30 results on '"Strom, A. B."'
Search Results
2. External Validation of the Identification of Need for Ultrasound Enhancing Agent Study (the IN-USE Study)
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Lehenbauer, Kyle R., Kennedy, Kevin, Fraiche, Ariane M., Strom, Jordan B., and Main, Michael L.
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Echocardiography ,Humans ,Radiology, Nuclear Medicine and imaging ,Cardiology and Cardiovascular Medicine ,Article ,Ultrasonography - Published
- 2022
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3. Comparability of Event Adjudication Versus Administrative Billing Claims for Outcome Ascertainment in the Dual Antiplatelet Therapy (DAPT) Study: Findings from the EXTEND-DAPT Study
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Faridi, Kamil F., Tamez, Hector, Butala, Neel M., Song, Yang, Shen, Changyu, Secemsky, Eric A., Mauri, Laura, Curtis, Jeptha P., Strom, Jordan B., and Yeh, Robert W.
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Male ,Stroke ,Percutaneous Coronary Intervention ,Treatment Outcome ,Myocardial Infarction ,Humans ,Drug Therapy, Combination ,Female ,Medicare ,Article ,Platelet Aggregation Inhibitors ,United States ,Aged - Abstract
BACKGROUND: Data from administrative claims may provide an efficient alternative for endpoint ascertainment in clinical trials. However, it is uncertain how well claims data compares to adjudication by a clinical events committee in trials of patients with cardiovascular disease. METHODS: We matched 1,336 patients ≥65 years old who received percutaneous coronary intervention in the Dual Antiplatelet Therapy (DAPT) Study with the National Cardiovascular Data Registry (NCDR) CathPCI Registry linked to Medicare claims as part of the Extending Trial-Based Evaluations of Medical Therapies Using Novel Sources of Data (EXTEND) Study. Adjudicated trial endpoints were compared to Medicare claims data with ICD-9 codes from inpatient hospitalizations using time-to-event analyses, sensitivity, specificity, positive predictive value (PPV), negative predictive value (NPV), and kappa statistics. RESULTS: At 21-month follow-up, the cumulative incidence of major adverse cardiovascular and cerebrovascular events (combined mortality, myocardial infarction [MI], and stroke) was similar between trial-adjudicated events and claims data (7.9% vs. 7.2%, respectively; p = 0.50). Bleeding rates were lower using adjudicated events compared with claims (5.0% vs. 8.6%, respectively; p
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- 2021
4. Applicability of Transcatheter Aortic Valve Replacement Trials to Real-World Clinical Practice: Findings From EXTEND-CoreValve
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Butala, Neel M, Secemsky, Eric, Kazi, Dhruv S, Song, Yang, Strom, Jordan B, Faridi, Kamil F, Brennan, J Matthew, Elmariah, Sammy, Shen, Changyu, and Yeh, Robert W
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Heart Valve Prosthesis Implantation ,Transplantation ,Aging ,Clinical Trials and Supportive Activities ,real world ,Aortic Valve Stenosis ,TAVR ,Cardiorespiratory Medicine and Haematology ,Cardiovascular ,Medicare ,Article ,United States ,Transcatheter Aortic Valve Replacement ,Heart Disease ,Treatment Outcome ,Cardiovascular System & Hematology ,Clinical Research ,Risk Factors ,Aortic Valve ,Humans ,Patient Safety ,generalizability ,Aged - Abstract
ObjectivesThe aim of this study was to examine the applicability of pivotal transcatheter aortic valve replacement (TAVR) trials to the real-world population of Medicare patients undergoing TAVR.BackgroundIt is unclear whether randomized controlled trial results of novel cardiovascular devices apply to patients encountered in clinical practice.MethodsCharacteristics of patients enrolled in the U.S. CoreValve pivotal trials were compared with those of the population of Medicare beneficiaries who underwent TAVR in U.S. clinical practice between November 2, 2011, and December 31, 2017. Inverse probability weighting was used to reweight the trial cohort on the basis of Medicare patient characteristics, and a "real-world" treatment effect was estimated.ResultsA total of 2,026 patients underwent TAVR in the U.S. CoreValve pivotal trials, and 135,112 patients underwent TAVR in the Medicare cohort. Trial patients were mostly similar to real-world patients at baseline, though trial patients were more likely to have hypertension (50% vs 39%) and coagulopathy (25% vs 17%), whereas real-world patients were more likely to have congestive heart failure (75% vs 68%) and frailty. The estimated real-world treatment effect of TAVR was an 11.4% absolute reduction in death or stroke (95% CI: 7.50%-14.92%) and an 8.7% absolute reduction in death (95% CI: 5.20%-12.32%) at 1 year with TAVR compared with conventional therapy (surgical aortic valve replacement for intermediate- and high-risk patients and medical therapy for extreme-risk patients).ConclusionsThe trial and real-world populations were mostly similar, with some notable differences. Nevertheless, the extrapolated real-world treatment effect was at least as high as the observed trial treatment effect, suggesting that the absolute benefit of TAVR in clinical trials is similar to the benefit of TAVR in the U.S. real-world setting.
