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6. The prophenoloxidase system is activated during the tunic inflammatory reaction of Ciona intestinalis

Author

C. Cianciolo, Mirella Vazzana, Daniela Parrinello, Aiti Vizzini, Matteo Cammarata, Vincenzo Arizza, Giuseppina Salerno, Nicolò Parrinello, CAMMARATA, M, ARIZZA, V, CIANCIOLO COSENTINO, C, PARRINELLO, D, VAZZANA, M, VIZZINI, A, SALERNO, G, PARRINELLO, N, and CIANCIOLO, C

Subjects
Lipopolysaccharides, Proteases, Histology, Blotting, Western, Settore BIO/05 - Zoologia, Enzyme-Linked Immunosorbent Assay, Pathology and Forensic Medicine, medicine, Animals, Ciona intestinalis, Inflammation, chemistry.chemical_classification, Enzyme Precursors, biology, Kunitz STI protease inhibitor, prophenoloxidase, Ciona intestinalis, Cell Biology, Prophenoloxidase, biology.organism_classification, Trypsin, Immunohistochemistry, Molecular biology, In vitro, Up-Regulation, Ciona, Enzyme, chemistry, Phenoloxidase . Hemocyte . Tunic . Inflammation . Lipopolysaccharide . SDS-polyacrylamide gel electrophoresis . Ciona intestinalis, Electrophoresis, Polyacrylamide Gel, Catechol Oxidase, medicine.drug
Abstract

Phenoloxidase (PO) activity was examined in the tunic tissue of Ciona intestinalis following lipopolysaccharide (LPS) intratunic injection. Tunic homogenate supernatant (THS), assayed with the Dopa-MBTH reaction, displayed Ca(2+)-independent PO activity that was raised by LPS and further enhanced by proteases. Specific inhibitors (tropolone, phenylthiourea, diethylthiocarbamate) supported the specificity of the reaction. Assay with soybean trypsin inhibitor showed that, in the tunic, PO activation with trypsin was not significantly inhibited suggesting that proteases diverse from serine proteases were involved. In vivo experiments were carried out by injecting isosmotic medium or LPS, and THS was assayed for its PO activity. Analysis of variance of the time-course profiles showed that LPS was more effective in activating proPO. To disclose the PO response at the injured site, an assay with Dopa-MBTH was performed in vitro. Quinones were mainly contained in the tunic matrix enriched with inflammatory cells around the injection site. Microscopic observations and immunohistochemistry with anti-CinPO-2 antibodies showed granulocytes and unilocular refractile granulocytes containing PO, whereas few morula cells were stained. In THS zymograms (SDS-polyacrylamide gel electrophoresis), PO activity linked to 90-kDa and 120-kDa bands was observed as an effect of LPS injection, whereas the density of 170-kDa PO was weak. A third presumptive PO enzyme (CinPO-3) containing the CinPO-2 peptide was identified in the recent Ciona genome version. Presumably, LPS stimulated the production and dimerization (120 kDa) of CinPO-3 (66 kDa). Thus, the activated proPO system includes several POs that are distinguishable by size and that are contained and presumably released by tunic inflammatory cells and hemocytes of the pharynx bars.

Published
2008
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7. Cloning and expression of a novel component of the CAP superfamily enhanced in the inflammatory response to LPS of the ascidian Ciona intestinalis

Author

Aiti Vizzini, Giuseppina Salerno, Paolo Colombo, Daniela Parrinello, Angela Bonura, Valeria Longo, Nicolò Parrinello, Giovanna Montana, Bonura, A, Vizzini, A, Salerno, G, Parrinello, D, Parrinello, N, Longo, V, Montana, G, and Colombo, P

Subjects
Lipopolysaccharides, Histology, Hemocytes, Sequence analysis, In silico, Molecular Sequence Data, Settore BIO/05 - Zoologia, Sequence alignment, Polymerase Chain Reaction, Pathology and Forensic Medicine, Complementary DNA, Animals, Ciona intestinalis, Amino Acid Sequence, RNA, Messenger, Cloning, Molecular, Gene, Peptide sequence, In Situ Hybridization, Phylogeny, Inflammation, Messenger RNA, biology, Base Sequence, Sequence Homology, Amino Acid, Proteins, Cell Biology, Sequence Analysis, DNA, biology.organism_classification, Molecular biology, Innate immune system, differential display CAP protein, molecular biology, ciona intestinalis (Tunicata), Sequence Alignment
Abstract

