Your search keyword '"Tussiwand, Roxane"' showing total 71 results

51. Batf3 maintains autoactivation of Irf8 for commitment of a CD8α+ conventional DC clonogenic progenitor.

Author

Grajales-Reyes, Gary E, Iwata, Arifumi, Albring, Jörn, Wu, Xiaodi, Tussiwand, Roxane, KC, Wumesh, Kretzer, Nicole M, Briseño, Carlos G, Durai, Vivek, Bagadia, Prachi, Haldar, Malay, Schönheit, Jörg, Rosenbauer, Frank, Murphy, Theresa L, and Murphy, Kenneth M

Subjects

INTERFERON regulatory factors, CD8 antigen, DENDRITIC cells, TRANSCRIPTION factors, LABORATORY mice, CD4 antigen

Abstract

The transcription factors Batf3 and IRF8 are required for the development of CD8α+ conventional dendritic cells (cDCs), but the basis for their actions has remained unclear. Here we identified two progenitor cells positive for the transcription factor Zbtb46 that separately generated CD8α+ cDCs and CD4+ cDCs and arose directly from the common DC progenitor (CDP). Irf8 expression in CDPs required prior autoactivation of Irf8 that was dependent on the transcription factor PU.1. Specification of the clonogenic progenitor of CD8α+ cDCs (the pre-CD8 DC) required IRF8 but not Batf3. However, after specification of pre-CD8 DCs, autoactivation of Irf8 became Batf3 dependent at a CD8α+ cDC-specific enhancer with multiple transcription factor AP1-IRF composite elements (AICEs) within the Irf8 superenhancer. CDPs from Batf3−/− mice that were specified toward development into pre-CD8 DCs failed to complete their development into CD8α+ cDCs due to decay of Irf8 autoactivation and diverted to the CD4+ cDC lineage. [ABSTRACT FROM AUTHOR]

Published

2015

52. Disseminated and sustained HIV-infection in CD34+ cord blood cell transplanted Rag2-/-gc-/- mice

Author

Baenziger, Stefan, primary, Tussiwand, Roxane, additional, Schlaepfer, Erika, additional, Mazzucchelli, Luca, additional, Heikenwalder, Mathias, additional, Kurrer, Michael O, additional, Behnke, Silvia, additional, Frey, Joachim, additional, Oxenius, Annette, additional, Joller, Helen, additional, Aguzzi, Adriano, additional, Manz, Markus G, additional, and Speck, Roberto F, additional

Published

2006

53. Disseminated and Sustained HIV-Infection in CD34+ Cord Blood Cell Transplanted Rag2−/−gc−/− Mice.

Author

Manz, Markus G., primary, Baenziger, Stefan, primary, Tussiwand, Roxane, primary, and Speck, Roberto F., primary

Published

2006

54. Disseminated and sustained HIV infection in CD34+cord blood cell-transplanted Rag2−/−γc−/−mice

Author

Baenziger, Stefan, primary, Tussiwand, Roxane, additional, Schlaepfer, Erika, additional, Mazzucchelli, Luca, additional, Heikenwalder, Mathias, additional, Kurrer, Michael O., additional, Behnke, Silvia, additional, Frey, Joachim, additional, Oxenius, Annette, additional, Joller, Helen, additional, Aguzzi, Adriano, additional, Manz, Markus G., additional, and Speck, Roberto F., additional

Published

2006

55. Activation of the Flt3 signal transduction cascade rescues and enhances type I interferon–producing and dendritic cell development

Author

Onai, Nobuyuki, primary, Obata-Onai, Aya, additional, Tussiwand, Roxane, additional, Lanzavecchia, Antonio, additional, and Manz, Markus G., additional

Published

2006

56. Constitutional Segmental Uniparental Disomy in a Twin Pair with t(12;21) Positive Acute Lymphoblastic Leukemia Characterized by the Same Prenatal Clone and Divergent Clonal Evolution.

Author

Cazzaniga, Giovanni, primary, Irving, Julie, additional, Citterio, Marco, additional, Bungaro, Silvia, additional, Tussiwand, Roxane, additional, Mura, Rossella, additional, Hall, Andrew G., additional, and Biondi, Andrea, additional

Published

2005

57. Enforced STAT3 and PU.1 Expression Activates Type I Interferon-Producing Cell and Dendritic Cell Differentiation Programs in Megakaryocyte/Erythrocyte Progenitors.

