Your search keyword '"Specific Pathogen-Free Organism"' showing total 5 results

1. Alteration of immunological parameters in infectious bronchitis vaccinated–specific pathogen-free broilers after the use of different infectious bursal disease vaccines

Author

Roberta Salaroli, Elena Catelli, Giulia Mescolini, Sara Boldini, Giulia Quaglia, Elisa Russo, Monica Forni, Caterina Lupini, Lupini C., Quaglia G., Mescolini G., Russo E., Salaroli R., Forni M., Boldini S., and Catelli E.

Subjects

infectious bursal disease virus, infectious bursal disease viru, vectored vaccine, Infectious bronchitis virus, Birnaviridae Infection, Infectious bursal disease, Bursa of Fabricius, lcsh:SF1-1100, 0303 health sciences, Viral Vaccine, Vaccination, 04 agricultural and veterinary sciences, General Medicine, Birnaviridae Infections, avian coronaviru, Chicken, Specific Pathogen-Free Organisms, Poultry Disease, Infectious bronchitis viru, Coronavirus Infections, avian coronavirus, animal structures, Newcastle disease virus, Biology, Vaccines, Attenuated, Newcastle disease, Article, 03 medical and health sciences, Immune system, medicine, Animals, Specific Pathogen-Free Organism, Poultry Diseases, 030304 developmental biology, Animal, Coronavirus Infection, Newcastle disease viru, 0402 animal and dairy science, Viral Vaccines, medicine.disease, biology.organism_classification, 040201 dairy & animal science, Virology, immune-complex vaccine, Bursa of Fabriciu, Animal Science and Zoology, lcsh:Animal culture, Chickens, Blood sampling

Abstract

The vaccines currently available to control infectious bursal disease (IBD) include live-attenuated and inactivated vaccines, immune-complex vaccines, and vaccines consisting of viral constructs of herpesvirus of turkeys genetically engineered to express VP2 surface protein. To evaluate the impact of vaccines on the chicken immune system, 2 animal trials were performed in specific pathogen-free broiler chickens. In trial 1, birds were either vaccinated when they are one-day old with a dual recombinant herpes virus of turkey construct vaccine, expressing VP2 protein of (IBDV) and F protein of Newcastle disease virus, or an immune-complex IBDV vaccine or birds were not vaccinated. At 14, 28, and 35 D, the bursa of Fabricius was collected for bursa:body weight (B:BW) ratio calculation. In trial 2, birds were vaccinated when they were 1-day old according to the same protocol as trial 1, but at day 14, all groups also received a live infectious bronchitis (IB) vaccine. At 0, 7, 14, 21, and 28 days after IB vaccination, birds were tested by ELISA for IB serology and, soon after the last blood sampling, they were euthanized for collection of Harderian glands, trachea, and spleen and testing by flow cytometry for characterization of mononuclear cells. The immune-complex vaccine groups showed significantly lower B:BW ratio, lower IBV antibody titers, and higher mean percentage of CD8+ T cells in the spleen, trachea, and Harderian glands than those in the other experimental groups. The results of the in vivo trials coupled with a depth analysis of the repertoire of parameters involved in the immune response to IBD and IB vaccinations show one vaccine may influence the immune response of other vaccines included in the vaccination program.

Published

2020

2. Inoculation of specific pathogen-free chickens with an infectious bursal disease virus of the ITA genotype (G6) leads to a high and persistent viral load in lymphoid tissues and to a delayed antiviral response

Author

Valeria Listorti, Viviana Felice, Giacomo Berto, Flavio Silveira, Elena Catelli, Mattia Cecchinato, Caterina Lupini, Giovanni Franzo, Giulia Mescolini, Silveira F., Felice V., Franzo G., Mescolini G., Catelli E., Cecchinato M., Berto G., Listorti V., and Lupini C.

