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8 results on '"Manuela Battaglia"'

1. Preculture of PBMCs at high cell density increases sensitivity of T-cell responses, revealing cytokine release by CD28 superagonist TGN1412

Author

Ineke J. M. ten Berge, Susanne Berr, Paula S. Römer, Hermann Einsele, Elita Avota, Thomas Hünig, Manuela Battaglia, Shin Young Na, AII - Amsterdam institute for Infection and Immunity, and Nephrology

Subjects
T-Lymphocytes, medicine.medical_treatment, T cell, Immunology, Receptors, Antigen, T-Cell, Cell Count, Biology, Antibodies, Monoclonal, Humanized, Biochemistry, Proinflammatory cytokine, Interferon-gamma, CD28 Antigens, Antigen, medicine, Humans, Cells, Cultured, Cell Proliferation, Microscopy, Confocal, Tumor Necrosis Factor-alpha, T-cell receptor, CD28, hemic and immune systems, Cell Biology, Hematology, Flow Cytometry, TGN1412, medicine.disease, Cytokine release syndrome, Cytokine, medicine.anatomical_structure, Leukocytes, Mononuclear, Cytokines, Interleukin-2, Lymph Nodes, Muromonab-CD3
Abstract

Human volunteers receiving TGN1412, a humanized CD28-specific monoclonal antibody, experienced a life-threatening cytokine release syndrome during a recent trial. Preclinical tests using human PBMCs had failed to announce the rapid release of TNF, IFN-γ, and other toxic cytokines in response to this CD28 “superagonist” (CD28SA). CD28SA activate T-lymphocytes by ligating CD28 without overt engagement of the TCR. They do, however, depend on “tonic” TCR signals, which they amplify. Here we show that short-term preculture of PBMCs at high, but not at low, cell density results in massive cytokine release during subsequent stimulation with soluble TGN1412. Restoration of reactivity was cell-contact dependent, involved functional maturation of both monocytes and T cells, was sensitive to blockade by HLA-specific mAb, and was associated with TCR polarization and tyrosine phosphorylation. CD4 effector memory T cells were identified as the main source of proinflammatory cytokines. Importantly, responses to other T-cell activating agents, including microbial antigens, were also enhanced if PBMCs were first allowed to interact under tissue-like conditions. We provide a protocol, which strongly improves reactivity of circulating T cells to soluble stimulants, thereby allowing for more reliable preclinical testing of both activating and inhibitory immunomodulatory drugs.

Published
2011

2. The immune response to lentiviral-delivered transgene is modulated in vivo by transgene-expressing antigen-presenting cells but not by CD4+CD25+ regulatory T cells

Author

Lucia Sergi-Sergi, Manuela Battaglia, Maria Grazia Roncarolo, Angelo Lombardo, Andrea Annoni, Luigi Naldini, Antonia Follenzi, Annoni, A, Battaglia, MARCO MARIA, Follenzi, A, Lombardo, A, SERGI SERGI, L, Naldini, Luigi, and Roncarolo, M. G.

Subjects
CD4-Positive T-Lymphocytes, Adoptive cell transfer, Transgene, Genetic Vectors, Green Fluorescent Proteins, Immunology, Antigen-Presenting Cells, Cytomegalovirus, Enzyme-Linked Immunosorbent Assay, Mice, Transgenic, Mice, SCID, Biology, T-Lymphocytes, Regulatory, Biochemistry, Viral vector, Interferon-gamma, Mice, Immune system, Transduction, Genetic, Animals, Humans, Transgenes, IL-2 receptor, Antigen-presenting cell, Lentivirus, Interleukin-2 Receptor alpha Subunit, Cell Biology, Hematology, T lymphocyte, Adoptive Transfer, Cell biology, Mice, Inbred C57BL, Spleen, CD8
Abstract

Systemic delivery of lentiviral vector (LV) in immunocompetent mice leads to efficient in vivo cell transduction and expression of the encoded protein under the control of the ubiquitous promoter of human cytomegalovirus (CMV). However, antitransgene immune response results in clearance of transduced cells 4 weeks after injection. T regulatory cells (Tregs), which have been demonstrated to control immune responses in vivo, were tested for their ability to suppress antitransgene response leading to stable long-term expression. Adoptive transfer of natural CD4+CD25+ Tregs (nTregs) isolated from wild type (wt) mice or from transgene tolerant transgenic (tg) mice did not suppress the antitransgene immune response after LV delivery. These data demonstrate that neither increasing the endogenous pool of natural Tregs nor transferring nTregs selected in a transgene-expressing thymus can modulate the immune response and mediate sustained transgene expression. Conversely, adoptive transfer of antigen-presenting cells (APCs) isolated from transgene-tolerant tg mice efficiently reduced the immune response leading to stable LV-encoded protein expression in vivo. Reduction of CD8+ effector T cells was observed in LV-treated mice coinjected with transgene-expressing APCs compared with control mice. These data indicate that antitransgene immune response can be modulated by transgene-expressing APCs possibly through deletion of effector T cells.