Author

Onai, Nobuyuki, primary, Onai, Aya, additional, Tussiwand, Roxane, additional, Lanzavecchia, Antonio, additional, and Manz, Markus G, additional

Published

2005

58. Inhibition of Natural Type I IFN-Producing and Dendritic Cell Development by a Small Molecule Receptor Tyrosine Kinase Inhibitor with Flt3 Affinity

Author

Tussiwand, Roxane, primary, Onai, Nobuyuki, additional, Mazzucchelli, Luca, additional, and Manz, Markus G., additional

Published

2005

59. Flt3 Receptor Expression Rescues Dendritic Cell Developmental Potential in Megakaryocyte/Erythrocyte Progenitor Cells.

Author

Onai, Nobuyuki, primary, Onai, Aya, additional, Tussiwand, Roxane, additional, Lanzavecchia, Antonio, additional, and Manz, Markus G., additional

Published

2004

60. Identification of preleukemic precursors of hyperdiploid acute lymphoblastic leukemia in cord blood

Author

Maia, Ana Teresa, primary, Tussiwand, Roxane, additional, Cazzaniga, Giovanni, additional, Rebulla, Paolo, additional, Colman, Susan, additional, Biondi, Andrea, additional, and Greaves, Mel, additional

Published

2004

61. Migratory CD103+ dendritic cells suppress helminth-driven type 2 immunity through constitutive expression of IL-12

Author

Everts, Bart, Tussiwand, Roxane, Dreesen, Leentje, Fairfax, Keke C., Huang, Stanley Ching-Cheng, Smith, Amber M., O’Neill, Christina M., Lam, Wing Y., Edelson, Brian T., Urban, Joseph F., Murphy, Kenneth M., and Pearce, Edward J.

Abstract

CD8α+ and CD103+ dendritic cells (DCs) play a central role in the development of type 1 immune responses. However, their role in type 2 immunity remains unclear. We examined this issue using Batf3−/− mice, in which both of these DC subsets are missing. We found that Th2 cell responses, and related events such as eosinophilia, alternative macrophage activation, and immunoglobulin class switching to IgG1, were enhanced in Batf3−/− mice responding to helminth parasites. This had beneficial or detrimental consequences depending on the context. For example, Batf3 deficiency converted a normally chronic intestinal infection with Heligmosomoides polygyrus into an infection that was rapidly controlled. However, liver fibrosis, an IL-13–mediated pathological consequence of wound healing in chronic schistosomiasis, was exacerbated in Batf3−/− mice infected with Schistosoma mansoni. Mechanistically, steady-state production of IL-12 by migratory CD103+ DCs, independent of signals from commensals or TLR-initiated events, was necessary and sufficient to exert the suppressive effects on Th2 response development. These findings identify a previously unrecognized role for migratory CD103+ DCs in antagonizing type 2 immune responses.

Published

2016

62. BAFF-R expression correlates with positive selection of immature B cells.

Author

Tussiwand, Roxane, Rauch, Melanie, Flück, Lukas A., and Rolink, Antonius G.

Abstract

The interaction between BAFF and BAFF-R is crucial for the development of mature B cells. Here, we report that the expression of BAFF-R is first detectable on a fraction of mouse CD19+ CD93+ IgM+ CD23- and human CD19+ CD10+ IgM+ BM B cells. This BAFF-R+ BM B-cell population shows higher levels of surface IgM expression and decreased RAG-2 transcripts than BAFF-R- immature B cells. When cultured, mouse BAFF-R-, but not BAFF-R+ immature B cells spontaneously undergo B-cell receptor editing. However, BAFF-R+ immature B cells cultured in the presence of an anti-κ light chain antibody are induced to undergo receptor editing. This receptor editing correlates with down-modulation of surface BAFF-R expression and the up-regulation of RAG-2 at the RNA level. B-cell receptor (BCR) cross-linking on splenic T1 B cells results in down-modulation of the BAFF-R, and receptor editing and RAG-2 up-regulation in a minor fraction of B cells. BCR cross-linking on splenic T2/3 B cells results in partly down and partly up-modulation of BAFF-R expression and no evidence for receptor editing. Overall, our data indicate that BAFF-R expression is tightly regulated during B-cell development in mouse and human and its expression is correlated with positive selection. [ABSTRACT FROM AUTHOR]

Published

2012

63. Disseminated and sustained HIV infection in CD34+ cord blood cell-transplanted Rag2-/-Yc-/-mice.

Author

Baenziger, Stefan, Tussiwand, Roxane, Schlaepfer, Erika, Mazzucchelli, Luca, Heikenwalder, Mathias, Kurrer, Michael O., Behnkem, Silvia, Frey, Joachim, Oxenius, Annette, Joller, Helen, Aguzzi, Adriano, Manz, Markus G., and Speck, Roberto F.

