Briani, and Thomas Carzaniga

Subjects

Microbiology (medical), Exonuclease, Operon, QH301-705.5, poly-β-1,6-N-acetylglucosamine, Purine nucleoside phosphorylase, medicine.disease_cause, Microbiology, Article, biofilm, pgaABCD operon, 03 medical and health sciences, Virology, medicine, auto-aggregation, CsrA protein, Polynucleotide phosphorylase, CsrA, Biology (General), Escherichia coli, 030304 developmental biology, 0303 health sciences, PNPase, biology, 030306 microbiology, Chemistry, Biofilm, RNA, sRNA-dependent regulation, Cell biology, biology.protein, bacteria

Abstract

Escherichia coli C is a strong biofilm producer in comparison to E. coli K-12 laboratory strains due to higher expression of the pgaABCD operon encoding the enzymes for the biosynthesis of the extracellular polysaccharide poly-β-1,6-N-acetylglucosamine (PNAG). The pgaABCD operon is negatively regulated at the post-transcriptional level by two factors, namely CsrA, a conserved RNA-binding protein controlling multiple pathways, and the RNA exonuclease polynucleotide phosphorylase (PNPase). In this work, we investigated the molecular bases of different PNAG production in C-1a and MG1655 strains taken as representative of E. coli C and K-12 strains, respectively. We found that pgaABCD operon expression is significantly lower in MG1655 than in C-1a, consistently, CsrA protein levels were much higher in MG1655. In contrast, we show that the negative effect exerted by PNPase on pgaABCD expression is much stronger in C-1a than in MG1655. The amount of CsrA and of the small RNAs CsrB, CsrC, and McaS sRNAs regulating CsrA activity is dramatically different in the two strains, whereas PNPase level is similar. Finally, the compensatory regulation acting between CsrB and CsrC in MG1655 does not occur in E. coli C. Our results suggest that PNPase preserves CsrA-dependent regulation by indirectly modulating csrA expression.

Published

2021

19. Phage Therapy Application to Counteract Pseudomonas aeruginosa Infection in Cystic Fibrosis Zebrafish Embryos

Author

Marco, Cafora, Francesca, Forti, Federica, Briani, Daniela, Ghisotti, and Anna, Pistocchi

Subjects

Embryo, Nonmammalian, Cystic Fibrosis, Microinjections, Green Fluorescent Proteins, Reproducibility of Results, Anti-Bacterial Agents, Morpholinos, Pseudomonas aeruginosa, Animals, Cytokines, Bacteriophages, Pseudomonas Infections, Phage Therapy, Inflammation Mediators, Zebrafish

Abstract

Antimicrobial resistance, a major consequence of diagnostic uncertainty and antimicrobial overprescription, is an increasingly recognized cause of severe infections, complications, and mortality worldwide with a huge impact on our society and on the health system. In particular, patients with compromised immune systems or pre-existing and chronic pathologies, such as cystic fibrosis (CF), are subjected to frequent antibiotic treatments to control the infections with the appearance and diffusion of multidrug resistant isolates. Therefore, there is an urgent need to address alternative therapies to counteract bacterial infections. Use of bacteriophages, the natural enemies of bacteria, can be a possible solution. The protocol detailed in this work describes the application of phage therapy against Pseudomonas aeruginosa infection in CF zebrafish embryos. Zebrafish embryos were infected with P. aeruginosa to demonstrate that phage therapy is effective against P. aeruginosa infections as it reduces lethality, bacterial burden and pro-inflammatory immune response in CF embryos.

Published

2020

20. Phage Therapy Application to Counteract Pseudomonas aeruginosa Infection in Cystic Fibrosis Zebrafish Embryos

Author

Daniela Ghisotti, Francesca Forti, Federica Briani, Marco Cafora, and Anna Pistocchi

Subjects

General Immunology and Microbiology, Phage therapy, Pseudomonas aeruginosa, medicine.drug_class, business.industry, General Chemical Engineering, General Neuroscience, medicine.medical_treatment, Antibiotics, medicine.disease, medicine.disease_cause, Antimicrobial, Cystic fibrosis, General Biochemistry, Genetics and Molecular Biology, Microbiology, Multiple drug resistance, Antibiotic resistance, Immune system, medicine, business

Abstract

Antimicrobial resistance, a major consequence of diagnostic uncertainty and antimicrobial overprescription, is an increasingly recognized cause of severe infections, complications, and mortality worldwide with a huge impact on our society and on the health system. In particular, patients with compromised immune systems or pre-existing and chronic pathologies, such as cystic fibrosis (CF), are subjected to frequent antibiotic treatments to control the infections with the appearance and diffusion of multidrug resistant isolates. Therefore, there is an urgent need to address alternative therapies to counteract bacterial infections. Use of bacteriophages, the natural enemies of bacteria, can be a possible solution. The protocol detailed in this work describes the application of phage therapy against Pseudomonas aeruginosa infection in CF zebrafish embryos. Zebrafish embryos were infected with P. aeruginosa to demonstrate that phage therapy is effective against P. aeruginosa infections as it reduces lethality, bacterial burden and pro-inflammatory immune response in CF embryos.

Published

2020

21. Polynucleotide phosphorylase is implicated in homologous recombination and DNA repair in Escherichia coli

Author

Federica Briani, Thomas Carzaniga, Gianni Dehò, and Giulia Sbarufatti

Subjects

0301 basic medicine, Microbiology (medical), Polynucleotide phosphorylase, DNA repair, DNA damage, Zeocin, RNA Stability, 030106 microbiology, lcsh:QR1-502, DNA, Single-Stranded, Purine nucleoside phosphorylase, Biology, Microbiology, Genetic recombination, Gene Expression Regulation, Enzymologic, lcsh:Microbiology, Bleomycin, 03 medical and health sciences, chemistry.chemical_compound, Escherichia coli, RNA, Messenger, Homologous Recombination, Polyribonucleotide Nucleotidyltransferase, RNA metabolism, Escherichia coli Proteins, RNA, Gene Expression Regulation, Bacterial, RNA, Bacterial, Biochemistry, chemistry, Mutagenesis, Exoribonucleases, Mutation, Homologous recombination, Research Article, DNA Damage, Protein Binding

Abstract

Background Polynucleotide phosphorylase (PNPase, encoded by pnp) is generally thought of as an enzyme dedicated to RNA metabolism. The pleiotropic effects of PNPase deficiency is imputed to altered processing and turnover of mRNAs and small RNAs, which in turn leads to aberrant gene expression. However, it has long since been known that this enzyme may also catalyze template-independent polymerization of dNDPs into ssDNA and the reverse phosphorolytic reaction. Recently, PNPase has been implicated in DNA recombination, repair, mutagenesis and resistance to genotoxic agents in diverse bacterial species, raising the possibility that PNPase may directly, rather than through control of gene expression, participate in these processes. Results In this work we present evidence that in Escherichia coli PNPase enhances both homologous recombination upon P1 transduction and error prone DNA repair of double strand breaks induced by zeocin, a radiomimetic agent. Homologous recombination does not require PNPase phosphorolytic activity and is modulated by its RNA binding domains whereas error prone DNA repair of zeocin-induced DNA damage is dependent on PNPase catalytic activity and cannot be suppressed by overexpression of RNase II, the other major enzyme (encoded by rnb) implicated in exonucleolytic RNA degradation. Moreover, E. coli pnp mutants are more sensitive than the wild type to zeocin. This phenotype depends on PNPase phosphorolytic activity and is suppressed by rnb, thus suggesting that zeocin detoxification may largely depend on RNA turnover. Conclusions Our data suggest that PNPase may participate both directly and indirectly through regulation of gene expression to several aspects of DNA metabolism such as recombination, DNA repair and resistance to genotoxic agents.

