The Molecular Mechanisms of T Cell Clonal Anergy: A Dissertation
| dc.contributor.advisor | Aldo A. Rossini | |
| dc.contributor.author | Harris, John E. | |
| dc.date | 2022-08-11T08:08:43.000 | |
| dc.date.accessioned | 2022-08-23T16:05:48Z | |
| dc.date.available | 2022-08-23T16:05:48Z | |
| dc.date.issued | 2003-06-23 | |
| dc.date.submitted | 2006-06-02 | |
| dc.identifier.doi | 10.13028/4ag7-4w77 | |
| dc.identifier.uri | http://hdl.handle.net/20.500.14038/31945 | |
| dc.description.abstract | A side effect of generating an immune system for defense against invading pathogens is the potential to develop destructive cells that recognize self-tissues. Typically, through the "education" of developing immune cells, the organism inactivates potentially self-destructive cells, resulting in what is called self-tolerance. I proposed to explore the molecular mechanisms responsible for the induction and maintenance of tolerance. Our lab has developed a model of induced immune tolerance to skin and islet allografts utilizing a donor-specific transfusion of spleen cells and a brief course of anti-CD40L antibody. Because the difficulty in isolation of tolerant T cells from this system is prohibitive to performing large screens on these cells directly, I have chosen to study an in vitro CD4+Th1 cell line, A.E7, which can be made anergic via stimulation through the T cell receptor in the absence of costimulation. I hypothesized that anergized T cells upregulate genes that are responsible for the induction and maintenance of anergy and therefore exhibit a unique RNA expression profile. I have screened anergic cells using Affymetrix GeneChips and identified a small number of genes that are differentially expressed long-term in the anergic population compared to mock-stimulated and productively activated controls. The results have been confirmed by quantitative RT-PCR for each of the candidates. One of the most promising, the zinc-finger transcription factor Egr-2, was verified to be expressed long-term by western blotting, demonstrating perfect correlation between Egr-2 protein expression and the anergic phenotype. Silencing Egr-2 gene expression by siRNA in A.E7 T cells prior to anergy induction rescues the cells from the inability to phosphorylate ERK-1 and ERK-2 and also results in increased proliferation in response to antigen rechallenge. In this study I report that Egr-2 is specifically expressed long-term in anergic cells, protein expression correlates inversely with responsiveness to antigen rechallenge, and that Egr-2 is required for the full induction of anergy in T cell clones. | |
| dc.language.iso | en_US | |
| dc.rights | Copyright is held by the author, with all rights reserved. | |
| dc.subject | CD4-Positive T-Lymphocytes | |
| dc.subject | Clonal Anergy | |
| dc.subject | Self Tolerance | |
| dc.subject | T-Lymphocytes | |
| dc.subject | Transcription Factors | |
| dc.subject | Zinc Fingers | |
| dc.subject | Cells | |
| dc.subject | Immunology and Infectious Disease | |
| dc.subject | Tissues | |
| dc.title | The Molecular Mechanisms of T Cell Clonal Anergy: A Dissertation | |
| dc.type | Doctoral Dissertation | |
| dc.identifier.legacyfulltext | https://escholarship.umassmed.edu/cgi/viewcontent.cgi?article=1007&context=gsbs_diss&unstamped=1 | |
| dc.identifier.legacycoverpage | https://escholarship.umassmed.edu/gsbs_diss/6 | |
| dc.legacy.embargo | 2017-04-24T00:00:00-07:00 | |
| dc.identifier.contextkey | 171063 | |
| refterms.dateFOA | 2022-08-30T16:04:41Z | |
| html.description.abstract | <p>A side effect of generating an immune system for defense against invading pathogens is the potential to develop destructive cells that recognize self-tissues. Typically, through the "education" of developing immune cells, the organism inactivates potentially self-destructive cells, resulting in what is called self-tolerance. I proposed to explore the molecular mechanisms responsible for the induction and maintenance of tolerance. Our lab has developed a model of induced immune tolerance to skin and islet allografts utilizing a donor-specific transfusion of spleen cells and a brief course of anti-CD40L antibody. Because the difficulty in isolation of tolerant T cells from this system is prohibitive to performing large screens on these cells directly, I have chosen to study an in vitro CD4<sup>+</sup>Th1 cell line, A.E7, which can be made anergic via stimulation through the T cell receptor in the absence of costimulation. I hypothesized that anergized T cells upregulate genes that are responsible for the induction and maintenance of anergy and therefore exhibit a unique RNA expression profile. I have screened anergic cells using Affymetrix GeneChips and identified a small number of genes that are differentially expressed long-term in the anergic population compared to mock-stimulated and productively activated controls. The results have been confirmed by quantitative RT-PCR for each of the candidates. One of the most promising, the zinc-finger transcription factor Egr-2, was verified to be expressed long-term by western blotting, demonstrating perfect correlation between Egr-2 protein expression and the anergic phenotype. Silencing Egr-2 gene expression by siRNA in A.E7 T cells prior to anergy induction rescues the cells from the inability to phosphorylate ERK-1 and ERK-2 and also results in increased proliferation in response to antigen rechallenge. In this study I report that Egr-2 is specifically expressed long-term in anergic cells, protein expression correlates inversely with responsiveness to antigen rechallenge, and that Egr-2 is required for the full induction of anergy in T cell clones.</p> | |
| dc.identifier.submissionpath | gsbs_diss/6 | |
| dc.contributor.department | Molecular Medicine | |
| dc.description.thesisprogram | MD/PhD |