Subjects

*HIV infections, *HIV, *LEUCOCYTES, *THYMUS, *ENDOCRINE glands, *LABORATORY mice

Abstract

Because of species selectivity, HIV research is largely restricted to in vitro or clinical studies, both limited in their ability to rapidly assess new strategies to fight the virus. To prospectively study some aspects of HIV in vivo, immunodeficient mice, transplanted with either human peripheral blood leukocytes or human fetal tissues, have been developed. Although these are susceptible to HIV infection, xenoreactivity, and short infection spans, resource and ethical constraints, as well as biased I-IIV coreceptor tropic strain infection, pose substantial problems in their use. Rag2-/-γc-/- mice, transplanted as newborns with human CD34+ cells, were recently shown to develop human B, T, and dendritic cells, constituting lymphoid organs in situ. Here we tested these mice as a model system for HIV-1 infection. HIV RNA levels peaked to up to 2 × 106 copies per milliliter of plasma early after infection, and viremia was observed for up to 190 days, the longest time followed. A marked relative CD4+ T cell depletion in peripheral blood occurred in CXCR4-tropic strain-infected mice, whereas this was less pronounced in CCR5-tropic strain-infected animals. Thymus infection was almost exclusively observed in CXCR4-tropic strain-infected mice, whereas spleen and lymph node HIV infection occurred irrespective of coreceptor selectivity, consistent with respective coreceptor expression on human CD4+ T cells. Thus, this straightforward to generate and cost-effective in vivo model closely resembles HIV infection in man and therefore should be valuable to study virus-induced pathology and to rapidly evaluate new approaches aiming to prevent or treat HIV infection. [ABSTRACT FROM AUTHOR]

Published

2006

64. Human Adaptive Immune System Rag2-/-γc-/- Mice.

Author

CHICHA, LAURIE, TUSSIWAND, ROXANE, TRAGGIAI, ELISABETTA, MAZZUCCHELLI, LUCA, BRONZ, LUCIO, PIFFARETTI, JEAN‐CLAUDE, LANZAVECCHIA, ANTONIO, and MANZ, MARKUS G.

Subjects

IMMUNE system, PATHOGENIC microorganisms, HEMATOPOIETIC system, CORD blood, VACCINES, MICE

Abstract

Although many biologic principles are conserved in mice and humans, species-specific differences exist, for example, in susceptibility and response to pathogens, that often do not allow direct implementation of findings in experimental mice to humans. Research in humans, however, for ethical and practical reasons, is largely restricted to in vitro assays that lack components and the complexity of a living organism. To nevertheless study the human hematopoietic and immune system in vivo, xenotransplantation assays have been developed that substitute human components to small animals. Here, we summarize our recent findings that transplantation of human cord blood CD34+ cells to newborn Rag2-/-γc-/- mice leads to de novo development of major functional components of the human adaptive immune system. These human adaptive immune system Rag2-/-γc-/- (huAIS-RG) mice can now be used as a technically straightforward preclinical model to evaluate in vivo human adaptive immune system development as well as immune responses, for example, to vaccines or live infectious pathogens. [ABSTRACT FROM AUTHOR]

Published

2005

65. CD34+Cord Blood Cell-Transplanted Rag2−/−γc−/−Mice as a Model for Epstein-Barr Virus Infection

Author

Cocco, Mario, Bellan, Cristiana, Tussiwand, Roxane, Corti, Davide, Traggiai, Elisabetta, Lazzi, Stefano, Mannucci, Susanna, Bronz, Lucio, Palummo, Nazzareno, Ginanneschi, Chiara, Tosi, Piero, Lanzavecchia, Antonio, Manz, Markus G., and Leoncini, Lorenzo

