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5. Imaging increased metabolism in the spinal cord in mice after middle cerebral artery occlusion

Author

Ruiqing Ni, Nadja Straumann, Serana Fazio, Xose Luis Dean-Ben, Georgios Louloudis, Claudia Keller, Daniel Razansky, Simon Ametamey, Linjing Mu, César Nombela-Arrieta, and Jan Klohs

Subjects
fluorodeoxyglucose (FDG), Ischemic stroke, Metabolism, MSOT, Optoacoustic tomography, Oxygenation, Physics, QC1-999, Acoustics. Sound, QC221-246, Optics. Light, QC350-467
Abstract

Emerging evidence indicates crosstalk between the brain and hematopoietic system following cerebral ischemia. Here, we investigated metabolism and oxygenation in the spleen and spinal cord in a transient middle cerebral artery occlusion (tMCAO) model. Sham-operated and tMCAO mice underwent [18F]fluorodeoxyglucose (FDG)-positron emission tomography (PET) to assess glucose metabolism. Naïve, sham-operated and tMCAO mice underwent multispectral optoacoustic tomography (MSOT) assisted by quantitative model-based reconstruction and unmixing algorithms for accurate mapping of oxygenation patterns in peripheral tissues at 24 h after reperfusion. We found increased [18F]FDG uptake and reduced MSOT oxygen saturation, indicating hypoxia in the thoracic spinal cord of tMCAO mice compared with sham-operated mice but not in the spleen. Reduced spleen size was observed in tMCAO mice compared with sham-operated mice ex vivo. tMCAO led to an increase in the numbers of mature T cells in femoral bone marrow tissues, concomitant with a stark reduction in these cell subsets in the spleen and peripheral blood. The combination of quantitative PET and MSOT thus enabled observation of hypoxia and increased metabolic activity in the spinal cord of tMCAO mice at 24 h after occlusion compared to sham-operated mice.

Published
2023
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8. Opposite effects of interferon-beta on new B and T cell release from production sites in multiple sclerosis patients

Author

Zanotti, C, Chiarini, M, Serana, F, Capra, R, Rottoli, M, Rovaris, M, Cavaletti, G, Clerici, R, Rezzonico, M, Caimi, L, Imberti, L, Imberti, L., CAVALETTI, GUIDO ANGELO, Zanotti, C, Chiarini, M, Serana, F, Capra, R, Rottoli, M, Rovaris, M, Cavaletti, G, Clerici, R, Rezzonico, M, Caimi, L, Imberti, L, Imberti, L., and CAVALETTI, GUIDO ANGELO

Abstract

The release of newly produced B and T lymphocytes from the production sites was analyzed in 30 multiple sclerosis patients treated with interferon-beta by measuring T-cell receptor excision circles and k-deleting recombination excision circles. We found that the therapy induces opposite effects on B- and T-cell mobilization in 33% of patients. New B-cell production, which peaks after 6months of therapy and then decreases to levels that, however, are still higher than in controls, may cause a renewal of the B-cell compartment. On the contrary, the decreased number of newly produced T lymphocytes observed at 12months of treatment and the association between reduced thymic output and low peripheral T lymphocytes can be a cause of leukopenia, a frequent side effect of the therapy.

Published
2012

9. Modulation of the central memory and Tr1-like regulatory T cells in multiple sclerosis patients responsive to interferon-beta therapy

Author

Chiarini, M, Serana, F, Zanotti, C, Capra, R, Rasia, S, Rottoli, M, Rovaris, M, Caputo, D, Cavaletti, G, Frigo, M, Frigeni, B, Clerici, R, Rezzonico, M, Caimi, L, Imberti, L, Imberti, L., CAVALETTI, GUIDO ANGELO, Chiarini, M, Serana, F, Zanotti, C, Capra, R, Rasia, S, Rottoli, M, Rovaris, M, Caputo, D, Cavaletti, G, Frigo, M, Frigeni, B, Clerici, R, Rezzonico, M, Caimi, L, Imberti, L, Imberti, L., and CAVALETTI, GUIDO ANGELO

Abstract

Background: Interferon-beta is used to reduce disease activity in multiple sclerosis, but its action is incompletely understood, individual treatment response varies among patients, and biological markers predicting clinical benefits have yet to be identified. Since it is known that multiple sclerosis patients have a deficit of the regulatory T-cell subsets, we investigated whether interferon-beta therapy induced modifications of the two main categories of regulatory T cells (Tregs), natural and IL-10-secreting inducible Tr1 subset, in patients who are biologically responsive to the therapy. Methods: T-cell phenotype was determined by flow cytometry, while real-time PCR was used to evaluate interferon-beta bioactivity through MxA determination, and to measure the RNA for IL-10 and CD46 molecule in peripheral blood mononuclear cells stimulated with anti-CD46 and anti-CD3 monoclonal antibodies, which are known to expand a Tr1-like population. Results: Interferon-beta induced a redistribution of natural Treg subsets with a shift of naive Tregs towards the 'central memory-like' Treg population that expresses the CCR7 molecule required for the in vivo suppressive activity. Furthermore, in a subgroup of treated patients, the CD46/CD3 co-stimulation, probably through the Tr1-like subset modulation, increased the production of RNA for IL-10 and CD46. The same group showed a lower median EDSS score after two years of therapy. Conclusions: The selective increase of 'central memory-like' subset and the involvement of the Tr1-like population may be two of the mechanisms by which interferon-beta achieves its beneficial effects. The quantification of RNA for IL-10 and CD46 could be used to identify patients with a different response to interferon-beta therapy.

Published
2011

12. Modulation of the central memory and Tr1-like regulatory T cells in multiple sclerosis patients responsive to interferon-beta therapy

Author

Chiarini, M, primary, Serana, F, additional, Zanotti, C, additional, Capra, R, additional, Rasia, S, additional, Rottoli, M, additional, Rovaris, M, additional, Caputo, D, additional, Cavaletti, G, additional, Frigo, M, additional, Frigeni, B, additional, Clerici, R, additional, Rezzonico, M, additional, Caimi, L, additional, and Imberti, L, additional

Published
2011
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16. Newly produced T and B lymphocytes and T-cell receptor repertoire diversity are reduced in peripheral blood of fingolimod-treated multiple sclerosis patients.

Author

Chiarini, M, Sottini, A, Bertoli, D, Serana, F, Caimi, L, Rasia, S, Capra, R, and Imberti, L

Subjects
DRUG side effects, B cells, T cells, T-cell receptor genes, BLOOD testing, MULTIPLE sclerosis treatment, POLYMERASE chain reaction, PHENOTYPES
Abstract

The article presents a study which examines the reduction of newly produced T and B lymphocytes and T-cell receptor repertoire (TCR) diversity in the peripheral blood of multiple sclerosis (MS) patients treated with fingolimod. The study is investigated by real-time polymerase chain reaction (PCR), immune phenotyping, and spectratyping. Results show that newly produced T and B lymphocytes were reduced while T-cell repertoire increased after 12 months of treatment.

Published
2015
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17. Modulation of the central memory and Tr1-like regulatory T cells in multiple sclerosis patients responsive to interferon-beta therapy.

Author

Chiarini, M, Serana, F, Zanotti, C, Capra, R, Rasia, S, Rottoli, M, Rovaris, M, Caputo, D, Cavaletti, G, Frigo, M, Frigeni, B, Clerici, R, Rezzonico, M, Caimi, L, and Imberti, L

Subjects
*MULTIPLE sclerosis, *T cells, *BIOMARKERS, *INTERFERON beta-1a, *MONOCLONAL antibodies, *FLOW cytometry, *PATIENTS
Abstract

Background: Interferon-beta is used to reduce disease activity in multiple sclerosis, but its action is incompletely understood, individual treatment response varies among patients, and biological markers predicting clinical benefits have yet to be identified. Since it is known that multiple sclerosis patients have a deficit of the regulatory T-cell subsets, we investigated whether interferon-beta therapy induced modifications of the two main categories of regulatory T cells (Tregs), natural and IL-10-secreting inducible Tr1 subset, in patients who are biologically responsive to the therapy.Methods: T-cell phenotype was determined by flow cytometry, while real-time PCR was used to evaluate interferon-beta bioactivity through MxA determination, and to measure the RNA for IL-10 and CD46 molecule in peripheral blood mononuclear cells stimulated with anti-CD46 and anti-CD3 monoclonal antibodies, which are known to expand a Tr1-like population.Results: Interferon-beta induced a redistribution of natural Treg subsets with a shift of naive Tregs towards the ‘central memory-like’ Treg population that expresses the CCR7 molecule required for the in vivo suppressive activity. Furthermore, in a subgroup of treated patients, the CD46/CD3 co-stimulation, probably through the Tr1-like subset modulation, increased the production of RNA for IL-10 and CD46. The same group showed a lower median EDSS score after two years of therapy.Conclusions: The selective increase of ‘central memory-like’ subset and the involvement of the Tr1-like population may be two of the mechanisms by which interferon-beta achieves its beneficial effects. The quantification of RNA for IL-10 and CD46 could be used to identify patients with a different response to interferon-beta therapy. [ABSTRACT FROM AUTHOR]

Published
2012
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18. Renewal of the T-cell compartment in multiple sclerosis patients treated with glatiramer acetate.

Author

Chiarini, M., Sottini, A., Ghidini, C., Zanotti, C., Serana, F., Rottoli, M., Zaffaroni, M., Bergamaschi, R., Cordioli, C., Capra, R., and Imberti, L.