Published
2007

3. Coexistence of Two Functioning T-Cell Repertoires in Healthy Ex-Thalassemics Bearing a Persistent Mixed Chimerism Years After Bone Marrow Transplantation

Author

Arcangelo Nocera, P Tonucci, Gioacchino Robustelli della Cuna, Manuela Battaglia, Nesci S, Raffaele De Palma, M Manna, Guido Lucarelli, Barbara Persini, Marco Andreani, Jack Gorski, Battaglia, M, Andreani, M, Manna, M, Nesci, S, Tonucci, P, Persini, B, ROBUSTELLI DELLA CUNA, G, Nocera, A, Gorski, J, Lucarelli, G, and DE PALMA, Raffaele

Subjects
Adult, Male, Adolescent, T-Lymphocytes, T cell, Immunology, Receptors, Antigen, T-Cell, Human leukocyte antigen, Biology, Biochemistry, Cohort Studies, Immune system, Antigen, medicine, Humans, Phytohemagglutinins, Child, In Situ Hybridization, Fluorescence, Bone Marrow Transplantation, Transplantation Chimera, Cell Biology, Hematology, Donor Lymphocytes, Haematopoiesis, medicine.anatomical_structure, Child, Preschool, Leukocytes, Mononuclear, Thalassemia, Female, Bone marrow, Immunocompetence, Follow-Up Studies
Abstract

Bone marrow transplantation (BMT) from an HLA-identical donor is an established therapy to cure homozygous β-thalassemia. Approximately 10% of thalassemic patients developed a persistent mixed chimerism (PMC) after BMT characterized by stable coexistence of host and donor cells in all hematopoietic compartments. Interestingly, in the erythrocytic lineage, close to normal levels of hemoglobin can be observed in the absence of complete donor engraftment. In the lymphocytic lineage, the striking feature is the coexistence of immune cells. This implies a state of tolerance or anergy, raising the issue of immunocompetence of the host. To understand the state of the T cells in PMC, repertoire analysis and functional studies were performed on cells from 3 ex-thalassemics. Repertoire analysis showed a profound skewing. This was due to an expansion of some T cells and not to a collapse of the repertoire, because phytohemagglutinin stimulation showed the presence of a complex repertoire. The immunocompetence of the chimeric immune systems was further established by showing responses to alloantigens and recall antigens in vitro. Both host and donor lymphocytes were observed in the cultures. These data suggest that the expanded T cells play a role in specific tolerance while allowing a normal immune status in these patients.

Published
1999

4. Differentiation of type 1 T regulatory cells (Tr1) by tolerogenic DC-10 requires the IL-10-dependent ILT4/HLA-G pathway

Author

Ehud Hauben, Valentina Pacciani, Silvia Gregori, Daniela Tomasoni, Maria Grazia Roncarolo, Manuela Battaglia, Miriam Scirpoli, Chiara F. Magnani, Gregori, S, Tomasoni, D, Pacciani, V, Scirpoli, M, Battaglia, MARCO MARIA, Magnani, Cf, Hauben, E, Roncarolo, MARIA GRAZIA, Battaglia, M, Magnani, C, and Roncarolo, M

Subjects
Cellular differentiation, Immunology, Gene Expression, Cell Communication, Dendritic Cell, Monocyte, Biochemistry, T-Lymphocytes, Regulatory, Monocytes, Immune tolerance, Immunophenotyping, HLA-G Antigen, Antigen, HLA Antigens, Immune Tolerance, Humans, HLA Antigen, Receptors, Immunologic, CD86, HLA-G Antigens, CD40, Membrane Glycoproteins, biology, Histocompatibility Antigens Class I, Cell Differentiation, Hematology, Cell Biology, Dendritic Cells, Flow Cytometry, Interleukin-12, Cell biology, Interleukin-10, Interleukin 10, biology.protein, Interleukin 12, Membrane Glycoprotein, CD80, Human, Signal Transduction
Abstract