The CAP superfamily is a group of proteins that have been linked to several biological functions such as reproduction, cancer, and immune defense. A differential screening between lipopolysaccharide (LPS)-challenged and naive Ciona intestinalis has been performed to identify LPS-induced genes. This strategy has allowed the isolation of a full-length 1471-bp cDNA encoding for a 413-amino-acid protein (CiCAP). In silico analysis has shown that this polypeptide displays a modular structure with similarities to vertebrate CAP-superfamily proteins and to a collagen-binding adhesin of Streptococcus mutans. Domain organization analysis and alignment of CiCAP to other vertebrate CAP proteins have revealed a novel structure suggesting that this protein originated from a common ancestor gene that gave rise to many subfamilies of mosaic proteins with novel functions. Quantitative mRNA expression performed by real-time polymerase chain reaction analysis has demonstrated that this gene is rapidly activated in the pharynx of C. intestinalis a few hours after LPS injection. Moreover, in situ hybridization has shown that CiCAP mRNA is highly expressed by hemocytes with large granules contained inside the pharynx vessels. Thus, CiCAP represents a protein with novel structural domains involved in ascidian immune responses.

Published
2010

8. Inflamed adult pharynx tissues and swimming larva of Ciona intestinalis share CiTNFalpha-producing cells

Author

Maria Antonietta Sanfratello, Matteo Cammarata, Vincenzo Arizza, Mirella Vazzana, Aiti Vizzini, Nicolò Parrinello, Giuseppina Salerno, Daniela Parrinello, Parrinello, N, Vizzini, A, Salerno, G, Sanfratello, MA, Cammarata, M, Arizza, V, Vazzana, M, and Parrinello, D

Subjects
Lipopolysaccharides, Pathology, medicine.medical_specialty, Histology, Hemocytes, Endothelium, Evolution, Mesenchyme, Settore BIO/05 - Zoologia, Inflammation, In situ hybridization, Biology, Ascidia, Ciona intestinalis, Pathology and Forensic Medicine, medicine, Animals, Ciona intestinalis, Tumour necrosis factor, Pharynx, Haemocytes, Larval development, Innate immunity, In Situ Hybridization, Fluorescence, Phylogeny, Innate immune system, Tumor Necrosis Factor-alpha, Metamorphosis, Biological, Haemocyte, Pharyngitis, Cell Biology, biology.organism_classification, Immunohistochemistry, medicine.anatomical_structure, Larva, medicine.symptom, Granulocytes
Abstract

In situ hybridisation and immunohistochemistry analyses have shown that the Ciona intestinalis tumour necrosis factor alpha gene (CiTNFalpha), which has been previously cloned and sequenced, is expressed either during the inflammatory pharynx response to lipopolysaccharide (LPS) or during the swimming larval phase of development. Granulocytes with large granules and compartment/morula cells are CiTNFalpha-producing cells in both inflamed pharynx and larvae. Pharynx vessel endothelium also takes part in the inflammatory response. Haemocyte nodules in the vessel lumen or associated with the endothelium suggest the involvement of CiTNFalpha in recruiting lymphocyte-like cells and promoting the differentiation of inflammatory haemocytes. Specific antibodies against a CiTNFalpha peptide have identified a 43-kDa cell-bound form of the protein. Observations of pharynx histological sections (at 4 and 8 h post-LPS inoculation) from naive and medium-inoculated ascidians have confirmed the CiTNFalpha-positive tissue response. Larval histological sections and whole-mount preparations have revealed that CiTNFalpha is expressed by trunk mesenchyme, preoral lobe and tunic cells, indicating CiTNFalpha-expressing cell immigration events and an ontogenetic role.

Published
2010

9. Glucocorticoid receptor (DlGR1) is expressed in pre-larval and larval stages of the teleost fish Dicentrarchus labrax

Author

Mirella Vazzana, M. L. Di Bella, Aiti Vizzini, Nicolò Parrinello, DI BELLA, ML, VAZZANA ,M, VIZZINI, A, and PARRINELLO, N

Subjects
Fish Proteins, Histology, Settore BIO/05 - Zoologia, Gene Expression, In situ hybridization, Glucocorticoid receptor, Biology, Article, Pathology and Forensic Medicine, Receptors, Glucocorticoid, Complementary DNA, Gene expression, Animals, Dicentrarchus labrax (Teleostei), Larval development . Glucocorticoid receptor . In situ hybridization . Immunohistochemistry . Dicentrarchus labrax (Teleostei, Receptor, Peptide sequence, Riboprobe, Cell Biology, Molecular biology, Immunohistochemistry, Nuclear receptor, Larva, Larval development, Bass
Abstract