Published

2017

22. WS12.1 Potential action of phages as immunomodulators in cystic fibrosis

Author

Francesca Forti, Alessia Brix, Nicoletta Loberto, Massimo Aureli, Marco Cafora, Anna Pistocchi, and Federica Briani

Subjects

Pulmonary and Respiratory Medicine, Action (philosophy), business.industry, Pediatrics, Perinatology and Child Health, Immunology, Medicine, business, medicine.disease, Cystic fibrosis

Published

2020

23. Design of a Broad-Range Bacteriophage Cocktail That Reduces Pseudomonas aeruginosa Biofilms and Treats Acute Infections in Two Animal Models

Author

Maria Enrica Pasini, Martina Rossitto, Daniela Ghisotti, Francesca Forti, Ersilia Fiscarelli, Lisa Cariani, Laurent Debarbieux, David S. Horner, Marco Cafora, Federica Briani, Dwayne R. Roach, Department of Biosciences [Milano], Università degli Studi di Milano = University of Milan (UNIMI), Département de Microbiologie - Department of Microbiology, Institut Pasteur [Paris] (IP), Children's Hospital Bambino Gesù IRCCS [Rome], Fondazione IRCCS Ca' Granda - Ospedale Maggiore Policlinico, This work was supported by the Italian Cystic Fibrosis Foundation (FFC#17/2015 andFFC#16/2016). D.R.R. is the recipient of a European Respiratory Society Fellowship(RESPIRE2-2015-8416)., Università degli Studi di Milano [Milano] (UNIMI), and Institut Pasteur [Paris]

Subjects

0301 basic medicine, bacteriophages, phage therapy, Phage therapy, medicine.medical_treatment, Biology, Moths, medicine.disease_cause, Microbiology, Bacteriophage, cystic fibrosis, 03 medical and health sciences, medicine, Animals, Pharmacology (medical), Pseudomonas Infections, Experimental Therapeutics, Pharmacology, Pseudomonas aeruginosa, fungi, Biofilm, Respiratory infection, biology.organism_classification, medicine.disease, Antimicrobial, [SDV.MP.BAC]Life Sciences [q-bio]/Microbiology and Parasitology/Bacteriology, 3. Good health, Galleria mellonella, 030104 developmental biology, Infectious Diseases, Bacteremia, Biofilms, Larva, Pseudomonas Phages

Abstract

The alarming diffusion of multidrug-resistant (MDR) bacterial strains requires investigations on nonantibiotic therapies. Among such therapies, the use of bacteriophages (phages) as antimicrobial agents, namely, phage therapy, is a promising treatment strategy supported by the findings of recent successful compassionate treatments in Europe and the United States. In this work, we combined host range and genomic information to design a 6-phage cocktail killing several clinical strains ofPseudomonas aeruginosa, including those collected from Italian cystic fibrosis (CF) patients, and analyzed the cocktail performance. We demonstrated that the cocktail composed of four novel phages (PYO2, DEV, E215 and E217) and two previously characterized phages (PAK_P1 and PAK_P4) was able to lyseP. aeruginosaboth in planktonic liquid cultures and in biofilms. In addition, we showed that the phage cocktail could cure acute respiratory infection in mice and treat bacteremia in wax moth (Galleria mellonella) larvae. Furthermore, administration of the cocktail to larvae prior to bacterial infection provided prophylaxis. In this regard, the efficiency of the phage cocktail was found to be unaffected by the MDR or mucoid phenotype of the pseudomonal strain. The cocktail was found to be superior to the individual phages in destroying biofilms and providing a faster treatment in mice. We also found theGallerialarva model to be cost-effective for testing the susceptibility of clinical strains to phages, suggesting that it could be implemented in the frame of developing personalized phage therapies.

Published

2018

24. Pseudomonas aeruginosa mutants defective in glucose uptake have pleiotropic phenotype and altered virulence in non-mammal infection models

Author

Matteo Raneri, Irene Bianconi, Palma Ferrante, Giordano Rampioni, Clelia Peano, Chiara Dalmasio, Eva Pinatel, Livia Leoni, Olivier Jousson, Federica Briani, Raneri, Matteo, Pinatel, Eva, Peano, Clelia, Rampioni, Giordano, Leoni, Livia, Bianconi, Irene, Jousson, Olivier, Dalmasio, Chiara, Ferrante, Palma, and Briani, Federica

Subjects

0301 basic medicine, Transcription, Genetic, Glucose uptake, 030106 microbiology, Mutant, RNA-sequencing, lcsh:Medicine, Virulence, Moths, Biology, medicine.disease_cause, Models, Biological, Article, 03 medical and health sciences, glucose uptake, Pseudomonas aeruginosa, virulence, quorum sensing, biofilm, transcriptomics, medicine, Animals, Pseudomonas Infections, Caenorhabditis elegans, lcsh:Science, Gene, Multidisciplinary, Bacteria, Pseudomonas aeruginosa, lcsh:R, Glucose transporter, Quorum Sensing, Genetic Pleiotropy, Gene Expression Regulation, Bacterial, Phenotype, Carbon, Cell biology, Disease Models, Animal, Glucose, Genes, Bacterial, Biofilms, Mutation, Pyocyanine, lcsh:Q, Transcriptome, Bacterial outer membrane, Oligopeptides, Oxidation-Reduction

Abstract

Pseudomonas spp. are endowed with a complex pathway for glucose uptake that relies on multiple transporters. In this work we report the construction and characterization of Pseudomonas aeruginosa single and multiple mutants with unmarked deletions of genes encoding outer membrane (OM) and inner membrane (IM) proteins involved in glucose uptake. We found that a triple ΔgltKGF ΔgntP ΔkguT mutant lacking all known IM transporters (named GUN for Glucose Uptake Null) is unable to grow on glucose as unique carbon source. More than 500 genes controlling both metabolic functions and virulence traits show differential expression in GUN relative to the parental strain. Consistent with transcriptomic data, the GUN mutant displays a pleiotropic phenotype. Notably, the genome-wide transcriptional profile and most phenotypic traits differ between the GUN mutant and the wild type strain irrespective of the presence of glucose, suggesting that the investigated genes may have additional roles besides glucose transport. Finally, mutants carrying single or multiple deletions in the glucose uptake genes showed attenuated virulence relative to the wild type strain in Galleria mellonella, but not in Caenorhabditis elegans infection model, supporting the notion that metabolic functions may deeply impact P. aeruginosa adaptation to specific environments found inside the host.

Published

2018

25. A Whole-Cell Assay for Specific Inhibitors of Translation Initiation in Bacteria

Author

B. Sciandrone, Federica Briani, Matteo Raneri, Raneri, M, Sciandrone, B, and Briani, F

Subjects

High-Throughput Screening Assay, Untranslated region, leaderless mRNA, Five prime untranslated region, Gene Expression, Microbial Sensitivity Tests, antibacterial drug, Biology, Sensitivity and Specificity, Biochemistry, Analytical Chemistry, Small Molecule Libraries, Eukaryotic translation, Genes, Reporter, Ribosomal protein, Eukaryotic initiation factor, Anti-Bacterial Agent, Drug Discovery, Escherichia coli, Initiation factor, 30S, Peptide Chain Initiation, Translational, Messenger RNA, Microbial Sensitivity Test, Molecular biology, Anti-Bacterial Agents, High-Throughput Screening Assays, Cell biology, Gram-negative bacteria, Molecular Medicine, S1 ribosomal protein, bacterial translation initiation, Biotechnology

Abstract

The bacterial translational apparatus is an ideal target for the search of new antibiotics. In fact, it performs an essential process carried out by a large number of potential subtargets for antibiotic action. Moreover, it is sufficiently different in several molecular details from the apparatus of Eukarya and Archaea to generally ensure specificity for the bacterial domain. This applies in particular to translation initiation, which is the most different step in the process. In bacteria, the 30S ribosomal subunit directly binds to the translation initiation region, a site within the messenger RNA (mRNA) 5'-untranslated region (5'-UTR). 30S binding is mediated by the interaction of both the 16S ribosomal RNA and the ribosomal protein S1 with specific regions of the mRNA 5'-UTR. An alternative, S1-independent pathway is enjoyed by leaderless mRNAs (i.e., transcripts devoid of a 5'-UTR). We have developed a simple fluorescence-based whole-cell assay in Escherichia coli to find inhibitors of the canonical S1-dependent translation initiation pathway. The assay has been set up both in a common E. coli laboratory strain and in a strain with an outer membrane permeability defect. Compared with other whole-cell assays for antibacterials, the major advantages of the screen described here are high sensitivity and specificity.