Type 1 T regulatory (Tr1) cells suppress immune responses in vivo and in vitro and play a key role in maintaining tolerance to self- and non–self-antigens. Interleukin-10 (IL-10) is the crucial driving factor for Tr1 cell differentiation, but the molecular mechanisms underlying this induction remain unknown. We identified and characterized a subset of IL-10–producing human dendritic cells (DCs), termed DC-10, which are present in vivo and can be induced in vitro in the presence of IL-10. DC-10 are CD14+, CD16+, CD11c+, CD11b+, HLA-DR+, CD83+, CD1a−, CD1c−, express the Ig-like transcripts (ILTs) ILT2, ILT3, ILT4, and HLA-G antigen, display high levels of CD40 and CD86, and up-regulate CD80 after differentiation in vitro. DC-10 isolated from peripheral blood or generated in vitro are potent inducers of antigen-specific IL-10–producing Tr1 cells. Induction of Tr1 cells by DC-10 is IL-10–dependent and requires the ILT4/HLA-G signaling pathway. Our data indicate that DC-10 represents a novel subset of tolerogenic DCs, which secrete high levels of IL-10, express ILT4 and HLA-G, and have the specific function to induce Tr1 cells.

Published
2010

5. Rapamycin selectively expands CD4+CD25+FoxP3+ regulatory T cells

Author

Angela Stabilini, Maria Grazia Roncarolo, Manuela Battaglia, Battaglia, MARCO MARIA, Stabilini, A, and Roncarolo, MARIA GRAZIA

Subjects
CD4-Positive T-Lymphocytes, Graft Rejection, T-Lymphocytes, Immunology, Cell Culture Techniques, Islets of Langerhans Transplantation, Cell Separation, Biology, Biochemistry, Polymerase Chain Reaction, Immune tolerance, Cell therapy, Mice, In vivo, Immune Tolerance, Animals, Humans, IL-2 receptor, Cells, Cultured, Cell Proliferation, Sirolimus, Mice, Inbred BALB C, Cell Death, Graft Survival, Peripheral tolerance, FOXP3, Forkhead Transcription Factors, Receptors, Interleukin-2, Cell Biology, Hematology, Flow Cytometry, In vitro, Coculture Techniques, Cell biology, DNA-Binding Proteins, Mice, Inbred C57BL, Female, Ex vivo, Immunosuppressive Agents
Abstract

Rapamycin is an immunosuppressive compound that is currently used to prevent acute graft rejection in humans. In addition, rapamycin has been shown to allow operational tolerance in murine models. However, a direct effect of rapamycin on T regulatory (Tr) cells, which play a key role in induction and maintenance of peripheral tolerance, has not been demonstrated so far. Here, we provide new evidence that rapamycin selectively expands the murine naturally occurring CD4+CD25+FoxP3+ Tr cells in vitro. These expanded Tr cells suppress proliferation of syngeneic T cells in vitro and prevent allograft rejection in vivo. Interestingly, rapamycin does not block activation-induced cell death and proliferation of CD4+ T cells in vitro. Based on this new mode of action, rapamycin can be used to expand CD4+CD25+FoxP3+ Tr cells for ex vivo cellular therapy in T-cell-mediated diseases. (Blood. 2005;105:4743-4748)

Published
2005

6. T-Cell-Mediated Suppression: From Bench to Bedside

Author

Rosa Bacchetta, Megan K. Levings, Maria Grazia Roncarolo, Silvia Gregori, and Manuela Battaglia

Subjects
Adoptive cell transfer, T cell, Immunology, Hematopoietic stem cell, FOXP3, hemic and immune systems, chemical and pharmacologic phenomena, Cell Biology, Hematology, Biology, Biochemistry, CD49b, Granzyme B, Cell therapy, medicine.anatomical_structure, medicine, Cancer research, IL-2 receptor
Abstract