Subjects
MULTIPLE sclerosis, T-cell receptor genes, ACETATES, CONTROL groups, FOLLOW-up studies (Medicine), PATIENTS
Abstract

The immunomodulating activity of glatiramer acetate on T-cells of multiple sclerosis patients has only been partially clarified. The objective of this work was to investigate whether glatiramer acetate modifies thymic release of newly produced T-cells and the peripheral composition of the T-cell repertoire. T-cell receptor excision circles, thymicnaive (CD4+CD45RA+CCR7+CD31+) T helper cells, and central (CD4+CD45RA-CCR7+) and effector (CD4+CD45RA-CCR7-) memory T-cells were evaluated in 89 untreated patients, 84 patients treated for at least 1 year, and 31 patients beginning treatment at the time of inclusion in the study and then followed-up for 12 months; controls were 81 healthy donors. The T-cell repertoire was analysed in selected samples. The percentage of thymicnaive T helper cells was diminished in untreated patients, but rose to control values in treated subjects; a decrease in central memory T-cells was also observed in treated patients. Follow-up patients could be divided into two subgroups, one showing unmodified thymicnaive T helper cells and T-cell diversity, the other in which the increased release of new T-cells was accompanied by modifications of the T-cell repertoire. Glatiramer acetate modifies the peripheral T-cell pool by activating a thymopoietic pathway of T-cell release that leads to a different setting of T-cell diversity and, likely, to a dilution of autoreactive T-cells. [ABSTRACT FROM AUTHOR]

Published
2010
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20. Effects of combined antiretroviral therapy on B- and T-cell release from production sites in long-term treated HIV-1+ patients

Author

Quiros-Roldan Eugenia, Serana Federico, Chiarini Marco, Zanotti Cinzia, Sottini Alessandra, Gotti Daria, Torti Carlo, Caimi Luigi, and Imberti Luisa

Subjects
KRECs, TRECs, HIV-1, cART, T lymphocytes, B lymphocytes, Medicine
Abstract

Abstract Background The immune system reconstitution in HIV-1- infected patients undergoing combined antiretroviral therapy is routinely evaluated by T-cell phenotyping, even though the infection also impairs the B-cell mediated immunity. To find new laboratory markers of therapy effectiveness, both B- and T- immune recovery were evaluated by means of a follow-up study of long-term treated HIV-1- infected patients, with a special focus on the measure of new B- and T-lymphocyte production. Methods A longitudinal analysis was performed in samples obtained from HIV-1-infected patients before therapy beginning and after 6, 12, and 72 months with a duplex real-time PCR allowing the detection of K-deleting recombination excision circles (KRECs) and T-cell receptor excision circles (TRECs), as measures of bone-marrow and thymic output, respectively. A cross sectional analysis was performed to detect B- and T-cell subsets by flow cytometry in samples obtained at the end of the follow-up, which were compared to those of untreated HIV-1-infected patients and uninfected controls. Results The kinetics and the timings of B- and T-cell release from the bone marrow and thymus during antiretroviral therapy were substantially different, with a decreased B-cell release and an increased thymic output after the prolonged therapy. The multivariable regression analysis showed that a longer pre-therapy infection duration predicts a minor TREC increase and a major KREC reduction. Conclusions The quantification of KRECs and TRECs represents an improved method to monitor the effects of therapies capable of influencing the immune cell pool composition in HIV-1-infected patients.

Published
2012
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21. Identification of a public CDR3 motif and a biased utilization of T-cell receptor V beta and J beta chains in HLA-A2/Melan-A-specific T-cell clonotypes of melanoma patients

Author

Natali Pier, Palermo Belinda, Caimi Luigi, Sottini Alessandra, Serana Federico, Nisticò Paola, and Imberti Luisa

Subjects
Medicine
Abstract

Abstract Background Assessment of T-cell diversity, besides giving insights about the molecular basis of tumor antigen recognition, has clinical implications since it provides criteria for evaluating antigen-specific T cells clinically relevant for spontaneous and vaccine-induced anti-tumor activity. Melan-A is one of the melanoma antigens most frequently recognized by peripheral and tumor-infiltrating lymphocytes in HLA-A2+ melanoma patients. Many clinical trials involving anti-tumor vaccination have been conducted using modified versions of this peptide. Methods We conducted an in-depth characterization of 210 T-cell receptor beta chain (TRB) clonotypes derived from T cells of HLA-A2+ melanoma patients displaying cytotoxic activity against natural and A27L-modified Melan-A peptides. One hundred and thirteen Melan-A-specific clonotypes from melanoma-free subjects, 199 clonotypes from T-cell clones from melanoma patients specific for melanoma antigens other than Melan-A, and 305 clonotypes derived from T cells of HLA-A2+ individuals showing unrelated specificities, were used as control. After sequence analysis, performed according to the IMGT definitions, TRBV and TRBJ usage, CDR3 length and amino acid composition were compared in the four groups of clonotypes. Results TRB sequences of Melan-A-specific clonotypes obtained from melanoma patients were highly heterogeneous, but displayed a preferential usage of few TRBV and TRBJ segments. Furthermore, they included a recurrent "public" amino acid motif (Glycine-Leucine-Glycine at positions 110-112-113 of the CDR3) rearranged with dominant TRBV and TRBJ segments and, in one case, associated with a full conservation of the entire TRB sequence. Conclusion Contrary to what observed for public anti-Melan-A T-cell receptor alpha motifs, which had been identified in several clonotypes of both melanoma patients and healthy controls, the unexpectedly high contribution of a public TRB motif in the recognition of a dominant melanoma epitope in melanoma patients may provide important information about the biology of anti-tumor T-cell responses and improve monitoring strategies of anti-tumor vaccines.

Published
2009
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22. Type I interferon-dependent gene MxA in perinatal HIV-infected patients under antiretroviral therapy as marker for therapy failure and blood plasmacytoid dendritic cells depletion

Author

Plebani Alessandro, Lonardi Silvia, Spinelli Elena, Chiarini Marco, Sottini Alessandra, Serana Federico, Facchetti Fabio, Ghidini Claudia, Badolato Raffaele, Caimi Luigi, and Imberti Luisa

Subjects
Medicine
Abstract

Abstract Background To determine the role of interferon-alpha in controlling HIV infection we phenotypically and functionally analyzed circulating plasmacytoid dendritic cells (pDC), which are known to be the highest interferon-alpha producing cells, in 33 perinatally infected HIV+ patients undergoing standard antiretroviral therapy. Methods Circulating pDC were identified by flow cytometry using anti-BDCA-2 monoclonal antibody and by measuring BDCA-2 mRNA by real-time PCR, while tissue-resident pDC were identified by immunohistochemistry. mRNA for interferon-alpha and MxA, a gene that is specifically induced by interferon-alpha, was quantified in peripheral blood cells by real-time PCR, while serum interferon-alpha protein was measured by ELISA. Results While median values of pDC, both in terms of percentage and absolute number, were not statistically different from age-matched controls, interferon-alpha mRNA was increased in HIV-infected patients. However, in a group of patients with long disease duration, having a low number of both pDC and CD4+ lymphocytes and a significant increase of serum interferon-alpha, MxA mRNA was produced at high level and its expression directly correlated with HIV RNA copy numbers. Furthermore in patients displaying a low CD4+ blood cell count, a severe depletion of pDC in the tonsils could be documented. Conclusion HIV replication unresponsive to antiretroviral treatment in perinatal-infected patients with advanced disease and pDC depletion may lead to interferon-alpha expression and subsequent induction of MxA mRNA. Thus, the latter measurement may represent a valuable marker to monitor the clinical response to therapy in HIV patients.

Published
2008
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23. Identification of a public CDR3 motif and a biased utilization of T-cell receptor V beta and J beta chains in HLA-A2/Melan-A-specific T-cell clonotypes of melanoma patients.

Author

Serana F, Sottini A, Caimi L, Palermo B, Natali PG, Nisticò P, Imberti L, Serana, Federico, Sottini, Alessandra, Caimi, Luigi, Palermo, Belinda, Natali, Pier Giorgio, Nisticò, Paola, and Imberti, Luisa

Abstract

Background: Assessment of T-cell diversity, besides giving insights about the molecular basis of tumor antigen recognition, has clinical implications since it provides criteria for evaluating antigen-specific T cells clinically relevant for spontaneous and vaccine-induced anti-tumor activity. Melan-A is one of the melanoma antigens most frequently recognized by peripheral and tumor-infiltrating lymphocytes in HLA-A2+ melanoma patients. Many clinical trials involving anti-tumor vaccination have been conducted using modified versions of this peptide.Methods: We conducted an in-depth characterization of 210 T-cell receptor beta chain (TRB) clonotypes derived from T cells of HLA-A2+ melanoma patients displaying cytotoxic activity against natural and A27L-modified Melan-A peptides. One hundred and thirteen Melan-A-specific clonotypes from melanoma-free subjects, 199 clonotypes from T-cell clones from melanoma patients specific for melanoma antigens other than Melan-A, and 305 clonotypes derived from T cells of HLA-A2+ individuals showing unrelated specificities, were used as control. After sequence analysis, performed according to the IMGT definitions, TRBV and TRBJ usage, CDR3 length and amino acid composition were compared in the four groups of clonotypes.Results: TRB sequences of Melan-A-specific clonotypes obtained from melanoma patients were highly heterogeneous, but displayed a preferential usage of few TRBV and TRBJ segments. Furthermore, they included a recurrent "public" amino acid motif (Glycine-Leucine-Glycine at positions 110-112-113 of the CDR3) rearranged with dominant TRBV and TRBJ segments and, in one case, associated with a full conservation of the entire TRB sequence.Conclusion: Contrary to what observed for public anti-Melan-A T-cell receptor alpha motifs, which had been identified in several clonotypes of both melanoma patients and healthy controls, the unexpectedly high contribution of a public TRB motif in the recognition of a dominant melanoma epitope in melanoma patients may provide important information about the biology of anti-tumor T-cell responses and improve monitoring strategies of anti-tumor vaccines. [ABSTRACT FROM AUTHOR]

Published
2009
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24. Type I interferon-dependent gene MxA in perinatal HIV-infected patients under antiretroviral therapy as marker for therapy failure and blood plasmacytoid dendritic cells depletion.