Subjects

animal structures, Genotype, Lymphoid Tissue, Palatine Tonsil, Spleen, Enzyme-Linked Immunosorbent Assay, Biology, Virus Replication, Microbiology, Infectious Bursal Disease Virus, qRT-PCR, TLR-3, Virus distribution, Infectious bursal disease virus, Birnaviridae Infection, Palatine tonsil, Virus, Infectious bursal disease, 03 medical and health sciences, Bone Marrow, medicine, Specific Pathogen-Free Organism, Animals, Poultry Diseases, 030304 developmental biology, Specific-pathogen-free, 0303 health sciences, General Veterinary, Animal, 030306 microbiology, General Medicine, Viral Load, medicine.disease, Birnaviridae Infections, Chicken, Virology, Infectious Bursal Disease Viru, Specific Pathogen-Free Organisms, Toll-Like Receptor 3, Lymphatic system, medicine.anatomical_structure, Poultry Disease, Viral replication, Viral load, Chickens

Abstract

Infectious Bursal Disease Virus (IBDV) of the ITA genotype (G6) was shown to have peculiar molecular characteristics and, despite a subclinical course, aggressiveness towards lymphoid tissues after experimental infection of specific-pathogen-free (SPF) chickens. The aim of the present study was to evaluate and compare with a Classical IBDV strain, ITA IBDV distribution and persistence in various tissues (bursa of Fabricious, spleen, thymus, bone marrow, caecal tonsils, Harderian gland, kidney, liver and proventriculus), its cloacal shedding and the involvement of gut TLR-3 in duodenum tissues. The 35-day-old SPF chickens were experimentally infected and sampled up to 28 days post infection (dpi) for IBDV detection and TLR-3 quantification by qRT-PCR. The ITA IBDV strain was detected in lymphoid and most non-lymphoid tissues up to the end of the trial, with higher loads compared to the Classical IBDV. Most of those differences were found during the first 2 weeks post-infection. Notably, bone marrow and caecal tonsils presented higher viral loads until 28 dpi, allowing to speculate that these organs may serve as non-bursal lymphoid tissues supporting virus replication. Differences in relative TLR-3 gene expression between ITA IBDV-infected birds and Classical-IBDV infected ones were observed at 4, 14 and 21 dpi, being initially higher in Classical group and later in ITA group. Our results provide new insights into IBDV pathogenesis showing that IBDV of ITA genotype leads to a high and persistent viral load in lymphoid tissues and to a delayed antiviral response.

Published

2019

3. Immunosurveillance of the liver by intravascular effector CD8+ T cells

Author

Zaverio M. Ruggeri, Giovanni Sitia, Andrea Raimondi, Stefano Sammicheli, Maurizio Vacca, Donato Inverso, Masanori Isogawa, Matteo Iannacone, Ulrike Protzer, Jessica Fioravanti, Luca G. Guidotti, Amleto Fiocchi, Marta Mainetti, Gloria González-Aseguinolaza, Tiziana Cataudella, Laura Sironi, Lucia Ganzer, Pietro Di Lucia, Roberto Aiolfi, Francis V. Chisari, Guidotti, L, Inverso, D, Sironi, L, Di Lucia, P, Fioravanti, J, Ganzer, L, Fiocchi, A, Vacca, M, Aiolfi, R, Sammicheli, S, Mainetti, M, Cataudella, T, Raimondi, A, Gonzalez Aseguinolaza, G, Protzer, U, Ruggeri, Z, Chisari, F, Isogawa, M, Sitia, G, Iannacone, M, Guidotti, Luca G., Inverso, Donato, Sironi, Laura, Di Lucia, Pietro, Fioravanti, Jessica, Ganzer, Lucia, Fiocchi, Amleto, Vacca, Maurizio, Aiolfi, Roberto, Sammicheli, Stefano, Mainetti, Marta, Cataudella, Tiziana, Raimondi, Andrea, Gonzalez-Aseguinolaza, Gloria, Protzer, Ulrike, Ruggeri, Zaverio M., Chisari, Francis V., Isogawa, Masanori, Sitia, Giovanni, and Iannacone, Matteo

