Your search keyword '"Colombatti M"' showing total 11 results

1. Comparative analysis of monoclonal antibodies against prostate-specific membrane antigen (PSMA).

Author

Tykvart J, Navrátil V, Sedlák F, Corey E, Colombatti M, Fracasso G, Koukolík F, Bařinka C, Sácha P, and Konvalinka J

Subjects

Adenocarcinoma diagnosis, Adenocarcinoma metabolism, Blotting, Western, Cell Line, Tumor, Enzyme-Linked Immunosorbent Assay, Epitope Mapping, Flow Cytometry, Humans, Immunohistochemistry, Male, Prostate-Specific Antigen metabolism, Prostatic Neoplasms diagnosis, Prostatic Neoplasms metabolism, Adenocarcinoma immunology, Antibodies, Monoclonal analysis, Antibodies, Monoclonal immunology, Prostate-Specific Antigen immunology, Prostatic Neoplasms immunology

Abstract

Background: Prostate-specific membrane antigen (PSMA), also known as glutamate carboxypeptidase II (GCPII), is generally recognized as a diagnostic and therapeutic cancer antigen and a molecular address for targeted imaging and drug delivery studies. Due to its significance in cancer research, numerous monoclonal antibodies (mAbs) against GCPII have been described and marketed in the past decades. Unfortunately, some of these mAbs are poorly characterized, which might lead to their inappropriate use and misinterpretation of the acquired results., Methods: We collected the 13 most frequently used mAbs against GCPII and quantitatively characterized their binding to GCPII by enzyme-linked immunosorbent assay (ELISA) and surface plasmon resonance (SPR). Using a peptide library, we mapped epitopes recognized by a given mAb. Finally, we assessed the applicability of these mAbs to routine experimental setups, including Western blotting, immunohistochemistry, and flow cytometry., Results: ELISA and SPR analyses revealed that mAbs J591, J415, D2B, 107-1A4, GCP-05, and 2G7 bind preferentially to GCPII in native form, while mAbs YPSMA-1, YPSMA-2, GCP-02, GCP-04, and 3E6 bind solely to denatured GCPII. mAbs 24.4E6 and 7E11-C5.3 recognize both forms of GCPII. Additionally, we determined that GCP-02 and 3E6 cross-react with mouse GCPII, while GCP-04 recognizes GCPII and GCPIII proteins from both human and mouse., Conclusion: This comparative analysis provides the first detailed quantitative characterization of the most commonly used mAbs against GCPII and can serve as a guideline for the scientific community to use them in a proper and efficient way., (© 2014 Wiley Periodicals, Inc.)

Published

2014

2. Cloning and characterization of canine prostate-specific membrane antigen.

Author

Schmidt S, Fracasso G, Colombatti M, and Naim HY

Subjects

Amino Acid Sequence, Animals, Antigens, Surface chemistry, Biomarkers, Tumor chemistry, Biomarkers, Tumor genetics, Biomarkers, Tumor metabolism, COS Cells, Cell Membrane metabolism, Chlorocebus aethiops, Dogs, Endoplasmic Reticulum metabolism, Glutamate Carboxypeptidase II chemistry, Glycosylation, Golgi Apparatus metabolism, Green Fluorescent Proteins genetics, Humans, Madin Darby Canine Kidney Cells, Male, Molecular Sequence Data, Prostatic Neoplasms metabolism, Protein Structure, Quaternary, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, Sequence Homology, Amino Acid, Species Specificity, Transfection, Translational Research, Biomedical, Antigens, Surface genetics, Antigens, Surface metabolism, Cloning, Molecular methods, Glutamate Carboxypeptidase II genetics, Glutamate Carboxypeptidase II metabolism, Prostatic Neoplasms genetics, Protein Transport physiology

Abstract

Background: Prostate-specific membrane antigen (PSMA) is a promising biomarker in the diagnosis of prostate cancer and a potential target for antibody-based therapeutic strategies. We isolated the canine PSMA cDNA and investigated the cellular and biochemical characteristics of the recombinant protein as a potential target for animal preclinical studies of antibody based-therapies., Methods: Canine PSMA cDNA was isolated by PCR, cloned into expression vectors and transfected into COS-1 and MDCK cells. The biosynthesis and glycosylation of the recombinant protein were investigated in pulse-chase experiments, the cellular localization by confocal laser microscopy, the mode of association of PSMA with the membrane with solubilization in different detergents and its quaternary structure in sucrose-density gradients., Results: Canine PSMA shows 91% amino acid homology to human PSMA, whereby the major difference is a longer cytoplasmic tail of canine PSMA compared to its human counterpart. Canine PSMA is trafficked efficiently along the secretory pathway, undergoes homodimerization when it acquires complex glycosylated mature form. It associates with detergent-resistant membranes, which act as platforms along its intracellular trafficking. Confocal analysis revealed canine PSMA at the cell surface, Golgi, and the endoplasmic reticulum. A similar distribution is revealed for human PSMA, yet with reduced cell surface levels., Conclusions: The cloning, expression, biosynthesis, processing and localization of canine PSMA in mammalian cells is described. We demonstrate that canine PSMA reveals similar characteristics to human PSMA rendering this protein useful as a translational model for investigations of prostate cancer as well as a suitable antigen for targeted therapy studies in dogs., (Copyright © 2013 Wiley Periodicals, Inc.)