Author

Badolato R, Ghidini C, Facchetti F, Serana F, Sottini A, Chiarini M, Spinelli E, Lonardi S, Plebani A, Caimi L, Imberti L, Badolato, Raffaele, Ghidini, Claudia, Facchetti, Fabio, Serana, Federico, Sottini, Alessandra, Chiarini, Marco, Spinelli, Elena, Lonardi, Silvia, and Plebani, Alessandro

Abstract

Background: To determine the role of interferon-alpha in controlling HIV infection we phenotypically and functionally analyzed circulating plasmacytoid dendritic cells (pDC), which are known to be the highest interferon-alpha producing cells, in 33 perinatally infected HIV+ patients undergoing standard antiretroviral therapy.Methods: Circulating pDC were identified by flow cytometry using anti-BDCA-2 monoclonal antibody and by measuring BDCA-2 mRNA by real-time PCR, while tissue-resident pDC were identified by immunohistochemistry. mRNA for interferon-alpha and MxA, a gene that is specifically induced by interferon-alpha, was quantified in peripheral blood cells by real-time PCR, while serum interferon-alpha protein was measured by ELISA.Results: While median values of pDC, both in terms of percentage and absolute number, were not statistically different from age-matched controls, interferon-alpha mRNA was increased in HIV-infected patients. However, in a group of patients with long disease duration, having a low number of both pDC and CD4+ lymphocytes and a significant increase of serum interferon-alpha, MxA mRNA was produced at high level and its expression directly correlated with HIV RNA copy numbers. Furthermore in patients displaying a low CD4+ blood cell count, a severe depletion of pDC in the tonsils could be documented.Conclusion: HIV replication unresponsive to antiretroviral treatment in perinatal-infected patients with advanced disease and pDC depletion may lead to interferon-alpha expression and subsequent induction of MxA mRNA. Thus, the latter measurement may represent a valuable marker to monitor the clinical response to therapy in HIV patients. [ABSTRACT FROM AUTHOR]

Published
2008
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25. Opposite effects of interferon-beta on new B and T cell release from production sites in multiple sclerosis patients

Author

Raffaella Clerici, Cinzia Zanotti, Monica Rezzonico, Marco Chiarini, Federico Serana, Marco Rovaris, M Rottoli, Luigi Caimi, Ruggero Capra, Guido Cavaletti, Luisa Imberti, Zanotti, C, Chiarini, M, Serana, F, Capra, R, Rottoli, M, Rovaris, M, Cavaletti, G, Clerici, R, Rezzonico, M, Caimi, L, and Imberti, L

Subjects
Adult, Male, Side effect, multiple sclerosis, lymphocytes, interferon-beta, T cell, Immunology, B-Lymphocyte Subsets, Biology, Young Adult, Multiple Sclerosis, Relapsing-Remitting, T-Lymphocyte Subsets, medicine, Humans, Immunology and Allergy, Receptor, Cell Proliferation, Leukopenia, T-cell receptor excision circles, Multiple sclerosis, Compartment (ship), Cell Differentiation, Interferon-beta, Middle Aged, medicine.disease, Peripheral, medicine.anatomical_structure, Neurology, Female, Neurology (clinical), medicine.symptom, Follow-Up Studies
Abstract

The release of newly produced B and T lymphocytes from the production sites was analyzed in 30 multiple sclerosis patients treated with interferon-beta by measuring T-cell receptor excision circles and k-deleting recombination excision circles. We found that the therapy induces opposite effects on B- and T-cell mobilization in 33% of patients. New B-cell production, which peaks after 6 months of therapy and then decreases to levels that, however, are still higher than in controls, may cause a renewal of the B-cell compartment. On the contrary, the decreased number of newly produced T lymphocytes observed at 12 months of treatment and the association between reduced thymic output and low peripheral T lymphocytes can be a cause of leukopenia, a frequent side effect of the therapy.

Published
2012

26. Modulation of the central memory and Tr1-like regulatory T cells in multiple sclerosis patients responsive to interferon-beta therapy

Author

Luigi Caimi, Monica Rezzonico, Luisa Imberti, Guido Cavaletti, Raffaella Clerici, Domenico Caputo, Ruggero Capra, Cinzia Zanotti, Marco Rovaris, Marco Chiarini, Federico Serana, Barbara Frigeni, Sarah Rasia, M Rottoli, Maura Frigo, Chiarini, M, Serana, F, Zanotti, C, Capra, R, Rasia, S, Rottoli, M, Rovaris, M, Caputo, D, Cavaletti, G, Frigo, M, Frigeni, B, Clerici, R, Rezzonico, M, Caimi, L, and Imberti, L

Subjects
Adult, Receptors, CCR7, CD3 Complex, medicine.drug_class, Biology, Monoclonal antibody, Real-Time Polymerase Chain Reaction, Peripheral blood mononuclear cell, T-Lymphocytes, Regulatory, Flow cytometry, Membrane Cofactor Protein, Young Adult, Multiple Sclerosis, Relapsing-Remitting, medicine, Humans, Immunologic Factors, RNA, Messenger, Cells, Cultured, Analysis of Variance, medicine.diagnostic_test, CD46, Reverse Transcriptase Polymerase Chain Reaction, Multiple sclerosis, Interferon beta-1a, Interferon-beta, Middle Aged, medicine.disease, Flow Cytometry, Phenotype, Interleukin-10, Interleukin 10, Treatment Outcome, Neurology, Italy, t-reg, Case-Control Studies, Immunology, Neurology (clinical), Immunologic Memory, Biomarkers, medicine.drug
Abstract

Background: Interferon-beta is used to reduce disease activity in multiple sclerosis, but its action is incompletely understood, individual treatment response varies among patients, and biological markers predicting clinical benefits have yet to be identified. Since it is known that multiple sclerosis patients have a deficit of the regulatory T-cell subsets, we investigated whether interferon-beta therapy induced modifications of the two main categories of regulatory T cells (Tregs), natural and IL-10-secreting inducible Tr1 subset, in patients who are biologically responsive to the therapy. Methods: T-cell phenotype was determined by flow cytometry, while real-time PCR was used to evaluate interferon-beta bioactivity through MxA determination, and to measure the RNA for IL-10 and CD46 molecule in peripheral blood mononuclear cells stimulated with anti-CD46 and anti-CD3 monoclonal antibodies, which are known to expand a Tr1-like population. Results: Interferon-beta induced a redistribution of natural Treg subsets with a shift of naive Tregs towards the ‘central memory-like’ Treg population that expresses the CCR7 molecule required for the in vivo suppressive activity. Furthermore, in a subgroup of treated patients, the CD46/CD3 co-stimulation, probably through the Tr1-like subset modulation, increased the production of RNA for IL-10 and CD46. The same group showed a lower median EDSS score after two years of therapy. Conclusions: The selective increase of ‘central memory-like’ subset and the involvement of the Tr1-like population may be two of the mechanisms by which interferon-beta achieves its beneficial effects. The quantification of RNA for IL-10 and CD46 could be used to identify patients with a different response to interferon-beta therapy.

Published
2011

27. MxA mRNA Quantification and Disability Progression in Interferon Beta-Treated Multiple Sclerosis Patients

Author

Vittorio Martinelli, Ruggero Capra, Maria Pia Amato, Angelo Ghezzi, Stefano Sotgiu, Luisa Imberti, M. Rottoli, Giancarlo Comi, Claudio Gasperini, Sergio Stecchi, Leandro Provinciali, Mauro Zaffaroni, Cinzia Cordioli, Michele Vecchio, Federico Serana, Serana, F, Imberti, L, Amato, Mp, Comi, Giancarlo, Gasperini, C, Ghezzi, A, Martinelli, V, Provinciali, L, Rottoli, Mr, Sotgiu, S, Stecchi, S, Vecchio, M, Zaffaroni, M, Cordioli, C, and Capra, R.

