Your search keyword '"David H. Margulies"' showing total 6 results

1. MHC‐restricted Ag85B‐specific CD8 + T cells are enhanced by recombinant BCG prime and DNA boost immunization in mice

Author

Satoshi Hayakawa, Jiansheng Jiang, Kazuhiro Matsuo, David H. Margulies, Mitsuo Honda, Lisa F. Boyd, Shihoko Komine-Aizawa, and Satoru Mizuno

Subjects

0301 basic medicine, biology, T cell, Immunology, biology.organism_classification, Major histocompatibility complex, Virology, Epitope, Mycobacterium tuberculosis, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, medicine.anatomical_structure, Immune system, Immunity, medicine, biology.protein, Immunology and Allergy, Cytotoxic T cell, CD8, 030215 immunology

Abstract

Despite efforts to develop effective treatments and vaccines, Mycobacterium tuberculosis (Mtb), particularly pulmonary Mtb, continues to provide major health challenges worldwide. To improve immunization against the persistent health challenge of Mtb infection, we have studied the CD8+ T cell response to Bacillus Calmette-Guerin (BCG) and recombinant BCG (rBCG) in mice. Here, we generated CD8+ T cells with an rBCG-based vaccine encoding the Ag85B protein of M. kansasii, termed rBCG-Mkan85B, followed by boosting with plasmid DNA expressing the Ag85B gene (DNA-Mkan85B). We identified two MHC-I (H2-Kd )-restricted epitopes that induce cross-reactive responses to Mtb and other related mycobacteria in both BALB/c (H2d ) and CB6F1 (H2b/d ) mice. The H2-Kd -restricted peptide epitopes elicited polyfunctional CD8+ T cell responses that were also highly cross-reactive with those of other proteins of the Ag85 complex. Tetramer staining indicated that the two H2-Kd -restricted epitopes elicit distinct CD8+ T cell populations, a result explained by the X-ray structure of the two peptide/H2-Kd complexes. These results suggest that rBCG-Mkan85B vector-based immunization and DNA-Mkan85B boost may enhance CD8+ T cell response to Mtb, and might help to overcome the limited effectiveness of the current BCG in eliciting tuberculosis immunity.

Published

2019

2. The cellular environment regulates in situ kinetics of T-cell receptor interaction with peptide major histocompatibility complex

Author

David H. Margulies, Baoyu Liu, Wei Chen, Cheng Zhu, Kannan Natarajan, and Zhenhai Li

Subjects

Immunology, Kinetics, T-cell receptor, hemic and immune systems, chemical and pharmacologic phenomena, Cellular Immunology, Biology, Major histocompatibility complex, Cell biology, law.invention, Antigen, law, Recombinant DNA, biology.protein, Immunology and Allergy, Surface plasmon resonance, Receptor

Abstract

T cells recognize antigens at the two-dimensional (2D) interface with antigen-presenting cells (APCs), which trigger T-cell effector functions. T-cell functional outcomes correlate with 2D kinetics of membrane-embedded T-cell receptors (TCRs) binding to surface-tethered peptide-major histocompatibility complex molecules (pMHCs). However, most studies have measured TCR-pMHC kinetics for recombinant TCRs in 3D by surface plasmon resonance, which differs drastically from 2D measurements. Here, we compared pMHC dissociation from native TCR on the T-cell surface to recombinant TCR immobilized on glass surface or in solution. Force on TCR-pMHC bonds regulated their lifetimes differently for native than recombinant TCRs. Perturbing the cellular environment suppressed 2D on-rates but had no effect on 2D off-rate regardless of whether force was applied. In contrast, for the TCR interacting with its monoclonal antibody, the 2D on-rate was insensitive to cellular perturbations and the force-dependent off-rates were indistinguishable for native and recombinant TCRs. These data present novel features of TCR-pMHC kinetics that are regulated by the cellular environment, underscoring the limitations of 3D kinetics in predicting T-cell functions and calling for further elucidation of the underlying molecular and cellular mechanisms that regulate 2D kinetics in physiological settings.

Published

2015

3. Availability of autoantigenic epitopes controls phenotype, severity, and penetrance in TCR Tg autoimmune gastritis

Author

Michael G. Mage, Lisa F. Boyd, Luc Teyton, Carine Brinster, Ditza Levin, Ethan M. Shevach, Kannan Natarajan, Maria Jamela Revilleza, Richard J. DiPaolo, and David H. Margulies

Subjects

CD4-Positive T-Lymphocytes, Autoimmune Gastritis, Immunology, Receptors, Antigen, T-Cell, Mice, Transgenic, chemical and pharmacologic phenomena, medicine.disease_cause, Major histocompatibility complex, Autoantigens, Article, Epitope, Autoimmune Diseases, Autoimmunity, Epitopes, Mice, Antigen, medicine, Animals, Immunology and Allergy, Avidity, Amino Acid Sequence, Cation Transport Proteins, Cells, Cultured, Cell Proliferation, Mice, Inbred BALB C, biology, T-cell receptor, Dendritic Cells, MHC restriction, Phenotype, Gastritis, biology.protein, Female, Lymph Nodes, Peptides

Abstract

We examined TCR:MHC/peptide interactions and in vivo epitope availability to explore the Th1- or Th2-like phenotype of autoimmune disease in two TCR Tg mouse models of autoimmune gastritis (AIG). The TCR of strains A23 and A51 recognize distinct IA(d)-restricted peptides from the gastric parietal cell H/K-ATPase. Both peptides form extremely stable MHC/peptide (MHC/p) complexes. All A23 animals develop a Th1-like aggressive, inflammatory AIG early in life, while A51 mice develop indolent Th2-like AIG at 6-8 wk with incomplete penetrance. A51 T cells were more sensitive than A23 to low doses of soluble antigen and to MHC/p complexes. Staining with IA(d)/peptide tetramers was only detectable on previously activated T cells from A51. Thus, despite inducing a milder AIG, the A51 TCR displays a higher avidity for its cognate IA(d)/peptide. Nonetheless, in vivo proliferation of adoptively transferred A51 CFSE-labeled T cells in the gastric lymph node was relatively poor compared with A23 T cells. Also, DC from WT gastric lymph node, presenting processed antigen available in vivo, stimulated proliferation of A23 T cells better than A51. Thus, the autoimmune potential of these TCR in their respective Tg lines is strongly influenced by the availability of the peptide epitope, rather than by differential avidity for their respective MHC/p complexes.