Published

2013

3. Lymphocyte phenotypic subsets in umbilical cord blood compared to peripheral blood from related mothers.

Author

Chirumbolo S, Ortolani R, Veneri D, Raffaelli R, Peroni D, Pigozzi R, Colombatti M, and Vella A

Subjects

Adult, Antigens, CD metabolism, Female, Humans, Leukocyte Count, Mothers, Phenotype, Fetal Blood cytology, Lymphocytes metabolism

Published

2011

4. N-terminal deletion affects catalytic activity of saporin toxin.

Author

Bonini F, Traini R, Comper F, Fracasso G, Tomazzolli R, Dalla Serra M, and Colombatti M

Subjects

Catalysis, Cell Line, Tumor, Colorimetry, Humans, Immunotoxins chemistry, Immunotoxins genetics, Immunotoxins toxicity, Membranes, Artificial, Mutation genetics, Protein Biosynthesis drug effects, Protein Isoforms chemistry, Protein Isoforms genetics, Protein Isoforms metabolism, Protein Isoforms toxicity, Protein Structure, Secondary, Substrate Specificity, Gene Deletion, Immunotoxins metabolism

Abstract

Single-chain ribosome inactivating proteins (RIPs) are cytotoxic components of macromolecular pharmaceutics for immunotherapy of cancer and other human diseases. Saporin belongs to a family of single-chain RIPs sharing sequence and structure homology. In a preliminary attempt to define an active saporin polypeptide of minimum size we have generated proteins with deletions at the N-terminus and at the C-terminus. An N-terminal (sapDelta1-20) deletion mutant of saporin displayed defective catalytic activity, drastically reduced cytotoxicity but increased ability to interact with liposomes inducing their permeabilization at low pH. A C-terminal (sapDelta239-253) deletion mutant showed instead a moderate reduction in cytotoxic activity. A substantial alteration of secondary structure was evidenced by Fourier transformed infrared spectroscopy (FTIR) in the sapDelta1-20 mutant. It can be hypothesized that the defective functions of sapDelta1-20 are due to alterations of its spatial configuration., ((c) 2006 Wiley-Liss, Inc.)

Published

2006

5. Anti-tumor effects of toxins targeted to the prostate specific membrane antigen.

Author

Fracasso G, Bellisola G, Cingarlini S, Castelletti D, Prayer-Galetti T, Pagano F, Tridente G, and Colombatti M

Subjects

Antibodies, Monoclonal therapeutic use, Bone Neoplasms secondary, Carboxypeptidases immunology, Glutamate Carboxypeptidase II, Humans, Immunotoxins immunology, Male, Ricin administration & dosage, Tumor Cells, Cultured, Antigens, Surface, Carboxypeptidases pharmacology, Carcinoma pathology, Immunotoxins pharmacology, Prostatic Neoplasms pathology, Ricin pharmacology

Abstract

Background: There is presently no effective therapy for relapsing, metastatic, androgen-independent prostate cancer. Immunotherapy with monoclonal antibody-vehicled toxins (Immunotoxins, ITs) may be a promising novel treatment option for the management of prostate cancer in these cases., Methods: Three anti-prostate specific membrane antigen (anti-PSMA) monoclonals (J591, PEQ226.5, and PM2P079.1) were cross-linked to ricin A-chain (RTA; native or recombinant), and their cytotoxic effects were investigated in monolayer and three-dimensional (3-D) cell cultures of prostate carcinoma cells (LNCaP)., Results: The various Immunotoxins showed effects in the nanomolar range (IC(50s) of 1.6-99 ng/ml) against PSMA+ cells (IC(50) being the concentration inhibiting 50% cell proliferation or protein synthesis). PSMA(-) cell lines were 62- to 277-fold less sensitive to anti-PSMA ITs, evidencing an appreciable therapeutic window. Treatment with J591-smpt-nRTA (0.35-31.7ng/ml) resulted in complete eradication of 3-D tumor micromasses or in 1.46- to 0.35-log reduction of target cells number, depending on the dose., Conclusion: Anti-PSMA ITs appear to be promising for use in the eradication of small prostate tumor cell aggregates present in tissues and in the bone marrow., (Copyright 2002 Wiley-Liss, Inc.)