Subjects
Male, Myxovirus Resistance Proteins, Epidemiology, lcsh:Medicine, Receptor, Interferon alpha-beta, Pathology and Laboratory Medicine, Biochemistry, Disability Evaluation, Medicine and Health Sciences, Protein Isoforms, lcsh:Science, Receptor, Cytopathic effect, Multidisciplinary, biology, Biological activity, Middle Aged, Neurology, Research Design, Genetic Epidemiology, Disease Progression, Female, Antibody, Research Article, Adult, Multiple Sclerosis, Patient Dropouts, Adolescent, Clinical Research Design, Immunology, Research and Analysis Methods, Autoimmune Diseases, MED/39 Neuropsichiatria infantile, Young Adult, Pharmacotherapy, Diagnostic Medicine, medicine, Humans, RNA, Messenger, Beta (finance), Population Biology, Multiple sclerosis, lcsh:R, Biology and Life Sciences, Interferon-beta, medicine.disease, Antibodies, Neutralizing, Demyelinating Disorders, Kinetics, Protein Subunits, Biomarker Epidemiology, biology.protein, lcsh:Q, Clinical Immunology, Protein A, Biomarkers, interferon beta-treated multiple sclerosis
Abstract

Even though anti-interferon beta (IFNβ) antibodies are the main determinants of IFNβ bioactivity loss and Myxovirus-resistance protein A (MxA) is the most established marker of IFNβ biological activity in IFNβ-treated multiple sclerosis patients, their usefulness in the routine clinical practice is still debated. Therefore, 118 multiple sclerosis patients naïve for treatment were enrolled for a 3-year longitudinal observational study mimicking the conditions of a real-world setting. In order to evaluate the kinetics of bioactivity loss in blood samples obtained every 6 months after therapy initiation, MxA and interferon receptor isoform/subunit mRNA were quantified by real-time PCR, anti-IFNβ binding antibodies were detected by radioimmunoprecipitation, and neutralizing antibodies by cytopathic effect inhibition assay. Clinical measures of disease activity and disability progression were also obtained at all time points. We found that, at the individual-patient level, the response to IFNβ therapy was extremely heterogeneous, including patients with stable or transitory, early or late loss of IFNβ bioactivity, and patients with samples lacking MxA mRNA induction in spite of absence of antibodies. No interferon receptor isoform alterations that could explain these findings were found. At the group level, none of these biological features correlated with the measures of clinical disease activity or progression. However, when MxA mRNA was evaluated not at the single time point as a dichotomic marker (induced vs. non-induced), but as the mean of its values measured over the 6-to-24 month period, the increasing average MxA predicted a decreasing risk of short-term disability progression, independently from the presence of relapses. Therefore, a more bioactive treatment, even if unable to suppress relapses, reduces their severity by an amount that is proportional to MxA levels. Together with its feasibility in the routine laboratory setting, these data warrant the quantification of MxA mRNA as a primary tool for a routine monitoring of IFNβ therapy.

Published
2014
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28. Diagnostic accuracy of bone marrow blood evaluation in haemophagocytic lymphohistiocytosis paediatric patients.

Author

Caravaggi E, Serana F, Carini M, Ferrari F, Tregambe D, Micheletti M, Martellosio G, Brugnoni D, Bresciani R, and Biasiotto G

Abstract

Introduction: Haemophagocytic lymphohistiocytosis (HLH) is a rare and serious immunological syndrome that involves a strong activation of cytotoxic T lymphocytes and macrophages. HLH determines a cytokine-mediated tissue injury with a contemporary multi-organ failure and a high fatality rate., Material and Methods: A retrospective study was performed considering the medical records of paediatric patients who underwent a bone marrow aspirate for suspect HLH. The biomarkers evaluated were among those included in the HLH-2004. Lactate dehydrogenase (LD) was also evaluated. Haemophagocytosis was evaluated in bone marrow blood smear slides., Results: Enrolled were 11 patients included in the HLH group and 8 patients as controls. Haemoglobin and fibrinogen resulted lower in HLH patients than in controls, while blood triglycerides, serum ferritin and LD resulted increased. Blood triglycerides and fibrinogen discriminated HLH cases perfectly, with a sensitivity and specificity of 100%. Ferritin had a sensitivity of 100% and a specificity of 83% (cut off ≥3,721 µg/L) and LD of 73% and of 100% (the cut off ≥1,903 U/L). Haemoglobin was found to have a sensitivity of 75% and a specificity of 100% (cut off ≤ 96 g/L). Total haemophagocytes cell counts were not different between patients and controls. Only the increased number of phagocytized nucleated red blood cells (NRBC) was found to be significantly increased in the patients. Erythrocytes phagocytosis (≥4/1,000 cells) only tended towards significance., Conclusions: The blood biomarkers showed better diagnostic performance than the morphological evaluation. Among the different cell lineages engulfed by haemophagocytes, the best diagnostic performance was obtained by phagocytosed mature erythrocytes and immature nucleated erythrocytes., Competing Interests: Declaration of conflicting interestsThe author(s) declared no potential conflicts of interest with respect to the research, authorship, and/or publication of this article.

Published
2024
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29. Clinical and transcriptomic characteristics of a novel SMARCD2 mutation that disrupts neutrophil maturation and function.

Author

Dotta L, Baresi G, Tamassia N, Calzetti F, Bianchetto-Aguilera F, Gasperini S, Gardiman E, Chiarini M, Moratto D, Martellosio G, Serana F, Micheletti M, Tregambe D, Pintabona V, Soncini E, Meini A, Girelli MF, Beghin A, Lanfranchi A, Bugatti M, Brugnoni D, Soresina A, Plebani A, Cassatella M, Vermi W, Porta F, and Badolato R

Abstract

We report a novel case of SMARCD2 (SWI/SNF-related, matrix-associated, actin-dependent regulator of chromatin, subfamily D, member 2) mutation successfully treated with hematopoietic stem cell transplantation. The female patient presented delayed cord separation, chronic diarrhea, skin abscesses, skeletal dysmorphisms, and neutropenia with specific granule deficiency. Analysis of the transcriptomic profile of peripheral blood sorted mature and immature SMARCD2 neutrophils showed defective maturation process that associated with altered expression of genes related to specific, azurophilic, and gelatinase granules, such as LTF, CRISP3, PTX3, and CHI3L1. These abnormalities account for the prevalence of immature neutrophils in the peripheral blood, impaired function, and deregulated inflammatory responses., (© 2023 Wiley Periodicals LLC.)

Published
2023
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30. Longitudinal Characterization of Immune Response in a Cohort of Children Hospitalized with Multisystem Inflammatory Syndrome.

Author

Dotta L, Moratto D, Cattalini M, Brambilla S, Giustini V, Meini A, Girelli MF, Cortesi M, Timpano S, Galvagni A, Viola A, Crotti B, Manerba A, Pierelli G, Verzura G, Serana F, Brugnoni D, Garrafa E, Ricci F, Tomasi C, Chiarini M, and Badolato R

Abstract

Background: Multisystem Inflammatory Syndrome in Children (MIS-C) is a severe complication of SARS-CoV-2 infection caused by hyperactivation of the immune system., Methods: this is a retrospective analysis of clinical data, biochemical parameters, and immune cell subsets in 40 MIS-C patients from hospital admission to outpatient long-term follow-up., Results: MIS-C patients had elevated inflammatory markers, associated with T- and NK-cell lymphopenia, a profound depletion of dendritic cells, and altered monocyte phenotype at disease onset, while the subacute phase of the disease was characterized by a significant increase in T- and B-cell counts and a rapid decline in activated T cells and terminally differentiated B cells. Most of the immunological parameters returned to values close to the normal range during the remission phase (20-60 days after hospital admission). Nevertheless, we observed a significantly reduced ratio between recently generated and more differentiated CD8+ T- and B-cell subsets, which partially settled at longer-term follow-up determinations., Conclusions: The characterization of lymphocyte distribution in different phases of MIS-C may help to understand the course of diseases that are associated with dysregulated immune responses and to calibrate prompt and targeted treatments.

Published
2023
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31. Autoantibodies to Interferons in Infectious Diseases.

Author

Quiros-Roldan E, Sottini A, Signorini SG, Serana F, Tiecco G, and Imberti L

Subjects
Humans, Autoantibodies, Interferons, Cytokines, Autoimmune Diseases, COVID-19, Interferon Type I, Communicable Diseases
Abstract

Anti-cytokine autoantibodies and, in particular, anti-type I interferons are increasingly described in association with immunodeficient, autoimmune, and immune-dysregulated conditions. Their presence in otherwise healthy individuals may result in a phenotype characterized by a predisposition to infections with several agents. For instance, anti-type I interferon autoantibodies are implicated in Coronavirus Disease 19 (COVID-19) pathogenesis and found preferentially in patients with critical disease. However, autoantibodies were also described in the serum of patients with viral, bacterial, and fungal infections not associated with COVID-19. In this review, we provide an overview of anti-cytokine autoantibodies identified to date and their clinical associations; we also discuss whether they can act as enemies or friends, i.e., are capable of acting in a beneficial or harmful way, and if they may be linked to gender or immunosenescence. Understanding the mechanisms underlying the production of autoantibodies could improve the approach to treating some infections, focusing not only on pathogens, but also on the possibility of a low degree of autoimmunity in patients.

Published
2023
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32. Lack of a prompt normalization of immunological parameters is associated with long-term care and poor prognosis in COVID-19 affected patients receiving convalescent plasma: a single center experience.