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- 2020
5. Distinct mechanisms for the induction and maintenance of allograft tolerance with CTLA4-Fc treatment
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Tran, H. M., Peter Nickerson, Restifo, A. C., Ivis-Woodward, M. A., Patel, A., Allen, R. D., Strom, T. B., and O Connell, P. J.
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Immunology ,Immunology and Allergy - Abstract
A murine CTLA4/Fc gamma2a heavy chain (mCTLA4-Fc) chimeric fusion molecule was used in B6AF1 recipients of BALB/c pancreatic islet allografts to study the induction and maintenance of tolerance following inhibition of the CD28-B7 pathway for T cell activation. Donor-specific tolerance was achieved by administering 100 microg of mCTLA4-Fc on alternate days for 14 days (8 total doses) or a single 500 microg dose of mCTLA4-Fc on day 2 after transplant. Tolerance was mediated by long-lived peripheral lymphocytes and showed features of organ and alloantigen specificity. Whereas tolerance could not be established in allograft recipients receiving simultaneous mCTLA4-Fc and rIL-2, previously tolerant animals did not reject their grafts when given IL-2, suggesting that the induction and maintenance phases of tolerance were distinct and separate. The maintenance of donor-specific tolerance was an active immunologic process that was CD4+ T cell dependent and could be adoptively transferred to naive lymphocytes, but could not be explained by apoptosis or deletion of alloreactive T cells. Although an IL-2-sensitive mechanism such as anergy may contribute toward the induction of tolerance, its maintenance involves active suppression.
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- 1997
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6. Type 2 helper T cell-type cytokines and the development of 'infectious' tolerance in rat cardiac allograft recipients
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Onodera, K., Hancock, W. W., Elmara Graser, Lehmann, M., Sayegh, M. H., Strom, T. B., Volk, H. -D, and Kupiec-Weglinski, J. W.
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Immunology ,Immunology and Allergy - Abstract
CD4-targeted therapy with a nondepleting RIB-5/2 mAb abrogates accelerated (< 36 h) rejection in presensitized LEW rats and results in permanent acceptance of LBNF1 cardiac allografts in conjunction with the features of infectious tolerance. This study examined the role and functional significance of the Th1 and Th2 cytokine network and systemic host allospecific Ab (allo-Ab) responses in the development of the infectious tolerance pathway in this model. Long term survival of cardiac transplants in rats treated with the tolerizing RIB-5/2 mAb regimen was accompanied by profound depression of Th1 (IL-2 and IFN-gamma) and Th2 (IL-4, IL-10) cytokines at the graft site, as shown by competitive template reverse transcription-PCR and immunohistochemistry. In contrast, the expression of Th2-type cytokines was selectively up-regulated after transfer of infectious tolerance by spleen cells into new generations of primary and secondary test recipients. Donor-specific circulating IgM allo-Ab responses were diminished throughout, and the switch from IgM to IgG allo-Ab was completely prevented in tolerant hosts, as shown by flow cytometry. The demonstration that treatment with cytolytic anti-CD4, but not anti-CD8, mAb recreated rejection of test cardiac allografts with simultaneous down-regulation of IL-4 mRNA/protein expression underlines the importance of this cytokine in the development of infectious tolerance. Hence, this report documents distinct cytokine elaboration patterns in animals tolerized by CD4-targeted therapy compared with those rendered tolerant by putative regulatory Th2-like cells. The mechanism of tolerance in anti-CD4 mAb-treated hosts appears distinct from that operating in the absence of mAb, when the tolerant state is being transferred in an infectious manner to new cohorts of test recipients.
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- 1997
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7. IL-2 knockout recipient mice reject islet cell allografts
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Steiger, J., Peter Nickerson, Steurer, W., Moscovitch-Lopatin, M., and Strom, T. B.