Subjects

Liver Cirrhosis, Hepatitis B virus, Liver Cirrhosi, CD8-Positive T-Lymphocytes, Biology, General Biochemistry, Genetics and Molecular Biology, Pathogenesis, Mice, Platelet Adhesiveness, Antigen, Cell Movement, Monitoring, Immunologic, medicine, Animals, Specific Pathogen-Free Organism, Cytotoxic T cell, Hepatocyte, Hyaluronic Acid, Platelet Adhesivene, Endothelial Cell, Biochemistry, Genetics and Molecular Biology (all), Effector, Biochemistry, Genetics and Molecular Biology(all), Animal, CD44, Endothelial Cells, CD8-Positive T-Lymphocyte, Hepatitis B viru, Hepatitis B, medicine.disease, 3. Good health, Cell biology, Specific Pathogen-Free Organisms, Immunosurveillance, Mice, Inbred C57BL, Liver, Immunology, Hepatocytes, biology.protein, CD8

Abstract

SummaryEffector CD8+ T cells (CD8 TE) play a key role during hepatotropic viral infections. Here, we used advanced imaging in mouse models of hepatitis B virus (HBV) pathogenesis to understand the mechanisms whereby these cells home to the liver, recognize antigens, and deploy effector functions. We show that circulating CD8 TE arrest within liver sinusoids by docking onto platelets previously adhered to sinusoidal hyaluronan via CD44. After the initial arrest, CD8 TE actively crawl along liver sinusoids and probe sub-sinusoidal hepatocytes for the presence of antigens by extending cytoplasmic protrusions through endothelial fenestrae. Hepatocellular antigen recognition triggers effector functions in a diapedesis-independent manner and is inhibited by the processes of sinusoidal defenestration and capillarization that characterize liver fibrosis. These findings reveal the dynamic behavior whereby CD8 TE control hepatotropic pathogens and suggest how liver fibrosis might reduce CD8 TE immune surveillance toward infected or transformed hepatocytes.

Published

2015

4. Mast Cells Infiltrating Inflamed or Transformed Gut Alternatively Sustain Mucosal Healing or Tumor Growth

Author

Alice Rigoni, Amy Lewis, Mario P. Colombo, Andrew Silver, Carla Guarnotta, Alessia Burocchi, Aroldo Rizzo, Sabina Sangaletti, Claudio Tripodo, Luca Danelli, Lucia Bongiovanni, Rigoni, A., Bongiovanni, L., Burocchi, A., Sangaletti, S., Danelli, L., Guarnotta, C., Lewis, A., Rizzo, A., Silver, A., Tripodo, C., and Colombo, M.

Subjects

Cancer Research, Pathology, Colorectal cancer, Cell Count, Animals, Animals, Congenic, Azoxymethane, Carcinoma, Cell Transformation, Neoplastic, Cells, Cultured, Colitis, Colonic Neoplasms, Dextran Sulfate, Epithelial Cells, Humans, Inflammatory Bowel Diseases, Interleukin-33, Intestinal Mucosa, Mast Cells, Mice, Mice, Inbred C57BL, Mice, Knockout, Models, Biological, Proto-Oncogene Proteins c-kit, Receptors, Interleukin, Regeneration, Serine Endopeptidases, Species Specificity, Specific Pathogen-Free Organisms, Oncology, Medicine (all), chemistry.chemical_compound, Mast Cell, Colonic Neoplasm, Intestinal epithelium, Serine Endopeptidase, medicine.symptom, Human, medicine.medical_specialty, Inflammation, Immune system, medicine, Specific Pathogen-Free Organism, Epithelial Cell, Animal, business.industry, Inflammatory Bowel Disease, medicine.disease, Interleukin-1 Receptor-Like 1 Protein, chemistry, business, Wound healing, Coliti, Homeostasis

