Your search keyword '"Pancino G"' showing total 8 results

1. Setting of Methods for Analysis of Mucosal Antibodies in Seminal and Vaginal Fluids of HIV Seropositive Subjects from Cambodian and Italian Cohorts

Author

Marie Ngyen, L. Diomede, Giulia Gallotta, Davide Ferrari, Janin Nouhin, Lorenza Scotti, Giovanni Corrao, Cinzia Bisighini, Gianfranco Pancino, Lucia DeSantis, Carla Donadoni, Lucia Lopalco, Antonella Zambon, Division of Immunology, Infectious Diseases and Transplantation, San Raffaele Scientific Institute, Department of Statistics, Università degli Studi di Milano-Bicocca [Milano] (UNIMIB), Institut Pasteur du Cambodge, Réseau International des Instituts Pasteur (RIIP), Department of Obsterics and Gynaecology, San Raffaele Scientific Institute-University Vita Salute, Department of Infectious Diseases, Régulation des Infections Rétrovirales, Institut Pasteur [Paris], Università degli Studi di Milano-Bicocca = University of Milano-Bicocca (UNIMIB), Institut Pasteur [Paris] (IP), Donadoni, C, Bisighini, C, Scotti, L, Diomede, L, Ngyen, M, Nouhin, J, Desantis, L, Zambon, A, Ferrari, D, Gallotta, G, Corrao, G, Pancino, G, and Lopalco, L

Subjects

Male, Immunoglobulin A, HIV Infections, MESH: Body Fluids, Cohort Studies, 0302 clinical medicine, Vaginal Fluid, HIV Seropositivity, 030212 general & internal medicine, MESH: Cohort Studies, Virology/Vaccines, 0303 health sciences, MESH: Middle Aged, Multidisciplinary, biology, MESH: Enzyme-Linked Immunosorbent Assay, Mucous membrane, MESH: HIV Infections, Middle Aged, Infectious Diseases/HIV Infection and AIDS, Body Fluids, 3. Good health, medicine.anatomical_structure, Italy, Vagina, Medicine, Female, Antibody, Cambodia, Research Article, Adult, Science, Enzyme-Linked Immunosorbent Assay, Semen, Antibodies, 03 medical and health sciences, MESH: HIV Seropositivity, Immune system, Immunity, Immunology/Immunity to Infections, Infectious Diseases/Viral Infections, Infectious Diseases/Sexually Transmitted Diseases, medicine, Humans, Seminal fluid, MESH: Immunoglobulin A, MESH: Semen, 030304 developmental biology, Antiserum, MESH: Humans, Mucous Membrane, MESH: Antibodies, MESH: Cambodia, HIV, MESH: Italy, MESH: Mucous Membrane, MESH: Adult, MESH: Male, MESH: Vagina, Immunology/Immune Response, Immunology, Mucosal Antibodie, biology.protein, Virology/Host Antiviral Responses, MESH: Female, [SDV.MHEP]Life Sciences [q-bio]/Human health and pathology

Abstract

BackgroundGenital mucosae play a key role in protection from STD and HIV infection, due to their involvement in both horizontal and vertical disease transmission. High variability of published observations concerning IgA isolation and quantification underlies the strong requirement of specific methods able to maximize investigation on HIV-specific IgA.MethodologyGenital fluids from 109 subjects, including male and female cohorts from Italy and Cambodia, were collected, aliquoted and processed with different techniques, to assess optimal conditions maximizing mucosal antibody recovery. Three sampling techniques, up to sixteen preservation conditions, six ELISA methods and four purifications protocols were compared.Principal findingsThe optimal method here described took advantage of Weck-Cel sampling of female mucosal fluids. Immediate processing of genital fluids, with the addition of antibiotics and EDTA, improved recovery of vaginal IgA, while the triple addition of EDTA, antibiotics and protease inhibitors provided the highest amount of seminal IgA. Due to low amount of IgA in mucosal fluids, a high sensitive sandwich ELISA assay was set; sensitivity was enhanced by milk-based overcoating buffer and by a two-step biotin-streptavidin signal amplification. Indeed, commercial antisera to detect human immunoglobulins showed weak cross-reactivity to different antibody types. Three-step affinity purification provided reproducible immunoglobulin recovery from genital specimens, while conventional immuno-affinity IgA purification was found poorly manageable. Affinity columns were suitable to isolate mucosal IgA, which are ten-fold less concentrated than IgG in genital specimens, and provided effective separation of IgA monomers, dimers, and J-chains. Jacalin-bound resin successfully separated IgA1 from IgA2 subfraction.Conclusions/significanceSpecific, effective and reliable methods to study local immunity are key items in understanding host mucosal response. The sequence of methods here described is effective and reliable in analysing humoral local responses, and may provide a solid advance to identify and measure the effective mucosal responses to HIV.