Published

2015

26. RNase III-Independent Autogenous Regulation of Escherichia coli Polynucleotide Phosphorylase via Translational Repression

Author

Federica Briani, Thomas Carzaniga, and Gianni Dehò

Subjects

inorganic chemicals, Polyribonucleotide Nucleotidyltransferase, Ribonuclease III, Messenger RNA, biology, RNase P, Escherichia coli Proteins, Down-Regulation, Purine nucleoside phosphorylase, Gene Expression Regulation, Bacterial, Articles, Microbiology, RNase PH, Gene Expression Regulation, Enzymologic, enzymes and coenzymes (carbohydrates), RNase MRP, Biochemistry, Protein Biosynthesis, Exoribonuclease, Escherichia coli, biology.protein, heterocyclic compounds, Polynucleotide phosphorylase, Molecular Biology

Abstract

The complex posttranscriptional regulation mechanism of the Escherichia coli pnp gene, which encodes the phosphorolytic exoribonuclease polynucleotide phosphorylase (PNPase), involves two endoribonucleases, namely, RNase III and RNase E, and PNPase itself, which thus autoregulates its own expression. The models proposed for pnp autoregulation posit that the target of PNPase is a mature pnp mRNA previously processed at its 5′ end by RNase III, rather than the primary pnp transcript (RNase III-dependent models), and that PNPase activity eventually leads to pnp mRNA degradation by RNase E. However, some published data suggest that pnp expression may also be regulated through a PNPase-dependent, RNase III-independent mechanism. To address this issue, we constructed isogenic Δ pnp rnc + and Δ pnp Δ rnc strains with a chromosomal pnp-lacZ translational fusion and measured β-galactosidase activity in the absence and presence of PNPase expressed by a plasmid. Our results show that PNPase also regulates its own expression via a reversible RNase III-independent pathway acting upstream from the RNase III-dependent branch. This pathway requires the PNPase RNA binding domains KH and S1 but not its phosphorolytic activity. We suggest that the RNase III-independent autoregulation of PNPase occurs at the level of translational repression, possibly by competition for pnp primary transcript between PNPase and the ribosomal protein S1. IMPORTANCE In Escherichia coli , polynucleotide phosphorylase (PNPase, encoded by pnp ) posttranscriptionally regulates its own expression. The two models proposed so far posit a two-step mechanism in which RNase III, by cutting the leader region of the pnp primary transcript, creates the substrate for PNPase regulatory activity, eventually leading to pnp mRNA degradation by RNase E. In this work, we provide evidence supporting an additional pathway for PNPase autogenous regulation in which PNPase acts as a translational repressor independently of RNase III cleavage. Our data make a new contribution to the understanding of the regulatory mechanism of pnp mRNA, a process long since considered a paradigmatic example of posttranscriptional regulation at the level of mRNA stability.

Published

2015

27. Cell-Based Fluorescent Screen to Identify Inhibitors of Bacterial Translation Initiation

Author

Federica Briani

Subjects

0301 basic medicine, Gram-negative bacteria, biology, Translation (biology), Computational biology, biology.organism_classification, Bioinformatics, Bacterial Processes, Ribosome, Chemical library, 03 medical and health sciences, chemistry.chemical_compound, 030104 developmental biology, Eukaryotic translation, chemistry, In vivo, Prokaryotic translation

Abstract

A strategy that can be applied to the research of new molecules with antibacterial activity is to look for inhibitors of essential bacterial processes within large collections of chemically heterogeneous compounds. The implementation of this approach requires the development of proper assays aimed at the identification of molecules interfering with specific cell pathways and potentially applicable to the high throughput analysis of large chemical library. Here, I describe a fluorescence-based whole-cell assay in Escherichia coli devised to find inhibitors of the translation initiation pathway. Translation is a complex and essential mechanism. It involves numerous sub-steps performed by factors that are in many cases sufficiently dissimilar in bacterial and eukaryotic cells to be targetable with domain-specific drugs. As a matter of fact, translation has been proven as one of the few bacterial mechanisms pharmacologically tractable with specific antibiotics. The assay described in this chapter is tailored to the identification of molecules affecting the first stage of translation initiation, which is the most dissimilar step in bacteria vs. mammals. The effect of the compounds under analysis is assayed in living cells, thus allowing evaluating their in vivo performance as inhibitors of translation initiation. Compared with other assays for antibacterials, the major advantages of this screen are its simplicity and high mechanism specificity.

Published

2016

28. Phage therapy against Pseudomonas aeruginosa infections in cystic fibrosis patients

Author

Francesca Forti, Federica Briani, and Daniela Ghisotti

Subjects

0301 basic medicine, 03 medical and health sciences, Pseudomonas aeruginosa Infections, Phage therapy, medicine.medical_treatment, viruses, 030106 microbiology, medicine, Biology, medicine.disease, Cystic fibrosis, Microbiology

Abstract

Pseudomonas aeruginosa is the most common pathogen found in the lung of cystic fibrosis patients. The use of phage therapy could help in fighting the alarming diffusion of antibiotic multi-resistant strains. A number of new phages were isolated from sewage samples in Milan, and tested for growth on a panel of P. aeruginosa strains collected in Italian hospitals. Comprehensively, we analyzed 23 new phages on 57 clinical or environmental P. aeruginosa strains. Six phages belonging to different classes, i.e. Myoviridae, Podoviridae and Siphoviridae, as assessed by TEM analysis, were mixed in a cocktail. The host range of the phage cocktail was larger than that of individual phages. Infection in liquid culture of strain PAO1 indicated that the phage cocktail efficiently killed the bacterial cells, although resistant mutants appeared at the end. The ability to infect P. aeruginosa growing in biofilm demonstrated that the phage cocktail was able to reduce the biomass of a preformed biofilm. DNA was extracted from the selected phages and send for whole genome shotgun sequencing using the Illumina MiSeq platform at the CNR IBBE institute in Bari. This project is financed by Italian Foundation of Cystic Fibrosis (# 17/2015)., Journal of Targeting Infectiuos Diseases, Vol 1, No 1 (2016)

Published

2016

29. Polynucleotide phosphorylase exonuclease and polymerase activities on single-stranded DNA ends are modulated by RecN, SsbA and RecA proteins

Author

Federica Briani, Thomas Carzaniga, Esther Garcia-Tirado, Gianni Dehò, Juan C. Alonso, Paula P. Cárdenas, and Sandro Zangrossi

Subjects

Exonuclease, DNA, Single-Stranded, Purine nucleoside phosphorylase, DNA-Directed DNA Polymerase, Bacillus subtilis, Genome Integrity, Repair and Replication, chemistry.chemical_compound, Deoxyadenine Nucleotides, Bacterial Proteins, Escherichia coli, Genetics, Nucleoid, Polynucleotide phosphorylase, Polymerase, Polyribonucleotide Nucleotidyltransferase, Manganese, biology, DNA Restriction Enzymes, biology.organism_classification, Rec A Recombinases, Exodeoxyribonucleases, chemistry, Biochemistry, biology.protein, Homologous recombination, DNA

Abstract

Bacillus subtilis pnpA gene product, polynucleotide phosphorylase (PNPase), is involved in double-strand break (DSB) repair via homologous recombination (HR) or non-homologous end-joining (NHEJ). RecN is among the first responders to localize at the DNA DSBs, with PNPase facilitating the formation of a discrete RecN focus per nucleoid. PNPase, which co-purifies with RecA and RecN, was able to degrade single-stranded (ss) DNA with a 3' → 5' polarity in the presence of Mn(2+) and low inorganic phosphate (Pi) concentration, or to extend a 3'-OH end in the presence dNDP · Mn(2+). Both PNPase activities were observed in evolutionarily distant bacteria (B. subtilis and Escherichia coli), suggesting conserved functions. The activity of PNPase was directed toward ssDNA degradation or polymerization by manipulating the Pi/dNDPs concentrations or the availability of RecA or RecN. In its dATP-bound form, RecN stimulates PNPase-mediated polymerization. ssDNA phosphorolysis catalyzed by PNPase is stimulated by RecA, but inhibited by SsbA. Our findings suggest that (i) the PNPase degradative and polymerizing activities might play a critical role in the transition from DSB sensing to end resection via HR and (ii) by blunting a 3'-tailed duplex DNA, in the absence of HR, B. subtilis PNPase might also contribute to repair via NHEJ.

Published

2011

30. S1 ribosomal protein and the interplay between translation and mRNA decay

Author

F. Delvillani, Federica Briani, Giulia Papiani, and Gianni Dehò

Subjects

Ribosomal Proteins, Messenger RNA, RNase P, Escherichia coli Proteins, RNA Stability, Biology, Ribosome, Molecular biology, Cell biology, Eukaryotic translation, Ribosomal protein, Protein Biosynthesis, Endoribonucleases, Escherichia coli, Genetics, Protein biosynthesis, RNA, 30S, RNA, Messenger, Translation initiation complex, 5' Untranslated Regions, Ribosomes, Heat-Shock Proteins

Abstract

S1 is an 'atypical' ribosomal protein weakly associated with the 30S subunit that has been implicated in translation, transcription and control of RNA stability. S1 is thought to participate in translation initiation complex formation by assisting 30S positioning in the translation initiation region, but little is known about its role in other RNA transactions. In this work, we have analysed in vivo the effects of different intracellular S1 concentrations, from depletion to overexpression, on translation, decay and intracellular distribution of leadered and leaderless messenger RNAs (mRNAs). We show that the cspE mRNA, like the rpsO transcript, may be cleaved by RNase E at multiple sites, whereas the leaderless cspE transcript may also be degraded via an alternative pathway by an unknown endonuclease. Upon S1 overexpression, RNase E-dependent decay of both cspE and rpsO mRNAs is suppressed and these transcripts are stabilized, whereas cleavage of leaderless cspE mRNA by the unidentified endonuclease is not affected. Overall, our data suggest that ribosome-unbound S1 may inhibit translation and that part of the Escherichia coli ribosomes may actually lack S1.