Published

2008

4. Activating CTL precursors to reveal CTL function without skewing the repertoire byin vitro expansion

Author

David H. Margulies, Jay A. Berzofsky, Jeffrey D. Ahlers, James T. Snyder, Rima Koka, Igor M. Belyakov, Josephine H. Cox, Richard Tse, James S. Gibbs, and Jian Wang

Subjects

medicine.drug_class, Repertoire, Immunology, T-cell receptor, hemic and immune systems, chemical and pharmacologic phenomena, Biology, Monoclonal antibody, Molecular biology, In vitro, CTL, In vivo, medicine, Immunology and Allergy, Ex vivo, CD8

Abstract

Detection of the functional CD8+ CTL response usually requires in vitro restimulation. The differences between the CD8+ CTL repertoire in freshly isolated precursor cells and CD8+ CTL after short-term in vitro expansion have been generally assumed to be minimal, but have never been defined experimentally. Using staining with P18-I10/H-2Dd tetramers and monoclonal antibodies (mAb) against Vβ, we show the surprising result that there was significant skewing of the CD8+ CTL repertoire after just 7 days of stimulation. In contrast, we found that overnight incubation of precursor cells with peptide allows the functional assessment of CD8+ CTL (which cannot be detected ex vivo from freshly isolatedcells) without changing the absolute number of antigen-specific CTL as measured by tetramer staining or the repertoire of TCR analyzed with mAb. This study affords a better understanding of the differences between the ex vivo and in vitro stimulated CTL repertoire, and provides an approach to reveal a more faithful representation of the functional in vivo CTL response without skewing of the repertoire of T cells detected.

Published

2001

5. A T cell receptor transgenic model of severe, spontaneous organ-specific autoimmunity

Author

Kannan Natarajan, Ethan M. Shevach, David H. Margulies, and Rebecca S. McHugh

Subjects

Genetically modified mouse, Autoimmune Gastritis, Transgene, Immunology, T-cell receptor, Clone (cell biology), Biology, medicine.disease_cause, Autoimmunity, Transgenic Model, Antigen, medicine, Immunology and Allergy

Abstract

The development of mouse models of human organ-specific autoimmune diseases has been hampered by the need to immunize mice with autoantigens in potent adjuvants. Even autoantigen-specific T cell receptor transgenic models of autoimmunity have proven to be complex as the transgenic mice frequently fail to develop disease spontaneously. We have isolated a CD4(+) T cell clone (TxA23)that recognizes the gastric parietal cell antigen, H/K ATPase alpha-chain(630-641), from a mouse with autoimmune gastritis that developed after thymectomy on day 3 of life. The T cell receptor alpha and beta genes from this clone were used to generate A23 transgenic mice. All A23 transgenic animals spontaneously developed severe autoimmune gastritis, and evidence of disease was detected as early as day 10 of life. Gastritis could be transferred to immunocompromised mice with a limited number of transgenic thymocytes (10(3)), but as many as 10(7) induced only mild disease in wild-type animals. Due to the complete penetrance of spontaneous disease, identity of the auto-antigen, susceptibility to immunoregulation, and close relation to autoimmune gastritis in man, A23 transgenic mice represent a unique CD4(+) T cell-mediated disease model for understanding the multiple factors regulating organ-specific autoimmunity.

Published

2001

6. Post-thymectomy autoimmune gastritis: fine specificity and pathogenicity of anti-H/K ATPase- reactive T cells

Author

David H. Margulies, Kannan Natarajan, Anna Z. Amar, Ethan M. Shevach, Elisabeth Suri-Payer, and Rebecca S. McHugh

Subjects

medicine.medical_specialty, education.field_of_study, biology, Regulatory T cell, ATPase, Immunology, Population, Spleen, medicine.disease_cause, medicine.disease, Molecular biology, Autoimmunity, Cellular infiltration, medicine.anatomical_structure, Endocrinology, Cell culture, Internal medicine, medicine, biology.protein, Immunology and Allergy, IL-2 receptor, education

Abstract

and I-A d restricted, and recognize distinct peptides from the H/K ATPase chain. One cell line secretes Th1 and the other Th2 cytokines, but both are equally potent in inducing gastri- tis with distinct profiles of cellular infiltration in nu/nu recipient animals. Neither of the cell lines induced disease in normal BALB/c recipients and transfer of disease to nu/nu recipi- ents was blocked by co-transfer of normal BALB/c spleen cells containing CD4 + CD25 + cells. Although CD4 + CD25 + T cells are thought to emigrate from the thymus after day 3 of life, they could be identified in LN of 2-day-old animals. The capacity of CD4 + CD25 + Tc ells to abro- gate the pathogenic activity in vivo of both activated Th1/Th2 lines strongly suggests that this suppressor T cell population may have a therapeutic role in other models of established autoimmunity. The availability of well-characterized lines of autoantigen-specific T cells should greatly facilitate the analysis of the mechanism of action and target of the CD4 + CD25 + immunoregulatory cells.

Published

1999