Published

2010

2. Dendritic Cells from HIV Controllers Have Low Susceptibility to HIV-1 Infection In Vitro but High Capacity to Capture HIV-1 Particles.

Author

Hamimi C, David A, Versmisse P, Weiss L, Bruel T, Zucman D, Appay V, Moris A, Ungeheuer MN, Lascoux-Combe C, Barré-Sinoussi F, Muller-Trutwin M, Boufassa F, Lambotte O, Pancino G, and Sáez-Cirión A

Subjects

Antigens, Viral immunology, CD8-Positive T-Lymphocytes cytology, CD8-Positive T-Lymphocytes immunology, Dendritic Cells cytology, Dendritic Cells metabolism, Disease Susceptibility, Gene Expression Regulation, Humans, Lectins, C-Type metabolism, Syndecan-3 metabolism, Virus Replication, Dendritic Cells immunology, Dendritic Cells virology, HIV Infections immunology, HIV-1 physiology

Abstract

HIV controllers (HICs), rare HIV-1 infected individuals able to control viral replication without antiretroviral therapy, are characterized by an efficient polyfunctional and cytolytic HIV-specific CD8+ T cell response. The mechanisms underlying the induction and maintenance of such response in many HICs despite controlled viremia are not clear. Dendritic cells play a crucial role in the generation and reactivation of T cell responses but scarce information is available on those cells in HICs. We found that monocyte derived dendritic cells (MDDCs) from HICs are less permissive to HIV-1 infection than cells from healthy donors. In contrast MDDCs from HICs are particularly efficient at capturing HIV-1 particles when compared to cells from healthy donors or HIV-1 patients with suppressed viral load on antiretroviral treatment. MDDCs from HICs expressed on their surface high levels of syndecan-3, DC-SIGN and MMR, which could cooperate to facilitate HIV-1 capture. The combination of low susceptibility to HIV-1 infection but enhanced capacity to capture particles might allow MDDCs from HICs to preserve their function from the deleterious effect of infection while facilitating induction of HIV-specific CD8+ T cells by cross-presentation in a context of low viremia.

Published

2016

3. Potential role for HIV-specific CD38-/HLA-DR+ CD8+ T cells in viral suppression and cytotoxicity in HIV controllers.

Author

Hua S, Lécuroux C, Sáez-Cirión A, Pancino G, Girault I, Versmisse P, Boufassa F, Taulera O, Sinet M, Lambotte O, and Venet A

Subjects

Adult, Antigens, CD immunology, Case-Control Studies, Cells, Cultured, Female, Flow Cytometry, HIV Infections prevention & control, HIV Infections virology, Humans, Immunophenotyping, Lymphocyte Activation, Male, Middle Aged, ADP-ribosyl Cyclase 1 immunology, CD8-Positive T-Lymphocytes immunology, HIV Infections immunology, HIV-1 immunology, HLA-DR Antigens immunology, T-Lymphocytes, Cytotoxic immunology