T regulatory cells (Tregs) play a pivotal role in promoting and maintaining tolerance. Several subsets of Tregs have been identified but, to date, the best characterized are the CD4+FOXP3+ Tregs (FOXP3+Tregs), thymic-derived or induced in the periphery, and the CD4+ IL-10-producing T regulatory type 1 (Tr1) cells. In the past decade much effort has been dedicated to develop methods for the in vitro induction and expansion of FOXP3+Tregs and of Tr1 cells for Treg-based cell therapy to promote and restore tolerance in T-cell mediated diseases, and for expanding antigen (Ag)-specific Tregs in vivo. FOXP3+Tregs constitutively express high levels of CD25 and of the transcription factor FOXP3. FOXP3+Tregs are distinguished from activated CD4+ T cells by the low expression of CD127, and by the DNA demethylation of a specific region of the FOXP3 gene called Treg-specific demethylated region (TSDR). FOXP3+Tregs suppress effector T-cell responses through cell-to-cell contact-dependent mechanisms and suppression requires activation via TCR and is IL-2 dependent. In vitro protocols to expand FOXP3+Tregs for adoptive transfer in vivo have been established. We demonstrated that rapamycin permits the in vitro expansion of FOXP3+Tregs while impairing the proliferation of non-Tregs. Moreover, rapamycin-expanded FOXP3+Tregs maintain their regulatory phenotype in a proinflammatory environment and Th17 cells do not expand in the presence of rapamycin. Despite the progress in FOXP3+Tregs expansion protocols, adoptive transfer of FOXP3+Tregs in humans remains a difficult experimental procedure due to the ability to expand a sufficient number of Ag-specific FOXP3+Tregs in vitro. To propagate a homogenous population of FOXP3+Tregs we developed a lentiviral vector (LV)-based strategy to ectopically express FOXP3 in CD4+ T cells. This method results in the development of suppressive cells that are super-imposable to FOXP3+Tregs. Conversion of effector T cells into FOXP3+Tregs upon LV-mediated gene transfer of wild-type FOXP3 was also obtained in CD4+T cells from immunodysregulation polyendocrinopathy enteropathy X-linked (IPEX) patients. We also developed a LV platform, which selectively targets expression of the transgene in hepatocytes, to induce tolerance to self or exogenous Ags. Using this approach we showed that systemic administration of LV encoding for the gene of interest leads to the induction of Ag-specific FOXP3+ Tregs, which mediate tolerance even in pre-immunized hosts. Tr1 cells are identified by their cytokine profile (IL-10+TGF-b+IL-4-IL-17-). Tr1 cells express transiently FOXP3 upon activation; but FOXP3 expression never reaches the high levels characteristic of FOXP3+Tregs. Tr1 cell differentiation and function is independent of FOXP3 since suppressive Tr1 cells can be isolated or generated from peripheral blood of IPEX patients. Tr1 cells were first discovered in peripheral blood of patients who developed tolerance after HLA-mismatched fetal liver hematopoietic stem cell transplant (HSCT). Since their discovery, Tr1 cells have proven to be important in mediating tolerance in several immune-mediated diseases. The immuno-regulatory mechanisms of Tr1 cells have been studied over the years thanks to the possibility to generate these cells in vitro. Tr1 cells suppress T-cell responses via the secretion of IL-10 and TGF-β and by the specific killing of myeloid APC via Granzyme B and perforin. Tr1 cells can be induced in vitro in an Ag-specific manner in the presence of IL-10 or of DC-10. Proof-of-principle clinical trials in allogeneic HSCT demonstrated the safety of Treg-based cell therapy with these polarized Tr1 cells. We are currently planning a phase I/II trial using in vitro polarized Tr1 cells with DC-10 in patients after kidney transplantation. An alternative strategy for the induction of high numbers of human Tr1 cells is the LV-mediated gene transfer of human IL-10 into conventional CD4+ T cells. Stable ectopic expression of IL-10 leads to the differentiation of homogeneous populations of Tr1-like cells displaying potent suppressive functions both in vitro and in vivo. A major hurdle, which limited the studies and the clinical use of Tr1 cells, was the lack of specific biomarkers. By gene expression profiling of human Tr1 cell clones we identified two surface markers (CD49b and LAG-3), which are stably and selectively co-expressed on murine and human Tr1 cells induced in vitro or in vivo. The co-expression of CD49b and LAG-3 enables the isolation of highly suppressive Tr1 cells from in vitro IL-10-polarized Tr1 cells and allows tracking of Tr1 cells in peripheral blood of patients who developed tolerance after allogeneic HSCT. The identification of CD49b and LAG-3 as Tr1-specific biomarkers will facilitate the study of Tr1 cells in vivo in healthy and pathological conditions and the use of Tr1 cells for forthcoming therapeutic interventions. In conclusion, Tregs play a key role in maintaining immunological homeostasis in the periphery. Several open questions regarding FOXP3+ Tregs or Tr1 cell-based therapy in humans remain: how long do Tregs survive after transfer? Is their phenotype stable in pathological conditions and inflammatory environments? Is their mechanism of suppression in vivo Ag-specific? Carefully designed and standardized future clinical protocols reflecting a concerted action among different investigators will help to address these questions and to advance the field. Disclosures: No relevant conflicts of interest to declare.

Published
2013

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