Published

2011

31. Identification and expression profiling of Ceratitis capitata genes coding for β-hexosaminidases

Author

Federica Briani, Maria Enrica Pasini, Jari Intra, Katia Petroni, V. Calvenzani, Ludvik M. Gomulski, and Maria Elisa Perotti

Subjects

Male, Molecular Sequence Data, Testis, Genetics, medicine, Melanogaster, Animals, Hexosaminidase, Amino Acid Sequence, Spermatogenesis, Gene, Spermatid, biology, Gene Expression Profiling, Ovary, Ceratitis capitata, General Medicine, Oocyte, biology.organism_classification, Spermatids, beta-N-Acetylhexosaminidases, HEXB, Gene expression profiling, medicine.anatomical_structure, Female

Abstract

The goal of this study was to identify the genes coding for β-N-acetylhexosaminidases in the Mediterranean fruit fly (medfly) Ceratitis capitata, one of the most destructive agricultural pests, belonging to the Tephritidae family, order Diptera. Two dimeric β-N-acetylhexosaminidases, HEXA and HEXB, have been recently identified on Drosophila sperm. These enzymes are involved in egg binding through interactions with complementary carbohydrates on the surface of the egg shell. Three genes, Hexosaminidase 1 (Hexo1), Hexosaminidase 2 (Hexo2) and fused lobes (fdl), encode for HEXA and HEXB subunits. The availability of C. capitata EST libraries derived from embryos and adult heads allowed us to identify three sequences homologous to the D. melanogaster Hexo1, Hexo2 and fdl genes. Here, we report the expression profile analysis of CcHexo1, CcHexo2 and Ccfdld in several tissues, organs and stages. Ccfdl expression was highest in heads of both sexes and in whole adult females. In the testis and ovary the three genes showed distinct spatial and temporal expression patterns. All the mRNAs were detectable in early stages of spermatogenesis; CcHexo2 and Ccfdl were also expressed in early elongating spermatid cysts. All three genes are expressed in the ovarian nurse cells. CcHexo1 and Ccfdl are stage specific, since they have been observed in stages 12 and 13 during oocyte growth, when programmed cell death occurs in nurse cells. The expression pattern of the three genes in medfly gonads suggests that, as their Drosophila counterparts, they may encode for proteins involved in gametogenesis and fertilization.

Published

2011

32. Autogenous Regulation of Escherichia coli Polynucleotide Phosphorylase Expression Revisited

Author

Federica Briani, Paolo Marchi, Thomas Carzaniga, Giuseppe Merlino, Gianni Dehò, and Sandro Zangrossi

Subjects

Polyribonucleotide Nucleotidyltransferase, Ribonuclease III, RNA Stability, Messenger RNA, RNase P, Escherichia coli Proteins, Gene Expression Regulation, Bacterial, Biology, Microbiology, RNase PH, Gene Expression Regulation, Enzymologic, RNA, Bacterial, RNase MRP, Biochemistry, Protein Biosynthesis, Exoribonuclease, Endoribonucleases, Escherichia coli, biology.protein, Gene Regulation, Polynucleotide phosphorylase, Molecular Biology

Abstract

The Escherichia coli polynucleotide phosphorylase (PNPase; encoded by pnp ), a phosphorolytic exoribonuclease, posttranscriptionally regulates its own expression at the level of mRNA stability and translation. Its primary transcript is very efficiently processed by RNase III, an endonuclease that makes a staggered double-strand cleavage about in the middle of a long stem-loop in the 5′-untranslated region. The processed pnp mRNA is then rapidly degraded in a PNPase-dependent manner. Two non-mutually exclusive models have been proposed to explain PNPase autogenous regulation. The earlier one suggested that PNPase impedes translation of the RNase III-processed pnp mRNA, thus exposing the transcript to degradative pathways. More recently, this has been replaced by the current model, which maintains that PNPase would simply degrade the promoter proximal small RNA generated by the RNase III endonucleolytic cleavage, thus destroying the double-stranded structure at the 5′ end that otherwise stabilizes the pnp mRNA. In our opinion, however, the first model was not completely ruled out. Moreover, the RNA decay pathway acting upon the pnp mRNA after disruption of the 5′ double-stranded structure remained to be determined. Here we provide additional support to the current model and show that the RNase III-processed pnp mRNA devoid of the double-stranded structure at its 5′ end is not translatable and is degraded by RNase E in a PNPase-independent manner. Thus, the role of PNPase in autoregulation is simply to remove, in concert with RNase III, the 5′ fragment of the cleaved structure that both allows translation and prevents the RNase E-mediated PNPase-independent degradation of the pnp transcript.

Published

2009

33. Regulation of Escherichia coli Polynucleotide Phosphorylase by ATP

Author

Paolo Tortora, Sandro Zangrossi, Elisa Mazzantini, Gianni Dehò, Marta Del Favero, Federica Briani, Del Favero, M, Mazzantini, E, Briani, F, Zangrossi, S, Tortora, P, and Dehò, G

Subjects

RNA Stability, Purine nucleoside phosphorylase, Biology, Settore BIO/19 - Microbiologia Generale, RNA decay, Biochemistry, chemistry.chemical_compound, Adenosine Triphosphate, Allosteric Regulation, Escherichia coli, Polynucleotide phosphorylase, polyadenylation, Molecular Biology, Phosphorolysis, Polyribonucleotide Nucleotidyltransferase, chemistry.chemical_classification, PNPase, RNA, energy charge, Cell Biology, BIO/10 - BIOCHIMICA, ATP, RNA, Bacterial, Settore BIO/18 - Genetica, Enzyme, chemistry, Degradosome, Adenosine triphosphate

Abstract

Polynucleotide phosphorylase (PNPase), an enzyme conserved in bacteria and eukaryotic organelles, processively catalyzes the phosphorolysis of RNA, releasing nucleotide diphosphates, and the reverse polymerization reaction. In Escherichia coli, both reactions are implicated in RNA decay, as addition of either poly(A) or heteropolymeric tails targets RNA to degradation. PNPase may also be associated with the RNA degradosome, a heteromultimeric protein machine that can degrade highly structured RNA. Here, we report that ATP binds to PNPase and allosterically inhibits both its phosphorolytic and polymerization activities. Our data suggest that PNPase-dependent RNA tailing and degradation occur mainly at low ATP concentrations, whereas other enzymes may play a more significant role at high energy charge. These findings connect RNA turnover with the energy charge of the cell and highlight unforeseen metabolic roles of PNPase.

Published

2008

34. Autogenous regulation of Escherichia coli polynucleotide phosphorylase during cold acclimation by transcription termination and antitermination

Author

Federica Briani, Vera Longhi, Elisa Gaetani, Sandro Zangrossi, Paolo Marchi, and Gianni Dehò

Subjects

rho GTP-Binding Proteins, Transcription, Genetic, Molecular Sequence Data, Biology, transcription termination/antitermination, cold shock, polynucleotide phosphorylase, Settore BIO/19 - Microbiologia Generale, Gene Expression Regulation, Enzymologic, RNA, Transfer, Genes, Reporter, Transcription (biology), Gene expression, Escherichia coli, Genetics, Cold acclimation, Polynucleotide phosphorylase, Molecular Biology, Gene, Alleles, Polyribonucleotide Nucleotidyltransferase, Regulation of gene expression, Base Sequence, Wild type, Gene Expression Regulation, Bacterial, General Medicine, Molecular biology, Cold Temperature, Settore BIO/18 - Genetica, Antitermination, Nucleic Acid Conformation, 5' Untranslated Regions, Plasmids

Abstract

Adaptation of Escherichia coli at low temperature implicates a drastic reprogramming of gene expression patterns. Mechanisms operating downstream of transcription initiation, such as control of transcription termination, mRNA stability and translatability, play a major role in controlling gene expression in the cold acclimation phase. It was previously shown that Rho-dependent transcription termination within pnp, the gene encoding polynucleotide phosphorylase (PNPase), was suppressed in pnp nonsense mutants, whereas it was restored by complementation with wild type allele. Using a tRNA gene as a reporter and the strong Rho-dependent transcription terminator t ( imm ) of bacteriophage P4 as a tester, here we show that specific sites in the 5'-untranslated region of pnp mRNA are required for PNPase-sensitive cold-induced suppression of Rho-dependent transcription termination. We suggest that suppression of Rho-dependent transcription termination within pnp and its restoration by PNPase is an autogenous regulatory circuit that modulates pnp expression during cold acclimation.