Author

Moratto D, Mimiola E, Serana F, Garuti M, Giustini V, Roccaro AM, Casari S, Beccaria M, Brugnoni D, Chiarini M, and Franchini M

Subjects
Humans, SARS-CoV-2, Long-Term Care, Immunization, Passive, COVID-19 Serotherapy, COVID-19 therapy
Abstract

Objectives: Being COVID-19 convalescent plasma (CCP) a therapeutic option that can have a potential impact on the normalization of immunological parameters of COVID-19 affected patients, a detailed analysis of post-infusion immunological changes was conducted in CCP treated patients, aiming to identify possible predictive hallmarks of disease prognosis., Methods: This prospective observational study describes a cohort of 28 patients who received CCP shortly after being hospitalized for COVID-19 and diagnosed for Acute Respiratory Distress Syndrome. All patients were subjected to a detailed flow cytometry based evaluation of immunological markers at baseline and on days +3 and +7 after transfusion., Results: At baseline almost all patients suffered from lymphopenia (25/28 on T-cells and 16/28 on B-cells) coupled with neutrophil-lymphocyte ratio exceeding normal values (26/28). Lymphocyte subsets were generally characterized by increased percentages of CD19+CD20-CD38hiCD27+ plasmablasts and reduction of CD4+CD45RA+CCR7+CD31+ recent thymic emigrants, while monocytes presented a limited expression of CD4 and HLA-DR molecules. Amelioration of immunological parameters began to be evident from day +3 and became more significant at day +7 post-CCP transfusion in 18 patients who recovered within 30 days from hospitalization. Conversely, baseline immunological characteristics generally persisted in ten critical patients who eventually progressed to death (6) or long-term care (4)., Conclusions: This study demonstrates that proper immunophenotyping panels can be potentially useful for monitoring CCP treated patients from the first days after infusion in order to presume higher risk of medical complications., (© 2022 Walter de Gruyter GmbH, Berlin/Boston.)

Published
2022
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33. A case of discrepant laboratory results in samples obtained from a central venous catheter and peripheral veins: when solving a pre-analytical mystery could improve patient care.

Author

Carini M, Micheletti M, Martellosio G, Caravaggi E, Portesi N, Biasiotto G, Marini M, Brugnoni D, and Serana F

Subjects
Male, Humans, Middle Aged, Phlebotomy methods, Specimen Handling, Patient Care, Central Venous Catheters
Abstract

It is now generally accepted that laboratory errors or inaccurate results are mainly due to deficiencies in the pre-analytical phase. In this report, we describe the case of a 64-year-old male affected by a relapsing follicular lymphoma, who has been treated with chemotherapy through a central venous catheter (CVC). Four different samples were collected alternatively through peripheral venipuncture and CVC sampling. Unexpectedly, the samples collected from the two different sources showed contrasting results, with the presence of unusual macrophage-like cells in the samples obtained from CVC. It was later found that the CVC was displaced into the pleural space. This case report shows how the sampling process can sometimes influence test results and how it can help clinicians identify clinical conditions that have not yet manifested., Competing Interests: Potential conflict of interest None declared., (Croatian Society of Medical Biochemistry and Laboratory Medicine.)

Published
2022
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34. Long pentraxin 3 as a marker of COVID-19 severity: evidences and perspectives.

Author

Assandri R, Accordino S, Canetta C, Buscarini E, Scartabellati A, Tolassi C, and Serana F

Subjects
Biomarkers, C-Reactive Protein metabolism, Ferritins, Humans, ROC Curve, Retrospective Studies, Serum Amyloid P-Component, COVID-19 diagnosis
Abstract

Introduction: Several laboratory tests are characteristically altered in Coronavirus Disease 2019 (COVID-19), but are not totally accurate in predicting the disease outcome. The long pentraxin 3 (PTX3) is quickly released directly at inflammation sites by many immune cell types. Previous studies have shown that PTX3 correlated with disease severity in various inflammatory conditions. Our study investigated the use of PTX3 as a potential marker of COVID-19 severity and compared its performance in detecting a more severe form of the disease with that of routine laboratory parameters., Materials and Methods: Stored serum samples of RT-PCR confirmed COVID-19 cases that had been obtained at hospital admission were retrospectively analysed. Intensive care unit (ICU) stay was considered a surrogate endpoint of severe COVID-19. Pentraxin 3 was measured by a commercial enzyme-linked immunosorbent assay., Results: A total of 96 patients were recruited from May 1st, 2020 to June 30th, 2020; 75/96 were transferred to ICU. Pentraxin 3 was higher in ICU vs non-ICU patients (35.86 vs 10.61 ng/mL, P < 0.001). Univariate and multivariate logistic regression models demonstrated that the only significant laboratory predictor of ICU stay was PTX3 (OR: 1.68 (1.19-2.29), P = 0.003), after controlling for comorbidities. The Receiver Operator Characteristic curve analysis showed that PTX3 had a higher accuracy compared to C-reactive protein (CRP), lactate dehydrogenase (LD), ferritin in identifying ICU patients (AUC of PTX3 = 0.98; CRP = 0.66; LD = 0.70; ferritin = 0.67, P < 0.001). A cut-off of PTX3 > 18 ng/mL yielded a sensitivity of 96% and a specificity of 100% in identifying patients requiring ICU., Conclusion: High values of PTX3 predict a more severe COVID-19., Competing Interests: Potential conflict of interest None declared., (Croatian Society of Medical Biochemistry and Laboratory Medicine.)

Published
2022
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35. Flow Cytometry Identifies Risk Factors and Dynamic Changes in Patients with COVID-19.

Author

Moratto D, Chiarini M, Giustini V, Serana F, Magro P, Roccaro AM, Imberti L, Castelli F, Notarangelo LD, and Quiros-Roldan E

Subjects
Adult, Aged, Aged, 80 and over, Betacoronavirus pathogenicity, COVID-19, COVID-19 Testing, Cell Separation, Coronavirus Infections blood, Coronavirus Infections diagnosis, Coronavirus Infections immunology, Female, Host Microbial Interactions immunology, Humans, Kaplan-Meier Estimate, Lymphocyte Count, Lymphocyte Subsets metabolism, Male, Middle Aged, Pandemics, Pneumonia, Viral blood, Pneumonia, Viral diagnosis, Pneumonia, Viral immunology, Receptors, Antigen, T-Cell, gamma-delta metabolism, Risk Factors, SARS-CoV-2, Severity of Illness Index, Betacoronavirus immunology, Clinical Laboratory Techniques methods, Coronavirus Infections mortality, Flow Cytometry, Lymphocyte Subsets immunology, Pneumonia, Viral mortality
Published
2020
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36. Simultaneous quantification of natural and inducible regulatory T-cell subsets during interferon-β therapy of multiple sclerosis patients.

Author

Chiarini M, Capra R, Serana F, Bertoli D, Sottini A, Giustini V, Scarpazza C, Rovaris M, Torri Clerici V, Ferraro D, Galgani S, Solaro C, Conti MZ, Visconti A, and Imberti L

Subjects
Humans, Interferon-beta therapeutic use, Longitudinal Studies, Prospective Studies, T-Lymphocyte Subsets, T-Lymphocytes, Regulatory, Multiple Sclerosis drug therapy, Multiple Sclerosis, Relapsing-Remitting
Abstract

Background: The mechanisms underlying the therapeutic activity of interferon-β in multiple sclerosis are still not completely understood. In the present study, we evaluated the short and long-term effects of interferon-β treatment on different subsets of regulatory T cells in relapsing-remitting multiple sclerosis patients biologically responsive to treatment because of mixovirus resistance protein A inducibility., Methods: In this prospective longitudinal study, subsets of natural regulatory T cells (naïve, central memory and effector memory) and inducible regulatory T cells (Tr1), as well as in vitro-induced regulatory T cells (Tr1-like cells), were simultaneously quantified by flow cytometry in samples prepared from 148 therapy-naïve multiple sclerosis patients obtained before and after 6, 12, 18, and 24 months of interferon-β-1a treatment. mRNA for interleukin-10 and Tr1-related genes (CD18, CD49b, and CD46, together with Cyt-1 and Cyt-2 CD46-associated isoforms) were quantified in Tr1-like cells., Results: Despite profound inter-individual variations in the modulation of all regulatory T-cell subsets, the percentage of natural regulatory T cells increased after 6, 12, and 24 months of interferon-β treatment. This increase was characterized by the expansion of central and effector memory regulatory T-cell subsets. The percentage of Tr1 significantly enhanced at 12 months of therapy and continued to be high at the subsequent evaluation points. Patients experiencing relapses displayed a higher percentage of naïve regulatory T cells and a lower percentage of central memory regulatory T cells and of Tr1 before starting interferon-β therapy. In addition, an increase over time of central memory and of Tr1 was observed only in patients with stable disease. However, in vitro-induced Tr1-like cells, prepared from patients treated for 24 months, produced less amount of interleukin-10 mRNA compared with pre-treatment Tr1-like cells., Conclusion: Interferon-β induces the expansion of T regulatory subsets endowed with a high suppressive activity, especially in clinically stable patients. The overall concurrent modulation of natural and inducible regulatory T-cell subsets might explain the therapeutic effects of interferon-β in multiple sclerosis patients.

Published
2020
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37. 7-Hydroxymatairesinol improves body weight, fat and sugar metabolism in C57BJ/6 mice on a high-fat diet.