Glucocorticoid hormone receptors (GR), members of the nuclear hormone receptor superfamily, are ligand-dependent transcription factors expressed in various tissues by binding to specific DNA sequences. Since glucocorticoids have a role in maintaining the homeostatic status in fish, we previously cloned and sequenced a GR (DlGR1) of adult Dicentrarchus labrax; we also showed mRNA expression (in situ hybridization) and tissue immunohistochemical localization of DlGR1 in several organs. This work has now been extended to the examination of the expression, tissue distribution, and cytolocalization of DlGR1 in larval developmental stages by similar methods to those used for the adult organs. The riboprobe included the DlGR1 cDNA transcriptional activation domain (1.0–1,300 nucleotide sequence) showing no significant similarity with a known second GR cDNA sequence of sea bass. The antibody was specific for an opportunely selected peptide sequence of the DlGR1 transcriptional domain. In histological sections of brain, head kidney, gills, liver, anterior intestine, and spleen cells, the riboprobe was mainly located in the cell nucleus. The antibody identified DlGR1 in the head kidney, gills, liver, and anterior intestine, mainly located in the cytosol. These results are in agreement with the receptor location in adult tissues. The greater presence of both the transcript and protein of DlGR1 in the late developmental stages suggests an increasing expression of this receptor. The cytolocalization (nuclear-cytosolic) and presumptive roles of DlGR1-containing tissues are discussed.

Published
2007

10. Inducible lectins with galectin properties and human IL1alpha epitopes opsonize yeast during the inflammatory response of the ascidian Ciona intestinalis

Author

Francesca Tiziana Giaramita, Vincenzo Arizza, Aiti Vizzini, Daniela Parrinello, Nicolò Parrinello, Margherita Pergolizzi, Mirella Vazzana, Matteo Cammarata, PARRINELLO, N, ARIZZA, V, CAMMARATA, M, GIARAMITA, FT, PERGOLIZZI, M, VAZZANA, M, VIZZINI, A, and PARRINELLO, D

Subjects
Lipopolysaccharides, Histology, Lipopolysaccharide, Galectins, Saccharomyces cerevisiae, Cross Reactions, Epitope, Evolution . Inflammatory response . Phagocytosis . Opsonins . Lectins . IL1α-like galectins . Ascidian, Ciona intestinalis (Tunicata), Antibodies, Pathology and Forensic Medicine, law.invention, chemistry.chemical_compound, Epitopes, Western blot, Phagocytosis, Opsonin Proteins, law, Hemolymph, Interleukin-1alpha, Lectins, medicine, Animals, Humans, Ciona intestinalis, Galectin, biology, medicine.diagnostic_test, Galactose, Galactosides, Cell Biology, Blood Proteins, biology.organism_classification, Molecular biology, Blood proteins, Recombinant Proteins, Hemagglutinins, Biochemistry, chemistry, Recombinant DNA, Calcium, Rabbits
Abstract

Studies on inducible ascidian lectins may shed light on the evolutionary emergence of cytokine functions. Here, we show that the levels of opsonins, with IL1alpha-epitopes, increase in Ciona intestinalis hemolymph as a response to an inflammatory stimulus and, in particular, to intratunic injection of lipopolysaccharide (LPS). The inflammatory agent promptly (within 4 h) enhances Ca(2+)-independent serum hemagglutinating and opsonizing activities, which are both inhibited by D-galactose and D-galactosides (alpha-lactose, N-acetyl-D-lactosamine, thio-digalactoside), suggesting that anti-rabbit erythrocyte lectins with galectin properties are involved as opsonins. Inducible galectin molecules contain interleukin-1alpha (IL1alpha) epitopes, and their activities are specifically inhibited by anti-human recombinant IL1alpha antibody. Analysis by SDS-polyacrylamide gel electrophoresis has revealed that the density of the bands of several serum proteins increases within 4 h after LPS injection, correlated with the enhanced serum activity. Moreover, Western blot patterns demonstrate that several serum proteins (59, 37, 30, 23, 15 kDa) cross-react with the antibody as early as 4 h post-injection. Although we have not been able to establish whether, in adition to galectins, various types of D-galactose-specific lectins are contained in the serum, we show, for the first time in invertebrates, that galectin molecules with opsonic properties can be enhanced in response to a non-specific inflammatory stimulus, and that their release can be further stimulated by LPS. Finally, we reveal that multiple galectins share human IL1alpha epitopes, probably because of steric configuration and the oligomerization process.

Published
2006

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