Published

2007

35. Regulation and functions of bacterial PNPase

Author

Federica Briani, Thomas Carzaniga, and Gianni Dehò

Subjects

0301 basic medicine, RNA Stability, 030106 microbiology, Endoribonuclease, Adaptation, Biological, Purine nucleoside phosphorylase, Biochemistry, Catalysis, Gene Expression Regulation, Enzymologic, 03 medical and health sciences, Structure-Activity Relationship, Exoribonuclease, Gene expression, Ribonuclease III, Polynucleotide phosphorylase, RNA Processing, Post-Transcriptional, Molecular Biology, Genetics, Polyribonucleotide Nucleotidyltransferase, biology, Bacteria, RNA, Gene Expression Regulation, Bacterial, Cell biology, Enzyme Activation, Multiprotein Complexes, biology.protein, Protein Binding

Abstract

Polynucleotide phosphorylase (PNPase) is an exoribonuclease that catalyzes the processive phosphorolytic degradation of RNA from the 3'-end. The enzyme catalyzes also the reverse reaction of polymerization of nucleoside diphosphates that has been implicated in the generation of heteropolymeric tails at the RNA 3'-end. The enzyme is widely conserved and plays a major role in RNA decay in both Gram-negative and Gram-positive bacteria. Moreover, it participates in maturation and quality control of stable RNA. PNPase autoregulates its own expression at post-transcriptional level through a complex mechanism that involves the endoribonuclease RNase III and translation control. The activity of PNPase is modulated in an intricate and still unclear manner by interactions with small molecules and recruitment in different multiprotein complexes. Not surprisingly, given the wide spectrum of PNPase substrates, PNPase-defective mutations in different bacterial species have pleiotropic effects and perturb the execution of genetic programs involving drastic changes in global gene expression such as biofilm formation, growth at suboptimal temperatures, and virulence.

Published

2015

36. Identification and expression analysis of Drosophilamelanogaster genes encoding β-hexosaminidases of the sperm plasma membrane

Author

Maria Enrica Pasini, M. Hoshi, Jari Intra, Maria-Elisa Perotti, M. Matsumoto, F. Cattaneo, and Federica Briani

Subjects

Male, Gene isoform, Somatic cell, Molecular Sequence Data, Biochemistry, Germline, Hexosaminidase A, Gene expression, Animals, Drosophila Proteins, Humans, Amino Acid Sequence, Gene, Sperm plasma membrane, Sperm-Ovum Interactions, biology, Gene Expression Profiling, Cell Membrane, biology.organism_classification, Spermatozoa, Sperm, Molecular biology, beta-N-Acetylhexosaminidases, Cell biology, Drosophila melanogaster, Gene Expression Regulation, Organ Specificity, Female

Abstract

Sperm surface beta-N-acetylhexosaminidases are among the molecules mediating early gamete interactions in invertebrates and vertebrates, including man. The plasma membrane of Drosophila spermatozoa contains two beta-N-acetylhexosaminidases, DmHEXA and DmHEXB, which are required for egg fertilization. Here, we demonstrate that three putative Drosophila melanogaster genes predicted to code for beta-N-acetylhexosaminidases, Hexo1, Hexo2, and fdl, are all expressed in the male germ line. fdl codes for a homolog of the alpha-subunit of the mammalian lysosomal beta-N-acetylhexosaminidase Hex A. Hexo1 and Hexo2 encode two homologs of the beta-subunit of all known beta-N-acetylhexosaminidases, which we have named beta(1) and beta(2), respectively. Immunoblot analysis of sperm proteins indicated that the gene products associate in different heterodimeric combinations forming DmHEXA, with an alphabeta(2) structure, and DmHEXB, with a beta(1)beta(2) structure. Immunofluorescence demonstrated that all the gene products localized to the sperm plasma membrane. Although none of the genes was testis-specific, fdl was highly and preferentially expressed in the testis, whereas Hexo1 and Hexo2 showed broader tissue expression. Enzyme assays carried out on testis and on a variety of somatic tissues corroborated the results of gene expression analysis. These findings for the first time show the in vivo expression in insects of genes encoding beta-N-acetylhexosaminidases, the only molecules so far identified as involved in sperm/egg recognition in this class, whereas in mammals, the organisms where these enzymes have been best studied, only two types of polypeptide chains forming dimeric functional beta-N-acetylhexosaminidases are present in Drosophila three different gene products are available that might generate numerous dimeric isoforms.

Published

2006

37. Analysis of the Escherichia coli RNA degradosome composition by a proteomic approach

Author

Maria Elena Regonesi, Paolo Tortora, Gianni Dehò, Marta Del Favero, Pierluigi Mauri, Louise Benazzi, Federica Briani, Fabrizio Basilico, Regonesi, M, Del Favero, M, Basilico, F, Briani, F, Benazzi, L, Tortora, P, Mauri, P, and Dehò, G

Subjects

Proteomics, Polynucleotide phosphorylase, Exosome complex, RNase P, Ribonuclease E, Endoribonuclease, Biology, degradosome, Biochemistry, DnaK, RNA degradation, Exoribonuclease, Endoribonucleases, Escherichia coli, Polyribonucleotide Nucleotidyltransferase, Mass spectrometry, Escherichia coli Proteins, E. coli, RNA, General Medicine, RNA Helicase A, MudPIT, Multiprotein Complexes, Phosphopyruvate Hydratase, Degradosome

Abstract

The RNA degradosome is a bacterial protein machine devoted to RNA degradation and processing. In Escherichia coli it is typically composed of the endoribonuclear RNase E, which also serves as a scaffold for the other components, the exoribonuclease PNPase, the RNA helicase RhIB, and enolase. Several other proteins have been found associated to the core complex. However, it remains Unclear in most cases whether Such proteins are occasional contaminants or specific components, and which is their function. To facilitate the analysis of the RNA degradosome composition under different physiological and genetic conditions we set up a simplified preparation procedure based on the affinity purification of FLAG epitope-tagged RNase E coupled to Multidimensional Protein Identification Technology (MudPIT) for the rapid and quantitative identification of the different components. By this proteomic approach, we show that the chaperone protein DnaK, previously identified as a "minor component" of the degradosome, associates with abnormal complexes under stressful conditions Such as overexpression of RNase E, low temperature, and in the absence of PNPase; however, DnaK does not seem to be essential for RNA degradosome structure nor for its assembly. In addition, we show that normalized score values obtain by MudPIT analysis may be taken as quantitative estimates of the relative protein abundance in different degradosome preparations. (c) 2005 Elsevier SAS. All rights reserved.

Published

2006

38. A mutation in polynucleotide phosphorylase from Escherichia coli impairing RNA binding and degradosome stability

Author

Daniela Ghisotti, Federica Briani, Sandro Zangrossi, Andrea Ghetta, Maria Elena Regonesi, Paolo Tortora, Gianni Dehò, Regonesi, M, Briani, F, Ghetta, A, Zangrossi, S, Ghisotti, D, Tortora, P, and Deho, G

Subjects

Exonuclease, RNA Stability, Polynucleotide phosphorylase, RNase P, Biology, Catalysis, Mutant protein, Escherichia coli, Genetics, Degradosome, RNA, Messenger, Polyribonucleotide Nucleotidyltransferase, Messenger RNA, Escherichia coli Proteins, RNA, Gene Expression Regulation, Bacterial, Articles, BIO/10 - BIOCHIMICA, RNA, Bacterial, RNA turnover, Amino Acid Substitution, Biochemistry, Mutation, biology.protein, Electrophoresis, Polyacrylamide Gel

Abstract

Polynucleotide phosphorylase (PNPase), a 3' to 5' exonuclease encoded by pnp, plays a key role in Escherichia coli RNA decay. The enzyme, made of three identical 711 amino acid subunits, may also be assembled in the RNA degradosome, a heteromultimeric complex involved in RNA degradation. PNPase autogenously regulates its expression by promoting the decay of pnp mRNA, supposedly by binding at the 5'-untranslated leader region of an RNase III-processed form of this transcript. The KH and S1 RNA-binding domains at the C-terminus of the protein (amino acids 552-711) are thought to be involved in pnp mRNA recognition. Here we show that a G454D substitution in E.coli PNPase impairs autogenous regulation whereas it does not affect the catalytic activities of the enzyme. Although the mutation maps outside of the KH and S1 RNA-binding domains, analysis of the mutant protein revealed a defective RNA binding, thus suggesting that other determinants may be involved in PNPase-RNA interactions. The mutation also caused a looser association with the degradosome and an abnormal electrophoretic mobility in native gels. The latter feature suggests an altered structural conformation of PNPase, which may account for the properties of the mutant protein.