Abstract

Background: HIV controllers (HIC) are rare HIV-1-infected patients who exhibit spontaneous viral control. HIC have high frequency of CD38-/HLA-DR+ HIV-specific CD8+ T cells. Here we examined the role of this subset in HIC status., Materials and Methods: We compared CD38-/HLA-DR+ CD8+ T cells with the classical CD38+/HLA-DR+ activated phenotype in terms of 1) their activation status, reflected by CD69, CD25, CD71, CD40 and Ki67 expression, 2) functional parameters: Bcl-2 expression, proliferative capacity, and IFN-γ and IL-2 production, and 3) cytotoxic activity. We also investigated how this particular profile is generated., Results: Compared to CD38+/HLA-DR+ cells, CD38-/HLA-DR+ cells exhibited lower expression of several activation markers, better survival capacity (Bcl-2 MFI, 367 [134-462] vs 638 [307-747], P = 0.001), higher frequency of polyfunctional cells (15% [7%-33%] vs 21% [16%-43%], P = 0.0003), greater proliferative capacity (0-fold [0-2] vs 3-fold [2]-[11], P = 0.007), and higher cytotoxicity in vitro (7% [3%-11%] vs 13% [6%-22%], P = 0.02). The CD38-/HLA-DR+ profile was preferentially generated in response to low viral antigen concentrations., Conclusions: These data highlight the role of CD38-/HLA-DR+ HIV-specific CD8+ T cell cytotoxicity in HIC status and provide insights into the mechanism by which they are generated. Induction of this protective CD8+ subset may be important for vaccine strategies.

Published

2014

4. Blunted response to combination antiretroviral therapy in HIV elite controllers: an international HIV controller collaboration.

Author

Boufassa F, Lechenadec J, Meyer L, Costagliola D, Hunt PW, Pereyra F, Deeks S, Pancino G, Taulera O, Lichterfeld M, Delobel P, Saez-Cirion A, and Lambotte O

Subjects

Adult, CD4 Lymphocyte Count, Cohort Studies, Female, HIV Infections immunology, Humans, Kinetics, Linear Models, Male, Middle Aged, Viremia virology, Antiretroviral Therapy, Highly Active, HIV Infections drug therapy, International Cooperation

Abstract

Objective: HIV "elite controllers" (ECs) spontaneously control viral load, but some eventually require combination antiretroviral treatment (cART), due to a loss of viral control or a decline in CD4 T-cell counts. Here we studied the CD4 T-cell count dynamics after cART initiation among 34 ECs followed in U.S. and European cohorts, by comparison with chronically viremic patients (VIRs)., Methods: ECs were defined as patients with at least ≥5 viral load (VL) measurements below 400 copies/mL during at least a 5-year period despite never receiving ART and were selected from the French ANRS CO18 cohort, the U.S. SCOPE cohort, the International HIV Controllers study and the European CASCADE collaboration. VIRs were selected from the ANRS COPANA cohort of recently-diagnosed (<1 year) ART-naïve HIV-1-infected adults. CD4 T-cell count dynamics after cART initiation in both groups were modelled with piecewise mixed linear models., Results: After cART initiation, CD4 T-cell counts showed a biphasic rise in VIRs with: an initial rapid increase during the first 3 months (+0.63√CD4/month), followed by +0.19√CD4/month. This first rapid phase was not observed in ECs, in whom the CD4Tc count increased steadily, at a rate similar to that of the second phase observed in VIRs. After cART initiation at a CD4 T-cell count of 300/mm(3), the estimated mean CD4 T-cell gain during the first 12 months was 139/mm(3) in VIRs and 80/mm(3) in ECs (p = 0.048)., Conclusions: cART increases CD4 T-cell counts in elite controllers, albeit less markedly than in other patients.