Abstract

Recent studies suggest that Epstein-Barr virus (EBV) can infect naïve B cells, driving them to differentiate into resting memory B cells via the germinal center reaction. This hypothesis has been inferred from parallels with the biology of normal B cells but has never been proven experimentally. Rag2−/−γc−/−mice that were transplanted with human CD34+cord blood cells as newborns were recently shown to develop human B, T, and dendritic cells, constituting lymphoid organs in situ. Here we used this model to better define the strategy of EBV infection of human B cells in vivoand to compare this model system with different conditions of EBV infection in humans. Our results support the model of EBV persistence in vivoin cases that were characterized by follicular hyperplasia and a relatively normal CD4+and CD8+T-cell distribution. Intriguingly, in cases that were characterized by nodular and diffuse proliferation with a preponderance of CD8+T cells, similar to infectious mononucleosis, EBV still infects naïve B cells but also induces clonal expansion and ongoing somatic mutations without germinal center reactions. Our results reveal different strategies of EBV infection in B cells that possibly result from variations in the host immune response. Future experiments might allow understanding of the mechanisms responsible for persistent EBV infection and provide targets for more highly tailored therapeutic interventions.

Published

2008

66. Disseminated and Sustained HIV-Infection in CD34+ Cord Blood Cell Transplanted Rag2-/-gc-/- Mice.

Author

Manz, Markus G., Baenziger, Stefan, Tussiwand, Roxane, and Speck, Roberto F.

Abstract

HIV research has been hampered due to the lack of assessable animal models that mirror infection in humans. HIV is a human-specific virus, and consequently laboratory rodents as mice or rats are not susceptible to infection. Although non-human primates as chimpanzees can be infected, they do not develop HIV-associated immunodeficiency, while sooty mangabeys, rhesus macaques, and baboons are only susceptible to HIV related simian-immunodeficiency virus. Efforts to genetically engineer rodents to become HIV targets have largely failed; even if infection in vitro was achieved, HIV replication in vivo was limited or absent. Thus, substitute xeno-chimeric models have been developed by transplanting immunodeficient mice with either human peripheral blood leukocytes (hu-PBL-SCID), or pieces of human fetal tissues containing hematopoietic cells (SCID-hu). Both hu-PBL-SCID and SCID-hu mice sustain HIV infection and replication in vivo. However, in hu-PBL-SCID mice xeno-reactivity and successive loss of human leukocytes limit infection to a relatively short time frame. In SCID-hu mice, HIV infection can be observed for extended times; however, availability of transplantable human fetal organs is restricted for practical and ethical reasons, and HIV pathology in these mice is mainly limited to tissue implants. Given these limitations hu-PBL-SCID and SCID-hu mice did not fully match the demand for a small animal model that closely mirrors infection in humans. Recently, we found that injection of human cord blood CD34+ cells into newborn Rag2-/-gc-/- mice leads to development of human T, B, and dendritic cells, successive formation of primary and secondary lymphoid organs in situ, and some in vivo immune responses. We here tested these mice as a model system for in vivo HIV-1 infection. Mice with a PB CD45+ and CD4+ cell chimerism of 29.4±18.2% and 2.7±3.0%, respectively, were infected i.p. with either CCR5-tropic YU-2 (n=15), or CXCR4-tropic NL4–3 (n=19) HIV-strains at 10–28 weeks of age. Independent of viral strains used, HIV-RNA levels peaked two to six weeks after infection, with up to about 2x10E6 copies/ml plasma, while thereafter viremia mostly stabilized at lower levels, and was maintained for up to 190 (YU-2) and 120 (NL4–3) days, the longest time followed. A marked relative CD4+ T cell depletion in peripheral blood occurred in CXCR4-tropic strain infected mice, while this was less pronounced in CCR5-tropic strain infected animals. Thymus infection, as determined by p24 immunohistochemistry, was almost exclusively observed in CXCR4-tropic strain infected mice, while spleen and lymph node HIV infection occurred irrespective of co-receptor selectivity, consistent with respective co-receptor expression on human CD4+ T-cells. P24 expressing, and thus productively HIV infected non-T cells such as CD68+ macrophages were only occasionally detected as expected in a non-inflammatory in vivo setting. In summary, the here presented data establishes newborn human CD34+ cell transplanted Rag2-/-gc-/- mice as a new tool to study HIV infection and pathogenesis in vivo, closely resembling HIV infection in humans. This straight-forward to generate, cost-effective, ethically unproblematic, and easy to monitor new in vivo model should thus be valuable to study virus-induced pathology, as well as pharmacologic or genetic approaches aiming to prevent or treat HIV infection.