Author

Biasiotto G, Zanella I, Predolini F, Archetti I, Cadei M, Monti E, Luzzani M, Pacchetti B, Mozzoni P, Andreoli R, De Palma G, Serana F, Smeds A, and Di Lorenzo D

Subjects
3T3-L1 Cells, 4-Butyrolactone analogs & derivatives, 4-Butyrolactone pharmacology, 4-Butyrolactone therapeutic use, Adipogenesis drug effects, Adipogenesis genetics, Adipose Tissue cytology, Adipose Tissue drug effects, Adipose Tissue metabolism, Animals, Anti-Obesity Agents pharmacology, Anti-Obesity Agents therapeutic use, Dietary Supplements, Fatty Liver drug therapy, Fatty Liver metabolism, Gene Expression, Insulin Resistance, Lignans therapeutic use, Lipids blood, Male, Metabolic Syndrome blood, Metabolic Syndrome etiology, Metabolic Syndrome metabolism, Mice, Mice, Inbred C57BL, Obesity blood, Obesity etiology, Obesity metabolism, Obesity prevention & control, Plant Extracts pharmacology, Plant Extracts therapeutic use, Blood Glucose metabolism, Body Weight drug effects, Diet, High-Fat, Lignans pharmacology, Lipid Metabolism drug effects, Metabolic Syndrome drug therapy, Picea chemistry
Abstract

7-Hydroxymatairesinol (7-HMR) is a plant lignan abundant in various concentrations in plant foods. The objective of this study was to test HMRLignan™, a purified form of 7-HMR, and the corresponding Picea abies extract (total extract P. abies; TEP) as dietary supplements on a background of a high-fat diet (HFD)-induced metabolic syndrome in mice and in the 3T3-L1 adipogenesis model. Mice, 3 weeks old, were fed a HFD for 60 d. Subgroups were treated with 3 mg/kg body weight 7-HMR (HMRLignan™) or 10 mg/kg body weight TEP by oral administration. 7-HMR and TEP limited the increase in body weight (-11 and -13 %) and fat mass (-11 and -18 %) in the HFD-fed mice. Epididymal adipocytes were 19 and -12 % smaller and the liver was less steatotic (-62 and -65 %). Serum lipids decreased in TEP-treated mice (-11 % cholesterol, -23 % LDL and -15 % TAG) and sugar metabolism was ameliorated by both lignan preparations, as shown by a more than 70 % decrease in insulin secretion and insulin resistance. The expression of several metabolic genes was modulated by the HFD with an effect that was reversed by lignan. In 3T3-L1 cells, the 7-HMR metabolites enterolactone (ENL) and enterodiol (END) showed a 40 % inhibition of cell differentiation accompanied by the inhibited expression of the adipogenic genes PPARγ, C/EBPα and aP2. Furthermore, END and ENL caused a 10 % reduction in TAG uptake in HEPA 1-6 hepatoma cells. In conclusion, 7-HMR and TEP reduce metabolic imbalances typical of the metabolic syndrome and obesity in male mice, whereas their metabolites inhibit adipogenesis and lipid uptake in vitro.

Published
2018
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38. Secondary acute myeloid leukaemia in elderly patients: Patient's fitness criteria and ELN prognostic stratification can be applied to guide treatment decisions. An analysis of 280 patients by the network rete ematologica lombarda (REL).

Author

Borlenghi E, Pagani C, Zappasodi P, Bernardi M, Basilico C, Todisco E, Fracchiolla N, Mancini V, Turrini M, Da Vià M, Sala E, Cattaneo C, Petullà M, Serana F, Ferrario A, Cairoli R, Cortelezzi A, Santoro A, Castagnola C, and Rossi G

Subjects
Aged, Aged, 80 and over, Exercise Test, Female, Humans, Leukemia, Myeloid, Acute diagnosis, Leukemia, Myeloid, Acute etiology, Male, Neoplasms, Second Primary, Prognosis, Treatment Outcome, Clinical Decision-Making methods, Leukemia, Myeloid, Acute therapy
Published
2018
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39. Serum levels of tumor necrosis factor-alpha in patients with psoriasis before, during and after narrow-band UVB phototherapy.

Author

Rossi MT, Venturini M, Zanca A, Arisi M, Fusano M, Sottini A, Serana F, Imberti L, and Calzavara-Pinton P

Subjects
Adult, Aged, Cytokines immunology, Female, Humans, Male, Middle Aged, Psoriasis blood, Psoriasis physiopathology, Severity of Illness Index, Th1 Cells immunology, Th17 Cells immunology, Time Factors, Treatment Outcome, Young Adult, Psoriasis radiotherapy, Tumor Necrosis Factor-alpha blood, Ultraviolet Therapy methods
Abstract

Background: Narrow-band UVB (NB-UVB) phototherapy is widely used worldwide for moderate and severe psoriasis, which is a chronic autoimmune inflammatory disease characterized by skin infiltrates of Th1-, Th17- and Th22-cells releasing locally pro-inflammatory cytokines. We investigate serum levels of tumor necrosis factor-α (TNF-α) in psoriatic patients before and after NB-UVB phototherapy., Methods: Twenty-eight subjects with moderate/severe plaque type psoriasis were enrolled. The severity of skin involvement was rated according to the Psoriasis Area and Severity Index (PASI) score at baseline (T0) and after 4 (T1) and 12 (T2) weeks of NB-UVB treatment. At the same time points, blood samples were taken for evaluation of TNF-α levels. NB-UVB phototherapy was administered twice weekly on non-consecutive days until 12 weeks., Results: The median PASI score significantly decreased from 12.0 at baseline (T0), to 6.9 after 4 weeks (T1, P<0.001) and to 0 after 12 weeks (T2, P<0.001). TNF-a serum levels significantly increased in respect to the baseline after 12 weeks of therapy., Conclusions: NB-UVB phototherapy is highly effective against psoriasis but, as it increases the TNF-α serum level, it seems unlikely that it can decrease the chronic inflammatory state that is thought to be responsible of the systemic co-morbidities of psoriasis.

Published
2018
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40. Bone Marrow Stroma and Vascular Contributions to Myeloma Bone Homing.

Author

Moschetta M, Kawano Y, Sacco A, Belotti A, Ribolla R, Chiarini M, Giustini V, Bertoli D, Sottini A, Valotti M, Ghidini C, Serana F, Malagola M, Imberti L, Russo D, Montanelli A, Rossi G, Reagan MR, Maiso P, Paiva B, Ghobrial IM, and Roccaro AM

Subjects
Bone Marrow metabolism, Connective Tissue metabolism, Endothelial Cells cytology, Humans, Mesenchymal Stem Cells cytology, Multiple Myeloma metabolism, Neoplasm Metastasis, Tumor Microenvironment, Bone Marrow blood supply, Bone Neoplasms secondary, Connective Tissue blood supply, Endothelial Cells metabolism, Mesenchymal Stem Cells metabolism, Multiple Myeloma pathology
Abstract

Purpose of the Review: Herein we dissect mechanisms behind the dissemination of cancer cells from primary tumor site to the bone marrow, which are necessary for metastasis development, with a specific focus on multiple myeloma., Recent Findings: The ability of tumor cells to invade vessels and reach the systemic circulation is a fundamental process for metastasis development; however, the interaction between clonal cells and the surrounding microenvironment is equally important for supporting colonization, survival, and growth in the secondary sites of dissemination. The intrinsic propensity of tumor cells to recognize a favorable milieu where to establish secondary growth is the basis of the "seed and soil" theory. This theory assumes that certain tumor cells (the "seeds") have a specific affinity for the milieu of certain organs (the "soil"). Recent literature has highlighted the important contributions of the vascular niche to the hospitable "soil" within the bone marrow. In this review, we discuss the crucial role of stromal cells and endothelial cells in supporting primary growth, homing, and metastasis to the bone marrow, in the context of multiple myeloma, a plasma cell malignancy with the unique propensity to primarily grow and metastasize to the bone marrow.

Published
2017
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41. Development of PBC/SSc overlap syndrome in chronic GVHD patient: immunological implications in the presence of mitochondrial, nucleolar and spindle midzone autoantigens.

Author

Assandri R, Serana F, and Montanelli A

Abstract

Chronic Graft versus Host Disease (cGVHD) is a complex disease resulting from donor T-cell recognition of a genetically disparate recipient that is unable to reject donor cells after allogeneic Stem Cell Transplantation (HSCT). cGVHD has some features resembling to autoimmune diseases (AD) such as Sjögren syndrome, primary biliary cirrhosis (PBC) and scleroderma (SSc). Also patients with cGVHD could develop extensive cGVHD with scleroderma-like skin manifestations and other clinical signs similar to those of patients with scleroderma. We take into consideration a patient with GVHD that developed PBC/SSc overlap syndrome with a complex and particular autoantibodies profile. Indirect immunofluorescence (IIF) with double coloration showed a cytoplasmic mitochondrial-like pattern, a clumpy nucleolar staining pattern, and a cell-cycle related staining pattern. Following anaphase onset, proteins regulator of cytokinesis localizes to the overlap zone on the ends of midzone microtubules and becomes compacted during furrow ingression to form the midbody. Second level tests confirmed the presence of anti-mitochondrial antibodies M2-subunit but no other autoantibodies were found. We performed a home-made immunoblot analysis that identified a 37 kDa fibrillarin band, and not identify 47 kDa, 31KDa and 18/20 kDa bands. After literature review of these possible cellular localizations, the proteins recognized by our patient's serum seem likely to be Aab to core midzone organizer components. However, due to the unavailability of the proper techniques in our laboratory, we were not able to further characterize them. The pathogenesis and morbidity of cGVHD after HSCT remains enigmatic, but the presence of specific autoantibodies are the hallmark of AD and represent a possibility of differential diagnosis. Standard techniques combined with the use of non-routinely laboratory techniques are a usefully and complementary method for studying difficult and particular cases. In fact, these autoantibodies will be considered as ''diagnostic'' and not as ''esoteric'' antibodies. In conclusion, a re-assessment of the diagnostic protocols in cGVHD together with a precise observation of the clinical and laboratory picture will ultimately help us clarify the disease and could provide a better understanding of the immune network deregulation.