Abstract

Mast cells (MC) are immune cells located next to the intestinal epithelium with regulatory function in maintaining the homeostasis of the mucosal barrier. We have investigated MC activities in colon inflammation and cancer in mice either wild-type (WT) or MC-deficient (KitW-sh) reconstituted or not with bone marrow-derived MCs. Colitis was chemically induced with dextran sodium sulfate (DSS). Tumors were induced by administering azoxymethane (AOM) intraperitoneally before DSS. Following DSS withdrawal, KitW-sh mice showed reduced weight gain and impaired tissue repair compared with their WT littermates or KitW-sh mice reconstituted with bone marrow-derived MCs. MCs were localized in areas of mucosal healing rather than damaged areas where they degraded IL33, an alarmin released by epithelial cells during tissue damage. KitW-sh mice reconstituted with MC deficient for mouse mast cell protease 4 did not restore normal mucosal healing or reduce efficiently inflammation after DSS withdrawal. In contrast with MCs recruited during inflammation-associated wound healing, MCs adjacent to transformed epithelial cells acquired a protumorigenic profile. In AOM- and DSS-treated WT mice, high MC density correlated with high-grade carcinomas. In similarly treated KitW-sh mice, tumors were less extended and displayed lower histologic grade. Our results indicate that the interaction of MCs with epithelial cells is dependent on the inflammatory stage, and on the activation of the tissue repair program. Selective targeting of MCs for prevention or treatment of inflammation-associated colon cancer should be timely pondered to allow tissue repair at premalignant stages or to reduce aggressiveness at the tumor stage. Cancer Res; 75(18); 3760–70. ©2015 AACR.

Published

2014

5. Mini-FLOTAC for counting Toxoplasma gondii oocysts from cat feces--comparison with cell counting plates

Author

Catherine Perret, Olgica Djurković-­Djaković, Delphine Le Roux, Tamara Ducry, Maria Paola Maurelli, Laura Rinaldi, Radu Blaga, Giuseppe Cringoli, Pascal Boireau, Vitomir Djokic, Djokic, Vitomir, Blaga, Radu, Rinaldi, Laura, Le Roux, Delphine, Ducry, Tamara, Maurelli, MARIA PAOLA, Perret, Catherine, Djurkovic Djakovic, Olgica, Cringoli, Giuseppe, and Boireau, Pascal

Subjects

Veterinary medicine, Serial dilution, Cost effectiveness, Immunology, Toxoplasma gondii, Cat Diseases, Sensitivity and Specificity, Microbiology, Oocyst, Feces, Mice, parasitic diseases, medicine, Specific Pathogen-Free Organism, Mini-FLOTAC, Animals, Kova slide, Parasite Egg Count, biology, Animal, Oocysts, Cat, General Medicine, biology.organism_classification, Cell counting, medicine.disease, Cat Disease, Toxoplasmosis, 3. Good health, Specific Pathogen-Free Organisms, Detection, Infectious Diseases, Toxoplasmosis, Animal, Cats, Parasitology, Fece, Toxoplasma, Field conditions

Abstract

Oocysts of Toxoplasma gondii represent one of the most common environmental contaminants causing the zoonotic infection toxoplasmosis. The aim of the present study was to compare the Mini-FLOTAC device with traditional cell counting plates (Kova Slide) for the detection of T. gondii oocysts from feline feces. Two types of experiments were performed: (i) purified oocysts were counted in different dilutions and (ii) specific pathogen free T. gondii -negative cat feces was inoculated with numbers of purified oocysts and counting was performed directly from feces. Our analysis showed a thousand times higher sensitivity of Mini-FLOTAC (5 × 10 2 oocysts) compared to Kova Slide (5 × 10 5 oocysts). Also, when compared by McNemar's test, counting of the purified oocysts showed a higher sensitivity of Mini-FLOTAC compared to Kova Slide, for a dilution of 10 3 oocysts/ml (chi 2 = 6.1; P 0.05). A better sensitivity was also found with Mini-FLOTAC in dilutions of 10 5 and 10 4 oocysts/ml, when counted from feces (chi 2 = 4.2 and 8.1, respectively, P 0.05). Our results show that Mini-FLOTAC is more sensitive than traditional methods of T. gondii oocysts detection and quantification is more accurate. Furthermore, Mini-FLOTAC simplicity and cost effectiveness allow it to be used with light microscopes in any laboratory or field conditions. We therefore recommend its use for regular screening. Further studies are needed to validate Mini-FLOTAC for the detection of oocysts in soil and water samples in field conditions.

Published

2014