Published

2004

39. Hfq affects the length and the frequency of short oligo(A) tails at the 3' end of Escherichia coli rpsO mRNAs

Author

Federica Briani, Jacques Le Derout, Philippe Régnier, Eliane Hajnsdorf, Gianni Dehò, and Marc Folichon

Subjects

Ribosomal Proteins, Genotype, Transcription, Genetic, Polyadenylation, RNase P, Molecular Sequence Data, Transcription (biology), Endoribonucleases, Escherichia coli, Genetics, RNA, Messenger, Polynucleotide phosphorylase, 3' Untranslated Regions, Polyribonucleotide Nucleotidyltransferase, Messenger RNA, Base Sequence, biology, RNA, Articles, Molecular biology, Terminator (genetics), Exoribonucleases, biology.protein, Nucleic Acid Conformation, DNA polymerase I, Poly A

Abstract

Polyadenylation plays an important role in RNA degradation in bacterial cells. In Escherichia coli, exoribonucleases, mostly RNase II and polynucleotide phosphorylase, antagonize the synthesis of poly(A) tails by poly(A) polymerase I (PAP I). In accordance with earlier observations showing that only a small fraction of bacterial RNA is polyadenylated, we demonstrate here that approximately 10% of rpsO mRNA harbors short oligo(A) tails ranging from one to five A residues in wild-type cells. We also compared the length, frequency and distribution of poly(A) tails at the 3'-end of rpsO transcripts in vivo in the presence and absence of Hfq, a host factor that in vitro stimulates the activity of PAP I, and found that Hfq affects all three parameters. In the hfq(+) strain the average length of oligo(A) tails and frequency of polyadenylated transcripts was higher than in the hfq(-) strain and a smaller proportion of tails was found at the 3' end of transcripts terminated at the Rho- independent terminator. Our data led us to the conclusion that Hfq is involved in the recognition of 3' RNA extremities by PAP I.

Published

2003

40. RNase E and Polyadenyl Polymerase I are Involved in Maturation of CI RNA, the P4 Phage Immunity Factor

Author

Daniela Ghisotti, Eliane Hajnsdorf, Federica Briani, Domenico Migliorini, Gianni Dehò, Philippe Régnier, and Emanuela Del Vecchio

Subjects

Base Sequence, RNase P, Molecular Sequence Data, Intron, Polynucleotide Adenylyltransferase, RNA, RNA-dependent RNA polymerase, gene expression, pcnB, regulatory RNA, RNA processing and degradation, stable RNA, Biology, Settore BIO/19 - Microbiologia Generale, Non-coding RNA, Coliphages, Molecular biology, Settore BIO/18 - Genetica, Structural Biology, Transcription (biology), Endoribonucleases, Escherichia coli, Nucleic Acid Conformation, RNA, Viral, RNA, Messenger, Polynucleotide phosphorylase, RNA Processing, Post-Transcriptional, Degradosome, Molecular Biology

Abstract

Bacteriophage P4 immunity is controlled by a small stable RNA (CI RNA) that derives from the processing of primary transcripts. In previous works, we observed that the endonuclease RNase P is required for the maturation of CI RNA 5'-end; moreover, we found that polynucleotide phosphorylase (PNPase), a 3' to 5' RNA-degrading enzyme, is required for efficient 5'-end processing of CI RNA, suggesting that 3'-end degradation of the primary transcript might be involved in the production of proper RNase P substrates. Here, we demonstrate that another Escherichia coli nuclease, RNase E, would appear to be involved in this process. We found that transcripts of the P4 immunity region are modified by the post-transcriptional addition of short poly(A) tails and heteropolymeric tails with prevalence of A residues. Most oligoadenylated transcripts encompass the whole cI locus and are thus compatible as intermediates in the CI RNA maturation pathway. On the contrary, in a polynucleotide phosphorylase (PNPase)-defective host, adenylation occurred most frequently within cI, implying that such transcripts are targeted for degradation. We did not find polyadenylation in a pcnB mutant, suggesting that the pcnB-encoded polyadenyl polymerase I (PAP I) is the only enzyme responsible for modification of P4 immunity transcripts. Maturation of CI RNA 5'-end in such a mutant was impaired, further supporting the idea that processing of the 3'-end of primary transcripts is an important step for efficient maturation of CI RNA by RNase P.

Published

2002

41. Transcriptional and post-transcriptional control of polynucleotide phosphorylase during cold acclimation in Escherichia coli

Author

Paolo Tortora, Sandro Zangrossi, Gianni Dehò, Maria Elena Regonesi, Daniela Ghisotti, and Federica Briani

Subjects

inorganic chemicals, Messenger RNA, Purine nucleoside phosphorylase, Cold-shock domain, Biology, medicine.disease_cause, Microbiology, Molecular biology, enzymes and coenzymes (carbohydrates), Transcription (biology), medicine, Cold acclimation, heterocyclic compounds, Polynucleotide phosphorylase, Molecular Biology, Escherichia coli, Post-transcriptional regulation

Abstract

Polynucleotide phosphorylase (PNPase, polyribonucleotide nucleotidyltransferase, EC 2.7.7.8) is one of the cold shock-induced proteins in Escherichia coli and pnp, the gene encoding it, is essential for growth at low temperatures. We have analysed the expression of pnp upon cold shock and found a dramatic transient variation of pnp transcription profile: within the first hour after temperature downshift the amount of pnp transcripts detectable by Northern blotting increased more than 10-fold and new mRNA species that cover pnp and the downstream region, including the cold shock gene deaD, appeared; 2 h after temperature downshift the transcription profile reverted to a preshift-like pattern in a PNPase-independent manner. The higher amount of pnp transcripts appeared to be mainly due to an increased stability of the RNAs. The abundance of pnp transcripts was not paralleled by comparable variation of the protein: PNPase steadily increased about twofold during the first 3 h at low temperature, as determined both by Western blotting and enzymatic activity assay, suggesting that PNPase, unlike other known cold shock proteins, is not efficiently translated in the acclimation phase. In experiments aimed at assessing the role of PNPase in autogenous control during cold shock, we detected a Rho-dependent termination site within pnp. In the cold acclimation phase, termination at this site depended upon the presence of PNPase, suggesting that during cold shock pnp is autogenously regulated at the level of transcription elongation.

Published

2002

42. Characterization of the small antisense CI RNA that regulates bacteriophage P4 immunity 1 1Edited by M. Gottesman

Author

Francesca Forti, Daniela Ghisotti, Gianni Dehò, Ilaria Dragoni, and Federica Briani

Subjects

Genetics, Small RNA, Structural Biology, Transcription (biology), Termination factor, Antitermination, RNA, Biology, Stem-loop, Non-coding RNA, Molecular Biology, Molecular biology, Nucleic acid secondary structure

Abstract

In the immune state bacteriophage P4 prevents expression of the replication functions by premature termination of transcription. A small RNA, the CI RNA, is the trans acting factor that regulates P4 immunity, by pairing to complementary target sequences and causing premature transcription termination. The CI RNA is matured by RNAse P and PNPase from the leader region of the same operon it regulates. In this work we better characterize this molecule. CI RNA copy number was determined to be around 500 molecules per lysogenic cell. By S 1 mapping we defined the 3′-end at 8423(±1); thus CI RNA is 79(±1) nt long. The minimum region for correct processing requires two bases upstream of the CI RNA 5′-end and the CCA sequence at the 3′-end. Computer analysis by FOLD RNA of CI RNA sequence predicts a cloverleaf-like structure formed by a double-stranded stalk, a minor and a major stem loop, and a single-stranded bulge. We analysed several cI mutations, which fall either in the single or double-stranded CI RNA regions. Base substitutions in the main loop and in the single-stranded bulge apparently did not change CI RNA structure, but affected its activity by altering the complementarity with the target sequences, whereas a mutation in the secondary stem had a disruptive effect on CI RNA secondary structure. The effects of this latter mutation were suppressed by a base substitution that restored the complementarity with the corresponding base in the stem. Base substitutions in the main stem caused only local alterations in the secondary structure of CI. However, when the substitutions concerned either G8501 or its complementary base at the bottom of the stem, CI RNA was not correctly processed.