Published

2006

67. CD4 T cell diversification in the tissue

Author

Swarnalekha, Nivedya, De Libero, Gennaro, King, Carolyn, and Tussiwand, Roxane

Subjects

endocrine system

Abstract

Heterogeneity is the hallmark feature of CD4 T cells with the ability to differentiate into effector cells of various phenotypes and perform distinct function. This diversification that is essential for optimal response has not been described in the tissue. Using influenza as an infection model, we investigated long-lived antigen-specific CD4 T cells in the tissue. We identified a heterogeneous population of T resident memory cells (TRM) in the tissue, specifically, a T follicular helper-like subset we called T resident helper (TRH) that was previously not reported. Further characterization by single cell RNA sequencing analysis revealed that TRH possess a unique tissue-specific transcriptional signature distinct from lymphoid TFH and that they can be generated independently of lymphoid replenishment. Histological analysis showed that TRH cluster closely with B cells in inducible bronchus-associated lymphoid tissue (iBALT) and require continued BCL6 signaling for their localization. Interestingly, at very late time points, signals through cognate antigen presentation were dispensable for TRH maintenance and iBALT integrity. Upon heterologous challenge, TRH cells support local antibody production highlighting a previously unexplored function of TRM.

Published

2021

68. Dissecting the development of plasmacytoid dendritic cells

Author

Rodrigues, Patrick Fernandes, Zeller, Rolf, Tussiwand, Roxane, and King, Carolyn

Subjects

hemic and immune systems

Abstract

Plasmacytoid dendritic cells (pDCs) are an immune subset specialized in the production of Type I Interferons (IFNs). Conventional dendritic cells (cDCs) originate mostly from a common dendritic cell progenitor (CDP), whereas pDCs have been shown to develop from both CDPs as well as common lymphoid progenitors (CLPs). In contrast to the current literature, we here show that pDCs mostly differentiate from an IL-7R expressing lymphoid progenitor. IL-7R+ progenitors can be subdivided into three distinct subsets based on the expression of SiglecH and Ly6D: double negative (DN), Ly6D+ single positive (SP) and double positive (DP) progenitors. Each of these subsets identifies a specific developmental stage along the pDC lineage, where commitment by IL-7R+ progenitors is achieved upon expression of Ly6D and SiglecH (DP pre-pDCs). Further, RNA sequencing analysis of IL-7R+ lymphoid progenitor subsets revealed the transcriptional landscape of pDC development along the lymphoid branch, where high expression of the transcription factor IRF8 marks pDC commitment and anticipates the increase of TCF4 levels. The transcriptional signature of DP pre-pDCs correlates with the lineage potential assessed in vitro, in which DP pre-pDCs are fully committed to the pDC lineage. Moreover, single cell RNA sequencing on bone marrow and splenic pDCs revealed pDC heterogeneity in both tissues and further supported the dual origin of pDC from myeloid and lymphoid precursors. While all pDCs have the potential to secrete Type I IFNs and have high expression levels of pDC-specific transcript, only myeloid-derived pDCs share with cDCs the capacity to process and present antigen, suggesting that functional specification is directly linked to developmental origin.

Published

2019

69. Sexual dimorphism in skin immunity is mediated by an androgen-ILC2-dendritic cell axis.

Author

Chi L, Liu C, Gribonika I, Gschwend J, Corral D, Han SJ, Lim AI, Rivera CA, Link VM, Wells AC, Bouladoux N, Collins N, Lima-Junior DS, Enamorado M, Rehermann B, Laffont S, Guéry JC, Tussiwand R, Schneider C, and Belkaid Y

Subjects

Female, Male, Gonadal Steroid Hormones metabolism, Animals, Mice, Mice, Inbred C57BL, Microbiota, Androgens metabolism, Dendritic Cells immunology, Immunity, Innate, Lymphocytes immunology, Sex Characteristics, Skin immunology

Abstract

Males and females exhibit profound differences in immune responses and disease susceptibility. However, the factors responsible for sex differences in tissue immunity remain poorly understood. Here, we uncovered a dominant role for type 2 innate lymphoid cells (ILC2s) in shaping sexual immune dimorphism within the skin. Mechanistically, negative regulation of ILC2s by androgens leads to a reduction in dendritic cell accumulation and activation in males, along with reduced tissue immunity. Collectively, our results reveal a role for the androgen-ILC2-dendritic cell axis in controlling sexual immune dimorphism. Moreover, this work proposes that tissue immune set points are defined by the dual action of sex hormones and the microbiota, with sex hormones controlling the strength of local immunity and microbiota calibrating its tone.