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Immunology ,Immunology and Allergy - Abstract
The IL-2 pathway is portrayed often as central to allograft rejection. To test this hypothesis, we studied IL-2-deficient mice as allograft recipients. IL-2 gene knockout (KO) mice reject islet allografts and demonstrate a classical mononuclear leukocytic infiltrate, containing CD4+ and CD8+ T cells, surrounding and invading the islet allografts. Moreover, allograft rejection in the IL-2 KO mouse is associated with intragraft expression of certain cytokine and CTL attack molecule genes (e.g. IFN-gamma, IL-4, IL-7, IL-10, and granzyme B). In separate experiments, IL-2 KO mice generated CTLs in response to in vivo challenge with allogeneic tumor cells. Although IL-2 KO mice reject allografts in vivo, spleen cells from immunologically naive IL-2 KO mice exhibit a diminished proliferative response to mitogens in vitro that could be restored largely by exogenous IL-2, IL-4, or IL-7. The paradoxical ability to execute graft rejection in vivo despite near absent T cell proliferative responses in vitro may result from the expression of IL-7 in vivo, but not in vitro. Con A-stimulated bulk spleen cell cultures derived from IL-2 KO mice were essentially devoid not only of IL-2 but also IL-7 gene transcripts. These data indicate that 1) IL-2 is not the sole T cell growth factor capable of supporting allograft rejection and 2) expression of IL-4, but not IL-2, during the allograft response does not lead inevitably to tolerance.
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- 1995
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8. Administration of noncytolytic IL-10/Fc in murine models of lipopolysaccharide-induced septic shock and allogeneic islet transplantation
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Xin Xiao Zheng, Steele, A. W., Peter Nickerson, Steurer, W., Steiger, J., and Strom, T. B.
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Immunology ,Immunology and Allergy - Abstract
Numerous studies have suggested the potential application of IL-10 as an anti-inflammatory and as an antirejection agent. Unfortunately, cytokines have short circulating t1/2 We developed a murine IL-10/Fc gamma 2a immunoligand that possesses the biologic functions of IL-10 and the long circulating t1/2 in vivo, characteristic of Igs. We mutated the Fc gamma 2a fragment to render the immunoligand ineffective in directing Ab-dependent cell-mediated cytotoxicity and complement-directed cytolysis (noncytolytic IL-10/Fc (IL-10/Fc2-)). In terms of IL-10 activity, IL-10/Fc2- was as effective as rIL-10 mole per mole in preventing lethal septic shock, but the immunoligand had a prolonged period of efficacy in accord with its extended circulating half-life. Contrary to expectations, IL-10/Fc2- treatment tended to accelerate the destruction of islet cell allografts and increase the levels of granzyme B gene expression in local draining lymph nodes. These data suggest that the enhanced cytotoxic activity of allograft-destroying CTLs may contribute to the accelerated allograft rejection. Finally, our studies suggest that a noncytolytic IL-10/Fc fusion protein provides a useful tool to study the biologic effects of IL-10 in vivo and may provide a useful agent for the prevention and treatment of septic shock.
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- 1995
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9. Effects of an Agonist IL-2/Fc Fusion Protein, A Mutant Antagonist IL-15Fc Fusion Protein and Sirolimus on Cardiac Allograft Survival in Non-Human Primates
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Millington, Timothy, Koulmanda, Maria, Ng, Choo, Boskovic, Svjetlan, Nadazdin, Ognjenka M., Benichou, Gilles, Zheng, Xin Xiao, Strom, Terry B., and Madsen, Joren C.
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CD4-Positive T-Lymphocytes ,Interleukin-15 ,Sirolimus ,Biopsy ,Myocardium ,Recombinant Fusion Proteins ,Graft Survival ,Interleukin-2 Receptor alpha Subunit ,Article ,Immunoglobulin Fc Fragments ,Macaca fascicularis ,Phenotype ,Models, Animal ,Animals ,Heart Transplantation ,Humans ,Interleukin-2 ,Transplantation, Homologous ,Immunosuppressive Agents - Abstract
To tilt the immunologic balance toward tolerance and away from rejection, non-human primate recipients of cardiac allografts were treated with interleukin (IL)-2/Fc, mutant (m) antagonist type mIL-15/Fc, and sirolimus.Heterotopic heart transplants were performed on 8 fully mismatched cynomolgus macaques. An untreated control recipient rejected its graft by post-operative Day 6. The remaining 7 animals received oral or intramuscular immunosuppression with sirolimus. A recipient treated with sirolimus alone rejected at the end of 28 days of immunosuppression. The remaining 6 monkeys also received IL-2/Fc and mIL-15/Fc intramuscularly until 28 days after transplant. One animal received a second 28-day course of fusion protein starting at Day 50. In these 6 animals, sirolimus was continued for 28 days (n = 4) or until protein levels were low (n = 2).In the 4 monkeys treated with a 28-day course of sirolimus and fusion proteins, mean graft survival was 51.5 days (range, 28-76 days). The animal receiving a second course of fusion protein rejected its graft on Day 177, despite detectable levels of the fusion proteins and sirolimus. The central memory, effector memory, and naïve CD4(+) and CD8(+) T-cell populations in the peripheral blood did not change significantly during fusion protein administration. A 2.5-fold expansion in CD4(+)CD25(+) lymphocytes occurred in recipients treated with fusion proteins and sirolimus that was not observed in the recipient treated with sirolimus alone.Although IL-2/Fc, mIL-15/Fc, and sirolimus administered in this manner permitted modest prolongation of graft survival and expansion of CD4(+)CD25(+) T cells, tolerance was not achieved.