Published

2002

6. Human MBP-specific T cells regulate IL-6 gene expression in astrocytes through cell-cell contacts and soluble factors.

Author

Colombatti M, Moretto G, Tommasi M, Fiorini E, Poffe O, Colombara M, Tanel R, Tridente G, and Ramarli D

Subjects

Astrocytes metabolism, Binding Sites drug effects, Binding Sites physiology, Cell Adhesion immunology, Cells, Cultured drug effects, Cells, Cultured immunology, Cells, Cultured metabolism, Cloning, Molecular, DNA-Binding Proteins drug effects, DNA-Binding Proteins immunology, DNA-Binding Proteins metabolism, Fetus, Humans, Integrin beta1 drug effects, Integrin beta1 immunology, Integrin beta1 metabolism, Interferon Regulatory Factor-1, Interferon-gamma pharmacology, Interleukin-6 metabolism, Multiple Sclerosis genetics, Multiple Sclerosis physiopathology, NF-kappa B metabolism, Phenotype, Phosphoproteins drug effects, Phosphoproteins immunology, Phosphoproteins metabolism, Phosphorylation drug effects, STAT1 Transcription Factor, T-Lymphocytes metabolism, Trans-Activators drug effects, Trans-Activators metabolism, Transcription, Genetic drug effects, Transcription, Genetic immunology, Up-Regulation drug effects, Up-Regulation immunology, Astrocytes immunology, Cell Communication immunology, Gene Expression Regulation immunology, Interleukin-6 genetics, Multiple Sclerosis immunology, Myelin Basic Protein immunology, T-Lymphocytes immunology

Abstract

One of the distinctive features of multiple sclerosis (MS) attacks is homing to the CNS of activated T cells able to orchestrate humoral and cell-based events, resulting in immune-mediated injury to myelin and oligodendrocytes. Of the complex interplay occurring between T cells and CNS constituents, we have examined some aspects of T-cell interactions with astrocytes, the major components of the glial cells. Specifically, we focused on the ability of T cells to regulate the gene expression of interleukin-6 (IL-6) in astrocytes, based on previous evidence showing the involvement of this cytokine in CNS disorders. We found that T-cell adhesion and T-cell soluble factors induce IL-6 gene expression in U251 astrocytes through distinct signaling pathways, respectively, resulting in the activation of NF-kappaB and IRF-1 transcription factors. In a search for effector molecules at the astrocyte surface, we found that alpha3beta1 integrins play a role in NF-kappaB activation induced by T-cell contact, whereas interferon-gamma (IFN-gamma) receptors dominate in IRF-1 induction brought about by T-cell-derived soluble factors. Similar phenomena were observed also in normal fetal astrocyte cultures. We therefore propose that through astrocyte induction, T cells may indirectly regulate the availability of a cytokine which is crucial in modulating fate and behavior of cell populations involved in the pathogenesis of MS inflammatory lesions., (Copyright 2001 Wiley-Liss, Inc.)

Published

2001

7. Genetic grafting of membrane-acting peptides to the cytotoxin dianthin augments its ability to de-stabilize lipid bilayers and enhances its cytotoxic potential as the component of transferrin-toxin conjugates.

Author

Lorenzetti I, Meneguzzi A, Fracasso G, Potrich C, Costantini L, Chiesa E, Legname G, Menestrina G, Tridente G, and Colombatti M

Subjects

Humans, Hydrogen-Ion Concentration, Jurkat Cells, Membranes, Artificial, Monensin pharmacology, Ribosome Inactivating Proteins, Type 1, Immunotoxins pharmacology, Lipid Bilayers, Plant Proteins pharmacology, Recombinant Fusion Proteins pharmacology, Transferrin pharmacology