Published
2017

42. Detection of newly produced T and B lymphocytes by digital PCR in blood stored dry on nylon flocked swabs.

Author

Tessitore MV, Sottini A, Roccaro AM, Ghidini C, Bernardi S, Martellosio G, Serana F, and Imberti L

Subjects
Adolescent, Adult, Aged, Aged, 80 and over, DNA isolation & purification, Electrophoresis, Agar Gel, HeLa Cells, Humans, Middle Aged, Recombination, Genetic genetics, Reproducibility of Results, Young Adult, B-Lymphocytes immunology, Blood Specimen Collection methods, Nylons chemistry, Real-Time Polymerase Chain Reaction methods, T-Lymphocytes immunology
Abstract

Background: A normal number of T-cell receptor excision circles (TRECs) and K-deleting recombination excision circles (KRECs) is considered a biomarker for adequate new T- and B-cell production. In newborns, detection of TRECs and KRECs by real time PCR from dried blood spotted on filter paper is used for the screening of severe immunodeficiency. In adults, elderly and during diseases, where the number of TRECs is lower than in newborns and children, a large amount of DNA and a sensitive method of amplification are necessary to identify newly produced lymphocytes., Methods: DNA was prepared from blood of 203 healthy adults (range: 18-91 years old) absorbed for 10 s on flocked swabs and let to dry, or from peripheral blood mononuclear cells. DNA was subjected to digital PCR and to well established conventional real time PCR-based method using TREC- and KREC-specific primers and probes. The number of TRECs and KRECs was expressed per mL of blood. Statistical analysis was performed by nested ANOVA, Pearson coefficient of determination, and by linear regression tests., Results: The novel method for the storage of dried blood on nylon flocked swabs and the use of digital PCR allow quantification of TRECs and KRECs with high degree of sensitivity, specificity, accuracy, and precision. TRECs and KRECs were amplified by digital PCR in all tested blood samples, including those obtained from elderly individuals (>70 years old) and that were negative by real time PCR. Furthermore, values of TRECs and KRECs obtained by digital PCR were in the range of those acquired by real time PCR., Conclusions: Our findings demonstrate that DNA isolation from dried blood on flocked swabs followed by digital PCR-based analysis represents a useful tool for studying new lymphocyte production in adults and elderly individuals. This suggests the potential use of the methodology when monitoring of clinical variables is limited by the number of molecules that can be amplified and detected, such as in patients with immunodeficiency or under immunosuppressive therapies.

Published
2017
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43. B- and T-lymphocyte number and function in HIV + /HIV - lymphoma patients treated with high-dose chemotherapy and autologous bone marrow transplantation.

Author

Bertoli D, Re A, Chiarini M, Sottini A, Serana F, Giustini V, Roccaro AM, Cattaneo C, Caimi L, Rossi G, and Imberti L

Subjects
Adult, Aged, Anti-Retroviral Agents pharmacology, Antineoplastic Agents pharmacology, B-Lymphocytes drug effects, Cell Proliferation drug effects, Combined Modality Therapy, Consolidation Chemotherapy, Female, HIV Infections immunology, HIV Infections virology, Humans, Lymphoma, Non-Hodgkin immunology, Lymphoma, Non-Hodgkin virology, Male, Middle Aged, Salvage Therapy, T-Lymphocytes drug effects, Transplantation, Autologous, Anti-Retroviral Agents administration & dosage, Antineoplastic Agents administration & dosage, B-Lymphocytes physiology, Bone Marrow Transplantation methods, HIV Infections therapy, Lymphoma, Non-Hodgkin therapy, T-Lymphocytes physiology
Abstract

Combination of anti-retroviral therapy, high-dose chemotherapy (HCT) and autologous stem cell transplantation (ASCT) has led to an improved survival of HIV + non-Hodgkin lymphoma (NHL) patients. We compared T- and B-cell subset recovery and related capability to respond to in-vitro stimulation, as well as T-cell repertoire modifications of HIV + and HIV - NHL patients undergoing HCT and ASCT as first-line consolidation or salvage treatment, using sequential blood samples obtained before and at 3, 6, 12 and 24 months after ASCT. B lymphocyte recovery occurred earlier, reaching higher levels in HIV + patients as compared to HIV - patients and healthy controls; in particular, immature and naïve B cells were significantly higher in HIV + patients who had received rituximab in the pre-ASCT period. These lymphocytes equally responded to in-vitro stimulation. Newly produced T cells similarly increased in HIV + and HIV - NHL patients, but their levels remained constantly lower than in healthy controls. T lymphocytes showed a reduced proliferative capacity, but their repertoire was reassorted by the treatment. The functional and numeric B-cell recovery and the qualitative modifications of T-cell receptor repertoire may explain, at least in part, the success of this aggressive therapeutic approach in HIV + patients.

Published
2016
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44. Diagnosis, Treatment and Long-Term Follow Up of Patients with ADA Deficiency: a Single-Center Experience.

Author

Baffelli R, Notarangelo LD, Imberti L, Hershfield MS, Serana F, Santisteban I, Bolda F, Porta F, and Lanfranchi A

Subjects
Adenosine Deaminase genetics, Agammaglobulinemia epidemiology, Agammaglobulinemia therapy, Child, Preschool, Consanguinity, DNA Mutational Analysis, Female, Follow-Up Studies, Humans, Infant, Italy, Male, Mutation genetics, Retrospective Studies, Roma, Severe Combined Immunodeficiency epidemiology, Severe Combined Immunodeficiency therapy, Treatment Outcome, Adenosine Deaminase deficiency, Adenosine Deaminase metabolism, Agammaglobulinemia diagnosis, Enzyme Replacement Therapy, Genetic Therapy, Hematopoietic Stem Cell Transplantation, Severe Combined Immunodeficiency diagnosis
Abstract

Purpose: We carried out a retrospective analysis of 27 patients with Adenosine Deaminase (ADA) deficiency diagnosed in a single center from 1997 to the 2013, for evaluating whether data regarding types of disease-inducing mutations, biochemical and immunological features as well as clinical outcomes of patients treated with enzyme replacement or transplantation, were comparable to those obtained in multicenter studies., Methods: The ADA deficiency diagnosis was performed with biochemical, immunological and molecular techniques. Ten patients treated with hematopoietic stem cell transplantation and three in treatment with enzyme replacement were followed up in our center., Results: Twenty-four different mutations were identified and five were not previously reported. Identical mutations were found among patients from the same Romani ethnic group or from the same geographical region. A more rapid recovery was observed in enzyme replacement treated patients in comparison with those transplanted that, however, showed a continuous and long-lasting improvement both in terms of immune and metabolic recovery., Conclusion: The data obtained in our single center are comparable with those that have been reported in multicenter surveys.

Published
2015
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45. Less Frequent and Less Severe Flu-Like Syndrome in Interferon Beta-1a Treated Multiple Sclerosis Patients with at Least One Allele Bearing the G>C Polymorphism at Position -174 of the IL-6 Promoter Gene.

Author

Bertoli D, Serana F, Sottini A, Cordioli C, Maimone D, Amato MP, Centonze D, Florio C, Puma E, Capra R, and Imberti L

Subjects
Adolescent, Adult, Enzyme-Linked Immunosorbent Assay, Female, Humans, Interleukin-6 blood, Male, Middle Aged, Multiple Sclerosis drug therapy, Polymerase Chain Reaction, Respiratory Tract Diseases diagnosis, Syndrome, Tumor Necrosis Factor-alpha genetics, Young Adult, Antineoplastic Agents therapeutic use, Interferon beta-1a therapeutic use, Interleukin-6 genetics, Multiple Sclerosis complications, Polymorphism, Single Nucleotide genetics, Promoter Regions, Genetic genetics, Respiratory Tract Diseases etiology
Abstract

One of the most common adverse event of interferon beta (IFNβ) therapy for multiple sclerosis is flu-like syndrome (FLS), which has been reportedly related to increased levels of cytokines such as interleukin 6 (IL-6) and tumor necrosis factor-alpha (TNF-α). Average cytokine levels can be affected by single nucleotide polymorphism in the gene promoter regions. To investigate whether IL-6 -174 G>C and TNF-α -376 G>A polymorphisms could be correlated to the incidence of FLS, and whether an anti-inflammatory/antipyretic therapy may influence FLS development, a prospective observational study was performed in 190 treatment naïve, multiple sclerosis patients who started IM IFNβ-1a 30mcg once weekly. The identification of IL-6 -174 G>C and TNF-α -376 G>A polymorphisms was achieved by performing an amplification-refractory mutation system. Serum IL-6 levels were measured using enzyme-linked immunosorbent assay in blood samples taken before therapy and then after the first and last IFNβ-1a injection of the follow-up. FLS-related symptoms were recorded by patients once per week during the first 12 weeks of therapy into a self-reported diary. We found that patients carrying at least one copy of the C allele at position -174 in the promoter of IL-6 gene produced lower levels of IL-6 and were less prone to develop FLS, which was also less severe. On the contrary, the polymorphism of TNF-α had no effect on FLS. Patients taking the first dose of anti-inflammatory/antipyretic therapy in the peri-injection period (within 1 hour) experienced a reduced FLS severity. In conclusion, the study of IL-6 -174 G>C polymorphism would allow the identification of patients lacking the C nucleotide on both alleles who are at risk of a more severe FLS, and may be addressed to a timely and stronger anti-inflammatory/antipyretic therapy for a more effective FLS prevention.