Published

2024

70. CD34+ cord blood cell-transplanted Rag2-/- gamma(c)-/- mice as a model for Epstein-Barr virus infection.

Author

Cocco M, Bellan C, Tussiwand R, Corti D, Traggiai E, Lazzi S, Mannucci S, Bronz L, Palummo N, Ginanneschi C, Tosi P, Lanzavecchia A, Manz MG, and Leoncini L

Subjects

Animals, B-Lymphocytes virology, Blood Cell Count, Cell Proliferation, Clone Cells, DNA-Binding Proteins metabolism, Disease Models, Animal, Epstein-Barr Virus Infections immunology, Epstein-Barr Virus Nuclear Antigens metabolism, Humans, Immunophenotyping, Lasers, Lymphoid Tissue pathology, Lymphoid Tissue virology, Mice, Microdissection, Viral Proteins metabolism, Virus Latency genetics, Antigens, CD34 metabolism, Cord Blood Stem Cell Transplantation, DNA-Binding Proteins deficiency, Epstein-Barr Virus Infections pathology, Fetal Blood cytology, Fetal Blood transplantation, Immunoglobulin G genetics

Abstract

Recent studies suggest that Epstein-Barr virus (EBV) can infect naïve B cells, driving them to differentiate into resting memory B cells via the germinal center reaction. This hypothesis has been inferred from parallels with the biology of normal B cells but has never been proven experimentally. Rag2(-/-) gamma(c)(-/-) mice that were transplanted with human CD34(+) cord blood cells as newborns were recently shown to develop human B, T, and dendritic cells, constituting lymphoid organs in situ. Here we used this model to better define the strategy of EBV infection of human B cells in vivo and to compare this model system with different conditions of EBV infection in humans. Our results support the model of EBV persistence in vivo in cases that were characterized by follicular hyperplasia and a relatively normal CD4(+) and CD8(+) T-cell distribution. Intriguingly, in cases that were characterized by nodular and diffuse proliferation with a preponderance of CD8(+) T cells, similar to infectious mononucleosis, EBV still infects naïve B cells but also induces clonal expansion and ongoing somatic mutations without germinal center reactions. Our results reveal different strategies of EBV infection in B cells that possibly result from variations in the host immune response. Future experiments might allow understanding of the mechanisms responsible for persistent EBV infection and provide targets for more highly tailored therapeutic interventions.

Published

2008

71. Human adaptive immune system Rag2-/-gamma(c)-/- mice.

Author

Chicha L, Tussiwand R, Traggiai E, Mazzucchelli L, Bronz L, Piffaretti JC, Lanzavecchia A, and Manz MG

Subjects

Animals, Antigens, CD34 immunology, Cell Transplantation, Cystatin C, Cystatins deficiency, Cystatins genetics, DNA-Binding Proteins, Fetal Blood cytology, Humans, Infant, Newborn, Lymphocytes cytology, Lymphocytes immunology, Mice, Mice, Mutant Strains, Nuclear Proteins, Transplantation, Heterologous, Cystatins physiology, Immune System physiology

Abstract

Although many biologic principles are conserved in mice and humans, species-specific differences exist, for example, in susceptibility and response to pathogens, that often do not allow direct implementation of findings in experimental mice to humans. Research in humans, however, for ethical and practical reasons, is largely restricted to in vitro assays that lack components and the complexity of a living organism. To nevertheless study the human hematopoietic and immune system in vivo, xenotransplantation assays have been developed that substitute human components to small animals. Here, we summarize our recent findings that transplantation of human cord blood CD34(+) cells to newborn Rag2(-/-)gamma(c)(-/-) mice leads to de novo development of major functional components of the human adaptive immune system. These human adaptive immune system Rag2(-/-)gamma(c)(-/-) (huAIS-RG) mice can now be used as a technically straightforward preclinical model to evaluate in vivo human adaptive immune system development as well as immune responses, for example, to vaccines or live infectious pathogens.

Published

2005