Abstract

Three chimeric proteins were obtained by fusing together the dianthin gene and DNA fragments encoding for the following membrane-acting peptides: the N-terminus of protein G of the vesicular stomatitis virus (KFT25), the N terminus of the HA2 hemagglutinin of influenza virus (pHA2), and a membrane-acting peptide (pJVE). Chimeric dianthins (KFT25DIA, pHA2DIA and pJVEDIA) retained full enzymatic activity in cell-free assays and showed increased ability to induce pH-dependent calcein release from large unilamellar vesicles (LUVs). pHA2DIA and pJVEDIA also showed faster kinetics of interaction with LUVs, while KFT25DIA and pHA2DIA displayed a reduced cytotoxicity as compared to wild-type dianthin. Conjugates made by chemically cross-linking KFT25DIA or pJVEDIA and human transferrin (Tfn) showed greater cell-killing efficiency than conjugates of Tfn and wild-type dianthin. As a consequence, by fusion of membrane-acting peptides to the dianthin sequence the specificity factor (i.e., the ratio between non-specific and specific toxicity) of Tfn-KFT25DIA, Tfn-pHA2DIA and Tfn-pJVEDIA was increased with respect to that of Tfn-based conjugates made with wild-type dianthin. Taken together, our results suggest that genetic fusion of membrane-acting peptides to enzymatic cytotoxins results in the acquisition of new physico-chemical properties exploitable for designing new recombinant cytotoxins and to tackle cell-intoxication mechanisms., (Copyright 2000 Wiley-Liss, Inc.)

Published

2000

8. Escape mechanisms of human leukemic cells to long-term immunotoxin treatment in an in vitro experimental model.

Author

Chignola R, Pasti M, Candiani C, Franceschi A, Anselmi C, Tridente G, and Colombatti M

Subjects

Antibodies, Monoclonal pharmacokinetics, Antibodies, Monoclonal therapeutic use, CD5 Antigens, Cell Death drug effects, Cell Division drug effects, Drug Resistance physiology, Evaluation Studies as Topic, Humans, Tumor Cells, Cultured, Antigens, CD immunology, Immunotoxins pharmacokinetics, Immunotoxins therapeutic use, Leukemia, Lymphoid drug therapy, Leukemia, Lymphoid metabolism, Ricin pharmacokinetics, Ricin therapeutic use

Abstract

In kinetic assays, an anti-CD5-ricin A chain (ST.I-RTA) immunoconjugate (immunotoxins, IT) specifically inhibited up to 40% the protein synthesis of Jurkat target cells within the first 40 hr. Longer exposures of leukemia cells to ST.I-RTA resulted in a progressively higher number of target cells escaping IT treatment and becoming resistant to further treatment with ST.I-RTA even in the presence of the RTA-IT enhancer monensin. Resistant Jurkat cells proliferated at the same rate as control untreated cells, and were as sensitive as control cells to a transferrin-RTA IT, indicating that the ST.I-RTA-resistant tumor-cell population did not become insensitive to the enzymatic activity of RTA. Binding studies revealed that the anti-CD5 IT treatment induced a transient modulation of CD5 antigens but not of the functionally related CD3 antigens. The CD5 antigens were re-expressed at the cell surface following removal of the IT molecules from the culture medium with 1.1% of the total CD5 Ag being re-expressed per hr. When our experimental data on the kinetics of cell intoxication by the IT were corrected for the proliferative potential of the resistant and of the sensitive tumor-cell populations, it appeared that the effect of ST.I-RTA treatment on Jurkat cells was only to delay cell growth for a limited time period (20 hr) without reducing effectively the tumor-cell burden. Our results may have implications for the long-term treatment of target tumor cells with IT.

Published

1995

9. Cytoreductive effects of anti-transferrin receptor immunotoxin in a multicellular tumor spheroid model.

Author

Chignola R, Foroni R, Candiani C, Franceschi A, Pasti M, Stevanoni G, Anselmi C, Tridente G, and Colombatti M

Subjects

Animals, Breast Neoplasms pathology, Glioblastoma pathology, Humans, Mice, Mice, Inbred BALB C, Receptors, Transferrin analysis, Immunotoxins pharmacology, Receptors, Transferrin immunology, Ricin pharmacology, Tumor Cells, Cultured drug effects

Abstract

We have evaluated the sensitivity to immunotoxins (IT) of monolayer and of 200-250 microns multicellular tumor spheroid (MTS) cultures obtained with human breast (MCF7) and glioblastoma (U118) tumor cells and with rat glioblastoma (9L) cells. Monolayer MCF7 and U118 cells were highly sensitive to antitransferrin receptor (anti-TfnR) ricin A chain (RTA)-IT (Tfn-RTA and MAb OKT9-RTA) treatment in the presence of the intracellular RTA-IT enhancing agent human serum albumin-monensin (HSA-Mo) conjugate. A 790- to 2000-fold higher concentration of anti-TfnR IT was instead required to reduce by 50% the volume of individually treated MCF7 spheroids, as evaluated by applying the Gompertz growth model. Monolayer 9L cells showed 230- to 5700-fold lower sensitivity to Tfn-RTA IT than MCF7 and U118 monolayers, yet 9L spheroid cells were almost as sensitive to anti-TfnR IT as monolayer 9L cultures. Binding studies performed with [125I]-Tfn and FITC-labelled anti-TfnR MAb revealed that 9L monolayers and MTS expressed 4.1-fold and 8.8-fold lower amounts of TfnR than MCF7 monolayers and MTS, respectively. However, Tfn bound to TfnR sites of 9L and of MCF7 cells with comparable affinity. Experiments carried out with the diphtheria toxin mutant CRM107 linked to Tfn confirmed the pattern observed with RTA-IT. Monolayers and spheroids showed no considerable differences in sensitivity to ricin toxin. Collectively, these results indicated that the efficacy of IT against 3-D tumors is heavily influenced by the number of target Ag expressed by the tumor cells, as well as by the affinity of IT/toxin-cell interaction.