Published

2002

43. Tet-Trap, a genetic approach to the identification of bacterial RNAthermometers: application to Pseudomonas aeruginosa

Author

Luca Petiti, Silvia Ferrara, Gianni Dehò, B. Sciandrone, Giovanni Bertoni, Clelia Peano, F. Delvillani, Federica Briani, Maria Enrica Pasini, Christian Berens, Christiane Georgi, Delvillani, F, Sciandrone, B, Peano, C, Petiti, L, Berens, C, Georgi, C, Ferrara, S, Bertoni, G, Pasini, M, Deho, G, and Briani, F

Subjects

Transcription Factor, DNA-Binding Protein, Bacterial Protein, Biology, medicine.disease_cause, Article, chemistry.chemical_compound, Bacterial Proteins, Escherichia coli Protein, Escherichia coli, medicine, Humans, TetR, RNA, Messenger, Molecular Biology, Gene, Transcription factor, Genetics, Messenger RNA, Phosphotransferases (Phosphate Group Acceptor), Ribosomal Protein S9, Pseudomonas aeruginosa, Escherichia coli Proteins, Temperature, RNA, Gene Expression Regulation, Bacterial, Molecular biology, PtxS, DNA-Binding Proteins, RNA, Bacterial, chemistry, PA5194, Bacterial riboregulator, Heat-Shock Response, DNA, LpxT, Human, Transcription Factors

Abstract

Modulation of mRNA translatability either by trans-acting factors (proteins or sRNAs) or by in cis-acting riboregulators is widespread in bacteria and controls relevant phenotypic traits. Unfortunately, global identification of post-transcriptionally regulated genes is complicated by poor structural and functional conservation of regulatory elements and by the limitations of proteomic approaches in protein quantification. We devised a genetic system for the identification of post-transcriptionally regulated genes and we applied this system to search for Pseudomonas aeruginosa RNA thermometers, a class of regulatory RNA that modulates gene translation in response to temperature changes. As P. aeruginosa is able to thrive in a broad range of environmental conditions, genes differentially expressed at 37°C versus lower temperatures may be involved in infection and survival in the human host. We prepared a plasmid vector library with translational fusions of P. aeruginosa DNA fragments (PaDNA) inserted upstream of TIP2, a short peptide able to inactivate the Tet repressor (TetR) upon expression. The library was assayed in a streptomycin-resistant merodiploid rpsL+/rpsL31 Escherichia coli strain in which the dominant rpsL+ allele, which confers streptomycin sensitivity, was repressed by TetR. PaDNA fragments conferring thermosensitive streptomycin resistance (i.e., expressing PaDNA–TIP2 fusions at 37°C, but not at 28°C) were sequenced. We identified four new putative thermosensors. Two of them were validated with conventional reporter systems in E. coli and P. aeruginosa. Interestingly, one regulates the expression of ptxS, a gene implicated in P. aeruginosa pathogenesis.

Published

2014

44. A conserved loop in polynucleotide phosphorylase (PNPase) essential for both RNA and ADP/phosphate binding

Author

Paolo Tortora, Luca De Gioia, Marco Nardini, Maria Elena Regonesi, Elisa Mazzantini, Gianni Dehò, Claudio Greco, Federica Briani, Thomas Carzaniga, Carzaniga, T, Mazzantini, E, Nardini, M, Regonesi, M, Greco, C, Briani, F, DE GIOIA, L, Deho, G, and Tortora, P

Subjects

Molecular Sequence Data, Purine nucleoside phosphorylase, Protomer, Biology, Arginine, Biochemistry, RNase PH, Protein Structure, Secondary, Phosphates, Catalytic Domain, Escherichia coli, Amino Acid Sequence, Polynucleotide phosphorylase, Phosphorolysis, Polyribonucleotide Nucleotidyltransferase, PNPase, Alanine, Sequence Homology, Amino Acid, Escherichia coli Proteins, RNA, General Medicine, Enzyme structure, Protein Structure, Tertiary, Adenosine Diphosphate, Molecular Docking Simulation, Kinetics, RNA, Bacterial, Mutation, Mutation testing, Sequence Alignment

Abstract

Polynucleotide phosphorylase (PNPase) reversibly catalyzes RNA phosphorolysis and polymerization of nucleoside diphosphates. Its homotrimeric structure forms a central channel where RNA is accommodated. Each protomer core is formed by two paralogous RNase PH domains: PNPase1, whose function is largely unknown, hosts a conserved FFRR loop interacting with RNA, whereas PNPase2 bears the putative catalytic site, ∼20 Å away from the FFRR loop. To date, little is known regarding PNPase catalytic mechanism. We analyzed the kinetic properties of two Escherichia coli PNPase mutants in the FFRR loop (R79A and R80A), which exhibited a dramatic increase in Km for ADP/Pi binding, but not for poly(A), suggesting that the two residues may be essential for binding ADP and Pi. However, both mutants were severely impaired in shifting RNA electrophoretic mobility, implying that the two arginines contribute also to RNA binding. Additional interactions between RNA and other PNPase domains (such as KH and S1) may preserve the enzymatic activity in R79A and R80A mutants. Inspection of enzyme structure showed that PNPase has evolved a long-range acting hydrogen bonding network that connects the FFRR loop with the catalytic site via the F380 residue. This hypothesis was supported by mutation analysis. Phylogenetic analysis of PNPase domains and RNase PH suggests that such network is a unique feature of PNPase1 domain, which coevolved with the paralogous PNPase2 domain. © 2013 Elsevier Masson SAS. All rights reserved.

Published

2014

45. The Plasmid Status of Satellite Bacteriophage P4

Author

Francesca Forti, Daniela Ghisotti, Federica Briani, and Gianni Dehò

Subjects

DNA Replication, Gene Expression Regulation, Viral, Genetics, biology, Phagemid, Circular bacterial chromosome, DNA Helicases, DNA replication, RNA Nucleotidyltransferases, Genome, Viral, biology.organism_classification, Satellite virus, DNA-Binding Proteins, Bacteriophage, Viral Proteins, Plasmid, Lytic cycle, Satellite Viruses, Escherichia coli, Bacteriophage T4, Molecular Biology, Prophage, Plasmids

Abstract

P4 is a natural phasmid (phage-plasmid) that exploits different modes of propagation in its host Escherichia coli. Extracellularly, P4 is a virion, with a tailed icosahedral head, which encapsidates the 11.6-kb-long double-stranded DNA genome. After infection of the E. coli host, P4 DNA can integrate into the bacterial chromosome and be maintained in a repressed state (lysogeny). Alternatively, P4 can replicate as a free DNA molecule; this leads to either the lytic cycle or the plasmid state, depending on the presence or absence of the genome of a helper phage P2 in the E. coli host. As a phage, P4 is thus a satellite of P2 phage, depending on the helper genes for all the morphogenetic functions, whereas for all its episomal functions (integration and immunity, multicopy plasmid replication) P4 is completely autonomous from the helper. Replication of P4 DNA depends on its alpha protein, a multifunctional polypeptide that exhibits primase and helicase activity and binds specifically the P4 origin. Replication starts from a unique point, ori1, and proceeds bidirectionally in a straight theta-type mode. P4 negatively regulates the plasmid copy number at several levels. An unusual mechanism of copy number control is based on protein-protein interaction: the P4-encoded Cnr protein interacts with the alpha gene product, inhibiting its replication potential. Furthermore, expression of the replication genes cnr and alpha is regulated in a complex way that involves modulation of promoter activity by positive and negative factors and multiple mechanisms of transcription elongation-termination control. Thus, the relatively small P4 genome encodes mostly regulatory functions, required for its propagation both as an episomal element and as a temperate satellite phage. Plasmids that, like P4, propagate horizontally via a specific transduction mechanism have also been found in the Archaea. The presence of P4-like prophages or cryptic prophages often associated with accessory bacterial functions attests to the contribution of satellite phages to bacterial evolution.

Published

2001

46. Antisense RNA-dependent transcription termination sites that modulate lysogenic development of satellite phage P4

Author

Federica Briani, Daniela Ghisotti, and Gianni Dehò

Subjects

rho GTP-Binding Proteins, Transcription, Genetic, Termination factor, Biology, Coliphages, Microbiology, Viral Proteins, Bacterial Proteins, Transcription (biology), Gene expression, RNA, Antisense, Viral Regulatory and Accessory Proteins, Molecular Biology, Terminator Regions, Genetic, Escherichia coli Proteins, RNA, Rho factor, Molecular biology, Antisense RNA, DNA-Binding Proteins, Repressor Proteins, Terminator (genetics), Antitermination, biology.protein, Nucleic Acid Conformation, Bacterial Outer Membrane Proteins, Transcription Factors

Abstract

In the lysogenic state, bacteriophage P4 prevents the expression of its own replication genes, which are encoded in the left operon, through premature transcription termination. The phage factor responsible for efficient termination is a small, untranslated RNA (CI RNA), which acts as an antisense RNA and controls transcription termination by pairing with two complementary sequences (seqA and seqC) located within the leader region of the left operon. A Rho-dependent termination site, timm, was previously shown to be involved in the control of P4 replication gene expression. In the present study, by making use of phage PhiR73 as a cloning vector and of suppressor tRNAGly as a reporter gene, we characterized two additional terminators, t1 and t4. Although transcription termination at neither site requires the Rho factor, only t1 has the typical structure of a Rho-independent terminator. t1 is located between the PLE promoter and the cI gene, whereas t4 is located between cI and timm. Efficient termination at t1 requires the CI RNA and the seqA target sequence; in vitro, the CI RNA enhanced termination at t1 in the absence of any bacterial factor. A P4 mutant, in which the t1 terminator has been deleted, can still lysogenize both Rho+ and Rho- strains and exhibits increased expression of CI RNA. These data indicate that t1 and the Rho-dependent timm terminators are not essential for lysogeny. t1 is involved in CI RNA autoregulation, whereas t4 appears to be the main terminator necessary to prevent expression of the lytic genes in the lysogenic state.