Published
2015
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46. Newly produced T and B lymphocytes and T-cell receptor repertoire diversity are reduced in peripheral blood of fingolimod-treated multiple sclerosis patients.

Author

Chiarini M, Sottini A, Bertoli D, Serana F, Caimi L, Rasia S, Capra R, and Imberti L

Subjects
Adult, Female, Humans, Male, Middle Aged, Multiple Sclerosis, Relapsing-Remitting blood, B-Lymphocytes drug effects, Cell Proliferation drug effects, Fingolimod Hydrochloride pharmacology, Immunosuppressive Agents pharmacology, Multiple Sclerosis, Relapsing-Remitting drug therapy, Receptors, Antigen, T-Cell drug effects, T-Lymphocyte Subsets drug effects
Abstract

Background: Fingolimod inhibits lymphocyte egress from lymphoid tissues, thus altering the composition of the peripheral lymphocyte pool of multiple sclerosis patients., Objective: The objective of this paper is to evaluate whether fingolimod determines a decrease of newly produced T- and B-lymphocytes in the blood and a reduction in the T-cell receptor repertoire diversity that may affect immune surveillance., Methods: Blood samples were obtained from multiple sclerosis patients before fingolimod therapy initiation and then after six and 12 months. Newly produced T and B lymphocytes were measured by quantifying T-cell receptor excision circles and K-deleting recombination excision circles by real-time PCR, while recent thymic emigrants, naive CD8(+) lymphocytes, immature and naive B cells were determined by immune phenotyping. T-cell receptor repertoire was analyzed by complementarity determining region 3 spectratyping., Results: Newly produced T and B lymphocytes were significantly reduced in peripheral blood of fingolimod-treated patients. The decrease was particularly evident in the T-cell compartment. T-cell repertoire restrictions, already present before therapy, significantly increased after 12 months of treatment., Conclusions: These results do not have direct clinical implications but they may be useful for further understanding the mode of action of this immunotherapy for multiple sclerosis patients., (© The Author(s), 2014.)

Published
2015
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47. Immunological biomarkers identifying natalizumab-treated multiple sclerosis patients at risk of progressive multifocal leukoencephalopathy.

Author

Serana F, Chiarini M, Sottini A, Bertoli D, Giustini V, Tessitore MV, Caimi L, Capra R, and Imberti L

Subjects
Biomarkers, Humans, JC Virus immunology, Multiple Sclerosis drug therapy, Natalizumab, Risk Factors, Antibodies, Monoclonal, Humanized adverse effects, Immunologic Factors adverse effects, Leukoencephalopathy, Progressive Multifocal chemically induced, Leukoencephalopathy, Progressive Multifocal diagnosis, Leukoencephalopathy, Progressive Multifocal immunology
Abstract

Natalizumab-induced progressive multifocal leukoencephalopathy appears to be unleashed by complex interactions between viral and immunological host factors leading the latent form of JC virus to become pathogenic. Positive anti-JC virus antibody status, prior use of immunosuppressants, and increasing duration of natalizumab treatment have been proposed as risk factors for progressive multifocal leukoencephalopathy in multiple sclerosis patients, but while they may help to identify the most appropriate patients for natalizumab, their use have some limitations. Therefore, a large body of studies is ongoing to identify alternative, reliable immunological markers capable to improve the safety and efficacy of therapy, and to guide tailored clinical decisions., (Copyright © 2014 Elsevier B.V. All rights reserved.)

Published
2014
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48. Simultaneous quantification of T-cell receptor excision circles (TRECs) and K-deleting recombination excision circles (KRECs) by real-time PCR.

Author

Sottini A, Serana F, Bertoli D, Chiarini M, Valotti M, Vaglio Tessitore M, and Imberti L

Subjects
Adolescent, Adult, B-Lymphocytes immunology, B-Lymphocytes physiology, Base Sequence, Child, Child, Preschool, DNA, Circular blood, DNA, Circular genetics, Female, Humans, Middle Aged, Molecular Sequence Data, Receptors, Antigen, T-Cell blood, Recombination, Genetic, T-Lymphocytes immunology, T-Lymphocytes physiology, Young Adult, DNA, Circular analysis, Real-Time Polymerase Chain Reaction methods, Receptors, Antigen, T-Cell genetics
Abstract

T-cell receptor excision circles (TRECs) and K-deleting recombination excision circles (KRECs) are circularized DNA elements formed during recombination process that creates T- and B-cell receptors. Because TRECs and KRECs are unable to replicate, they are diluted after each cell division, and therefore persist in the cell. Their quantity in peripheral blood can be considered as an estimation of thymic and bone marrow output. By combining well established and commonly used TREC assay with a modified version of KREC assay, we have developed a duplex quantitative real-time PCR that allows quantification of both newly-produced T and B lymphocytes in a single assay. The number of TRECs and KRECs are obtained using a standard curve prepared by serially diluting TREC and KREC signal joints cloned in a bacterial plasmid, together with a fragment of T-cell receptor alpha constant gene that serves as reference gene. Results are reported as number of TRECs and KRECs/10(6) cells or per ml of blood. The quantification of these DNA fragments have been proven useful for monitoring immune reconstitution following bone marrow transplantation in both children and adults, for improved characterization of immune deficiencies, or for better understanding of certain immunomodulating drug activity.

Published
2014
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49. MxA mRNA quantification and disability progression in interferon beta-treated multiple sclerosis patients.

Author

Serana F, Imberti L, Amato MP, Comi G, Gasperini C, Ghezzi A, Martinelli V, Provinciali L, Rottoli MR, Sotgiu S, Stecchi S, Vecchio M, Zaffaroni M, Cordioli C, and Capra R

Subjects
Adolescent, Adult, Antibodies, Neutralizing, Biomarkers metabolism, Female, Humans, Kinetics, Male, Middle Aged, Myxovirus Resistance Proteins metabolism, Patient Dropouts, Protein Isoforms genetics, Protein Isoforms metabolism, Protein Subunits genetics, Protein Subunits metabolism, RNA, Messenger genetics, RNA, Messenger metabolism, Receptor, Interferon alpha-beta metabolism, Young Adult, Disability Evaluation, Disease Progression, Interferon-beta therapeutic use, Multiple Sclerosis drug therapy, Multiple Sclerosis genetics, Myxovirus Resistance Proteins genetics
Abstract

Even though anti-interferon beta (IFNβ) antibodies are the main determinants of IFNβ bioactivity loss and Myxovirus-resistance protein A (MxA) is the most established marker of IFNβ biological activity in IFNβ-treated multiple sclerosis patients, their usefulness in the routine clinical practice is still debated. Therefore, 118 multiple sclerosis patients naïve for treatment were enrolled for a 3-year longitudinal observational study mimicking the conditions of a real-world setting. In order to evaluate the kinetics of bioactivity loss in blood samples obtained every 6 months after therapy initiation, MxA and interferon receptor isoform/subunit mRNA were quantified by real-time PCR, anti-IFNβ binding antibodies were detected by radioimmunoprecipitation, and neutralizing antibodies by cytopathic effect inhibition assay. Clinical measures of disease activity and disability progression were also obtained at all time points. We found that, at the individual-patient level, the response to IFNβ therapy was extremely heterogeneous, including patients with stable or transitory, early or late loss of IFNβ bioactivity, and patients with samples lacking MxA mRNA induction in spite of absence of antibodies. No interferon receptor isoform alterations that could explain these findings were found. At the group level, none of these biological features correlated with the measures of clinical disease activity or progression. However, when MxA mRNA was evaluated not at the single time point as a dichotomic marker (induced vs. non-induced), but as the mean of its values measured over the 6-to-24 month period, the increasing average MxA predicted a decreasing risk of short-term disability progression, independently from the presence of relapses. Therefore, a more bioactive treatment, even if unable to suppress relapses, reduces their severity by an amount that is proportional to MxA levels. Together with its feasibility in the routine laboratory setting, these data warrant the quantification of MxA mRNA as a primary tool for a routine monitoring of IFNβ therapy.

Published
2014
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50. Modulation of Regulatory T-Cell Subsets in Very Long-Term Treated Aviremic HIV(+) Patients and Untreated Viremic Patients.

Author

Serana F, Chiarini M, Quiros-Roldan E, Gotti D, Zanotti C, Sottini A, Bertoli D, Caimi L, and Imberti L

Abstract

Naïve, central- and effector-like memory regulatory T cells (Tregs) were evaluated in untreated and long-term antiretroviral-treated HIV(+) patients that showed comparable CD4(+) cell levels, while being, respectively, viremic and aviremic. In the untreated patients, the percentage of naïve-like Tregs was significantly increased to the detriment of central memory regulatory T cells. This redistribution of regulatory Treg subsets may contribute to explain the partially preserved CD4(+) cell counts seen in these patients despite the ongoing viremia. On the contrary, in the long-term treated patients, the percentages of Treg subsets were similar to those of healthy donors, demonstrating a restored Treg homeostasis. The characterization of Treg subsets, rather than an evaluation of the total Treg population, may lead to a deeper understanding of the Treg role in HIV infection and therapy.

Published
2014
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