Published

1994

10. Distribution of endocytosed molecules to intracellular acidic environments correlates with immunotoxin activity.

Author

Chignola R, Colombatti M, Dell'Arciprete L, Candiani C, and Tridente G

Subjects

Animals, Antibodies, Monoclonal pharmacokinetics, Cell Line, Flow Cytometry, Fluorescein-5-isothiocyanate, Fluoresceins, Humans, Hydrogen-Ion Concentration, Mice, Rats, Thiocyanates, Diphtheria Toxin pharmacokinetics, Endocytosis physiology, Immunotoxins pharmacokinetics, Intracellular Fluid metabolism, Transferrin pharmacokinetics

Abstract

We have investigated the internalization to low pH intracellular compartments of transferrin (Tfn), diphtheria toxin (DT) and of anti-cell surface antibodies (MAb) by a cytofluorometric assay based on low pH quenching of fluorescein (FITC) emission. FITC-labelled Tfn, anti-CD3, anti-CD5 and anti-Thy 1.2 MAb internalization resulted in a progressively lower FITC quenching effect. Following internalization, a distinction could be made between molecules that enter low pH compartments without undergoing intracellular degradation (e.g., Tfn, anti-CD3 MAb) and molecules that are internalized through low pH organelles and are then degraded within the cell (e.g., DT). A strict correlation was observed between quenching of internalized FITC-protein fluorescent emission and the cytotoxic activity of DT-based immunotoxins (IT).

Published

1990

11. Sensitivity of human glioma cells to cytotoxic heteroconjugates.

Author

Colombatti M, Bisconti M, Dell'Arciprete L, Gerosa MA, and Tridente G

Subjects

Animals, Antigens, Neoplasm immunology, Carmustine pharmacology, Cell Survival drug effects, Glioma immunology, HLA-DR Antigens immunology, Humans, Interferon-gamma pharmacology, Kinetics, Mice, Mice, Inbred BALB C, Protein Biosynthesis, Receptors, Transferrin immunology, Ricin pharmacology, Tumor Cells, Cultured drug effects, Glioma pathology, Immunotoxins pharmacology

Abstract

Several anti-human glioma cytotoxic conjugates were studied in vitro. Monoclonal antibodies (MAbs) to the GE2 glioma-associated antigen (anti-GE 2) and MAbs to HLA-DR antigens (D1/12) or human diferric transferrin (Tfn) were linked to the potent cytotoxin ricin (anti-GE 2-ricin) or to its A subunit (anti-GE 2-RTA, D1/12-RTA, Tfn-RTA). Anti-GE 2-RTA had low cytotoxic activity in both the absence and the presence of lysosomotropic substances inhibiting intracellular degradation. Anti-GE 2-ricin was about 1,000 times more toxic than RTA alone, but showed only 14-fold target specificity. D1/12-RTA was about 20 times more toxic than RTA and its cytotoxic effect increased about 6- to 7-fold when cell-surface HLA-DR antigen expression was enhanced by IFN-gamma treatment. Human diferric Tfn linked to RTA demonstrated the highest cytotoxic activity, being about 5,000 times more toxic than RTA alone for glioma cells and about 6,000 times more toxic for Jurkat cells in the presence of the carboxylic ionofore monensin. Ricin toxin was only about 5 times more toxic for Jurkat and glioma cells than Tfn-RTA-monensin. Tfn-RTA was over 100,000 times more potent than the chemotherapeutic agent BCNU in reducing glioma cell survival in vitro. Addition of 80% human pooled cerebrospinal fluid (CSF) reduced Tfn-RTA toxicity about 10-fold. Kinetics of Tfn-RTA cytotoxicity at non-saturating concentrations indicated that over 80% of target cells could be killed within 8-10 hr in the absence and within 10-12 hr in the presence of human pooled CSF.

Published

1988