Published

2014

5. CD8 T-cells from most HIV-infected patients lack ex vivo HIV-suppressive capacity during acute and early infection.

Author

Lécuroux C, Girault I, Chéret A, Versmisse P, Nembot G, Meyer L, Rouzioux C, Pancino G, Venet A, and Sáez-Cirión A

Subjects

Acute Disease, Adult, CD4-Positive T-Lymphocytes cytology, Cells, Cultured, Cytokines metabolism, Disease Progression, Female, HIV-1 physiology, Humans, Interleukin-2 metabolism, Leukocytes, Mononuclear metabolism, Male, Middle Aged, Time Factors, Viral Load, Virus Replication, CD8-Positive T-Lymphocytes immunology, CD8-Positive T-Lymphocytes virology, HIV Infections immunology, HIV Infections virology

Abstract

The strong CD8+ T-cell-mediated HIV-1-suppressive capacity found in a minority of HIV-infected patients in chronic infection is associated with spontaneous control of viremia. However, it is still unclear whether such capacities were also present earlier in the CD8+ T cells from non controller patients and then lost as a consequence of uncontrolled viral replication. We studied 50 patients with primary HIV-1-infection to determine whether strong CD8+ T-cell-mediated HIV suppression is more often observed at that time. Despite high frequencies of polyfunctional HIV-specific CD8+ T-cells and a strong CD4+ T-helper response, CD8+ T-cells from 48 patients lacked strong HIV-suppressive capacities ex vivo. This indicates that the superior HIV-suppressive capacity of CD8+ T-cells from HIV controllers is not a general characteristic of the HIV-specific CD8+ T cell response in primary HIV infection.

Published

2013

6. The AP-1 binding sites located in the pol gene intragenic regulatory region of HIV-1 are important for viral replication.

Author

Colin L, Vandenhoudt N, de Walque S, Van Driessche B, Bergamaschi A, Martinelli V, Cherrier T, Vanhulle C, Guiguen A, David A, Burny A, Herbein G, Pancino G, Rohr O, and Van Lint C

Subjects

Base Sequence, Binding Sites, Enhancer Elements, Genetic genetics, Genes, Dominant genetics, Humans, Jurkat Cells, Macrophages drug effects, Macrophages virology, Molecular Sequence Data, Monocytes drug effects, Monocytes virology, Point Mutation genetics, Protein Binding drug effects, Proto-Oncogene Proteins c-fos metabolism, Proto-Oncogene Proteins c-jun metabolism, RNA Polymerase II metabolism, T-Lymphocytes drug effects, T-Lymphocytes virology, Tetradecanoylphorbol Acetate pharmacology, tat Gene Products, Human Immunodeficiency Virus, Genes, pol genetics, HIV-1 genetics, HIV-1 physiology, Regulatory Sequences, Nucleic Acid genetics, Transcription Factor AP-1 metabolism, Virus Replication genetics

Abstract

Our laboratory has previously identified an important intragenic region in the human immunodeficiency virus type 1 (HIV-1) genome, whose complete functional unit is composed of the 5103 fragment, the DNaseI-hypersensitive site HS7 and the 5105 fragment. These fragments (5103 and 5105) both exhibit a phorbol 12-myristate 13-acetate (PMA)-inducible enhancer activity on the herpes simplex virus thymidine kinase promoter. Here, we characterized the three previously identified AP-1 binding sites of fragment 5103 by showing the PMA-inducible in vitro binding and in vivo recruitment of c-Fos, JunB and JunD to this fragment located at the end of the pol gene. Functional analyses demonstrated that the intragenic AP-1 binding sites are fully responsible for the PMA-dependent enhancer activity of fragment 5103. Moreover, infection of T-lymphoid Jurkat and promonocytic U937 cells with wild-type and mutant viruses demonstrated that mutations of the intragenic AP-1 sites individually or in combination altered HIV-1 replication. Importantly, mutations of the three intragenic AP-1 sites led to a decreased in vivo recruitment of RNA polymerase II to the viral promoter, strongly supporting that the deleterious effect of these mutations on viral replication occurs, at least partly, at the transcriptional level. Single-round infections of monocyte-derived macrophages confirmed the importance of intragenic AP-1 sites for HIV-1 infectivity.