Published

2000

47. A Rho-Dependent Transcription Termination Site Regulated by Bacteriophage P4 RNA Immunity Factor

Author

Sandro Zangrossi, Daniela Ghisotti, Federica Briani, and Gianni Dehò

Subjects

Gene Expression Regulation, Viral, Terminator Regions, Genetic, Genetics, Binding Sites, Base Sequence, Transcription, Genetic, General transcription factor, Termination factor, Molecular Sequence Data, RNA polymerase II, Biology, Coliphages, Rho Factor, Terminator (genetics), Transcription (biology), Antitermination, Virology, Mutation, biology.protein, RNA, Viral, bacteria, Transcription factor II D, Lysogeny, RNA polymerase II holoenzyme

Abstract

The genes required for replication of the temperate bacteriophage P4, which are coded by the phage left operon, are expressed from a constitutive promoter (P LE ). In the lysogenic state, repression of the P4 replication genes is achieved by premature transcription termination. The leader region of the left operon encodes all the genetic determinants required for prophage immunity, namely: (i) the P4 immunity factor, a short, stable RNA (CI RNA) that is generated by processing of the leader transcript; (ii) two specific target sequences that exhibit complementarity with the CI RNA. RNA–RNA interactions between the CI RNA and the target sites on the mRNA leader region are essential for transcription termination. To understand how transcription termination is elicited by the P4 immunity mechanism, it is relevant to identify the transcription termination site. This, however, could not be directly inferred from the 3′-end of the transcription products because of the extensive and complex processing and degradation of the leader RNA. In this work, by making use of a tRNA gene as a reporter, we identify the termination site of the immunity transcripts ( t imm ). This is a Rho-dependent terminator located within the first translated gene of the left operon and is regulated by P4 immunity. Analysis of the P4 transcription pattern in Escherichia coli rho mutants suggests that termination at t imm may also be important for the efficient processing of the CI RNA.

Published

1996

48. Multiple regulatory mechanisms controlling phage-plasmid P4 propagation

Author

Sandro Zangrossi, Susanna Terzano, Simona Polo, Gianni Dehò, Gianpiero Sironi, Massimo Zappone, Tiziana Sturniolo, Daniela Ghisotti, Federica Briani, Pierangela Sabbattini, Francesca Forti, and Flavia Piazza

Subjects

DNA Replication, Base Sequence, Transcription, Genetic, Operon, Molecular Sequence Data, DNA replication, Promoter, Biology, Virus Replication, Microbiology, Molecular biology, Plasmid maintenance, Infectious Diseases, Plasmid, Gene Expression Regulation, Lytic cycle, Transcription (biology), Lysogenic cycle, bacteria, Bacteriophages, Bacteriophage P1

Abstract

Bacteriophage P4 autonomous replication may result in the lytic cycle or in plasmid maintenance, depending, respectively, on the presence or absence of the helper phage P2 genome in the Escherichia coli host cell. Alternatively, P4 may lysogenize the bacterial host and be maintained in an immune-integrated condition. A key step in the choice between the lytic / plasmid vs. the lysogenic condition is the regulation of P4 α operon. This operon may be transcribed from two promoters, PLE and PLL, and encodes both immunity (promoter proximal) and replication (promoter distal) functions. PLE is a constitutive promoter and transcription of the downstream replication genes is regulated by transcription termination. The trans-acting immunity factor that controls premature transcription termination is a short RNA encoded in the PLE proximal part of the operon. Expression of the replication functions in the lytic/plasmid condition is achieved by activation of the PLL promoter. Transcription from PLL is insensitive to the termination mechanism that acts on transcription starting from PLE. PLL is also negatively regulated by P4 orf88, the first gene downstream of PLL. An additional control on P4 DNA replication is exerted by the P4 cnr gene product.

Published

1995

49. Polynucleotide phosphorylase hinders mRNA degradation upon ribosomal protein S1 overexpression in Escherichia coli

Author

Francesca Rossi, Federica Briani, Thomas Carzaniga, Gianni Dehò, Serena Curti, and Pierluigi Mauri

Subjects

Polyribonucleotide Nucleotidyltransferase, Ribosomal Proteins, Messenger RNA, Escherichia coli Proteins, RNA Stability, Purine nucleoside phosphorylase, RNA, MRNA stabilization, Gene Expression Regulation, Bacterial, Biology, Primary transcript, Settore BIO/19 - Microbiologia Generale, Molecular biology, Gene Expression Regulation, Enzymologic, Article, RNA, Bacterial, Settore BIO/18 - Genetica, Ribosomal protein, Exoribonuclease, Escherichia coli, Polynucleotide phosphorylase, RNA, Messenger, Molecular Biology, Protein Binding

Abstract

The exoribonuclease polynucleotide phosphorylase (PNPase, encoded by pnp) is a major player in bacterial RNA decay. In Escherichia coli, PNPase expression is post-transcriptionally regulated at the level of mRNA stability. The primary transcript is very efficiently processed by the endonuclease RNase III at a specific site and the processed pnp mRNA is rapidly degraded in a PNPase-dependent manner. While investigating the PNPase autoregulation mechanism we found, by UV-cross-linking experiments, that the ribosomal protein S1 in crude extracts binds to the pnp-mRNA leader region. We assayed the potential role of S1 protein in pnp gene regulation by modulating S1 expression from depletion to overexpression. We found that S1 depletion led to a sharp decrease of the amount of pnp and other tested mRNAs, as detected by Northern blotting, whereas S1 overexpression caused a strong stabilization of pnp and the other transcripts. Surprisingly, mRNA stabilization depended on PNPase, as it was not observed in a pnp deletion strain. PNPase-dependent stabilization, however, was not detected by chemical decay assay of bulk mRNA. Overall, our data suggest that PNPase exonucleolytic activity may be modulated by the translation potential of the target mRNAs and that, upon ribosomal protein S1 overexpression, PNPase protects from degradation a set of full-length mRNAs. It thus appears that a single mRNA species may be differentially targeted to either decay or PNPase-dependent stabilization, thus preventing its depletion in conditions of fast turnover.

Published

2008

50. Genetic analysis of polynucleotide phosphorylase structure and functions

Author

Paolo Tortora, Gianni Dehò, Marta Del Favero, Luca De Gioia, Sandro Zangrossi, Claudio Greco, Rossana Capizzuto, Chiara Consonni, Federica Briani, Briani, F, Del Favero, M, Capizzuto, R, Consonni, C, Zangrossi, S, Greco, C, DE GIOIA, L, Tortora, P, and Deho, G

Subjects

Exonuclease, RNase P, RNA Stability, autogenous control, Gene Expression, Purine nucleoside phosphorylase, Biology, Settore BIO/19 - Microbiologia Generale, Polymerase Chain Reaction, Biochemistry, RNA degradation, Gene expression, Cold acclimation, Escherichia coli, PNPase, cold shock, RNA, Messenger, Polynucleotide phosphorylase, Polyribonucleotide Nucleotidyltransferase, Messenger RNA, RNA, General Medicine, Blotting, Northern, BIO/10 - BIOCHIMICA, Protein Structure, Tertiary, Cold Temperature, Settore BIO/18 - Genetica, Gene Expression Regulation, Mutation, biology.protein, Electrophoresis, Polyacrylamide Gel

Abstract

Polynucleotide phosphorylase (PNPase) is a phosphate-dependent 3' to 5' exonuclease widely diffused among bacteria and eukaryotes. The enzyme, a homotrimer, can also be found associated with the endonuclease RNase E and other proteins in a heteromultimeric complex, the RNA degradosome. PNPase negatively controls its own gene (pnp) expression by destabilizing pnp mRNA. A current model of autoregulation maintains that PNPase and a short duplex at the 5'-end of pnp mRNA are the only determinants of mRNA stability. During the cold acclimation phase autoregulation is transiently relieved and cellular pnp mRNA abundance increases significantly. Although PNPase has been extensively studied and widely employed in molecular biology for about 50 years, several aspects of structure-function relationships of such a complex protein are still elusive. In this work, we performed a systematic PCR mutagenesis of discrete pnp regions and screened the mutants for diverse phenotypic traits affected by PNPase. Overall our results support previous proposals that both first and second core domains are involved in the catalysis of the phosphorolytic reaction, and that both phosphorolytic activity and RNA binding are required for autogenous regulation and growth in the cold, and give new insights on PNPase structure-function relationships by implicating the alpha-helical domain in PNPase enzymatic activity. (c) 2006 Elsevier Masson SAS. All rights reserved.

Published

2007