Published

2011

7. Human TRIM gene expression in response to interferons.

Author

Carthagena L, Bergamaschi A, Luna JM, David A, Uchil PD, Margottin-Goguet F, Mothes W, Hazan U, Transy C, Pancino G, and Nisole S

Subjects

Humans, Macrophages drug effects, Macrophages metabolism, Phylogeny, Promoter Regions, Genetic, Reverse Transcriptase Polymerase Chain Reaction, Adaptor Proteins, Signal Transducing genetics, Gene Expression Regulation drug effects, Interferons pharmacology, Membrane Proteins genetics

Abstract

Background: Tripartite motif (TRIM) proteins constitute a family of proteins that share a conserved tripartite architecture. The recent discovery of the anti-HIV activity of TRIM5alpha in primate cells has stimulated much interest in the potential role of TRIM proteins in antiviral activities and innate immunity., Principal Findings: To test if TRIM genes are up-regulated during antiviral immune responses, we performed a systematic analysis of TRIM gene expression in human primary lymphocytes and monocyte-derived macrophages in response to interferons (IFNs, type I and II) or following FcgammaR-mediated activation of macrophages. We found that 27 of the 72 human TRIM genes are sensitive to IFN. Our analysis identifies 9 additional TRIM genes that are up-regulated by IFNs, among which only 3 have previously been found to display an antiviral activity. Also, we found 2 TRIM proteins, TRIM9 and 54, to be specifically up-regulated in FcgammaR-activated macrophages., Conclusions: Our results present the first comprehensive TRIM gene expression analysis in primary human immune cells, and suggest the involvement of additional TRIM proteins in regulating host antiviral activities.

Published

2009

8. The CD85j+ NK cell subset potently controls HIV-1 replication in autologous dendritic cells.

Author

Scott-Algara D, Arnold V, Didier C, Kattan T, Pirozzi G, Barré-Sinoussi F, and Pancino G

Subjects

Coculture Techniques, Dendritic Cells virology, HIV Infections pathology, Humans, Killer Cells, Natural virology, Leukocyte Immunoglobulin-like Receptor B1, Leukocytes, Mononuclear cytology, Leukocytes, Mononuclear virology, Ligands, Models, Biological, Monocytes cytology, Monocytes metabolism, Monocytes virology, Phenotype, Recombinant Proteins chemistry, Antigens, CD biosynthesis, Dendritic Cells cytology, HIV-1 metabolism, Killer Cells, Natural cytology, Receptors, Immunologic biosynthesis, Virus Replication

Abstract

Natural killer (NK) cells and dendritic cells (DC) are thought to play critical roles in the first phases of HIV infection. In this study, we examined changes in the NK cell repertoire and functions occurring in response to early interaction with HIV-infected DC, using an autologous in vitro NK/DC coculture system. We show that NK cell interaction with HIV-1-infected autologous monocyte-derived DC (MDDC) modulates NK receptor expression. In particular, expression of the CD85j receptor on NK cells was strongly down-regulated upon coculture with HIV-1-infected MDDC. We demonstrate that CD85j(+) NK cells exert potent control of HIV-1 replication in single-round and productively HIV-1-infected MDDC, whereas CD85j(-) NK cells induce a modest and transient decrease of HIV-1 replication. HIV-1 suppression in MDCC by CD85j(+) NK cells required cell-to-cell contact and did not appear mediated by cytotoxicity or by soluble factors. HIV-1 inhibition was abolished when NK-MDDC interaction through the CD85j receptor was blocked with a recombinant CD85j molecule, whereas inhibition was only slightly counteracted by blocking HLA class I molecules, which are known CD85j ligands. After masking HLA class I molecules with specific antibodies, a fraction of HIV-1 infected MDDC was still strongly stained by a recombinant CD85j protein. These results suggest that CD85j(+) NK cell inhibition of HIV-1 replication in MDDC is mainly mediated by CD85j interaction with an unknown ligand (distinct from HLA class I molecules) preferentially expressed on HIV-1-infected MDDC.

Published

2008