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- 2012
10. Tim-1 Signaling Substitutes for Conventional Signal 1 and Requires Costimulation to Induce T Cell Proliferation1
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Mariat, Christophe, Degauque, Nicolas, Balasubramanian, Savithri, Kenny, James, DeKruyff, Rosemarie H., Umetsu, Dale T., Kuchroo, Vijay, Zheng, Xin Xiao, and Strom, Terry B.
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Mice, Knockout ,Cell Survival ,T-Lymphocytes ,Membrane Proteins ,Cell Differentiation ,Mice, Transgenic ,Dendritic Cells ,Ligands ,Lymphocyte Activation ,Article ,Coculture Techniques ,Clone Cells ,Mice, Inbred C57BL ,Mice ,Mice, Inbred DBA ,Animals ,Hepatitis A Virus Cellular Receptor 1 ,Cells, Cultured ,Cell Proliferation ,Signal Transduction - Abstract
Differentiation and clonal expansion of Ag-activated naive T cells play a pivotal role in the adaptive immune response. T cell Ig mucin (Tim) proteins influence the activation and differentiation of T cells. Tim-3 and Tim-2 clearly regulate Th1 and Th2 responses, respectively, but the precise influence of Tim-1 on T cell activation remains to be determined. We now show that Tim-1 stimulation in vivo and in vitro induces polyclonal activation of T cells despite absence of a conventional TCR-dependent signal 1. In this model, Tim-1-induced proliferation is dependent on strong signal 2 costimulation provided by mature dendritic cells. Ligation of Tim-1 upon CD4(+) T cells with an agonist anti-Tim-1 mAb elicits a rise in free cytosolic calcium, calcineurin-dependent nuclear translocation of NF-AT, and transcription of IL-2. Because Tim-4, the Tim-1 ligand, is expressed by mature dendritic cells, we propose that interaction between Tim-1(+) T cells and Tim-4(+) dendritic cells might ensure optimal stimulation of T cells, when TCR-derived signals originating within an inflamed environment are weak or waning.
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- 2009
11. Mechanisms Underlying Blockade of Allograft Acceptance by TLR Ligands1
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Porrett, Paige M., Yuan, Xueli, LaRosa, David F., Walsh, Patrick T., Yang, Jaeseok, Gao, Wenda, Li, Peiying, Zhang, Jidong, Ansari, Javeed M., Hancock, Wayne W., Sayegh, Mohamed H., Koulmanda, Maria, Strom, Terry B., and Turka, Laurence A.
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Graft Rejection ,Mice, Knockout ,Interleukin-6 ,Graft Survival ,Interleukin-17 ,Toll-Like Receptors ,Glycine ,hemic and immune systems ,chemical and pharmacologic phenomena ,Cell Differentiation ,Forkhead Transcription Factors ,Skin Transplantation ,T-Lymphocytes, Helper-Inducer ,T-Lymphocytes, Regulatory ,Article ,Immunity, Innate ,Mice ,surgical procedures, operative ,Animals ,Heart Transplantation ,Transplantation, Homologous ,Cells, Cultured ,Cell Proliferation - Abstract
Immune activation via TLRs is known to prevent transplantation tolerance in multiple animal models. To investigate the mechanisms underlying this barrier to tolerance induction, we used complementary murine models of skin and cardiac transplantation in which prolonged allograft acceptance is either spontaneous or pharmacologically induced with anti-CD154 mAb and rapamycin. In each model, we found that prolonged allograft survival requires the presence of natural CD4(+)Foxp3(+) T regulatory cells (Tregs), and that the TLR9 ligand CpG prevents graft acceptance both by interfering with natural Treg function and by promoting the differentiation of Th1 effector T cells in vivo. We further demonstrate that although Th17 cells differentiate from naive alloreactive T cells, these cells do not arise from natural Tregs in either CpG-treated or untreated graft recipients. Finally, we show that CpG impairs natural Treg suppressor capability and prevents Treg-dependent allograft acceptance in an IL-6-independent fashion. Our data therefore suggest that TLR signals do not prevent prolonged graft acceptance by directing natural Tregs into the Th17 lineage or by using other IL-6-dependent mechanisms. Instead, graft destruction results from the ability of CpG to drive Th1 differentiation and interfere with immunoregulation established by alloreactive natural CD4(+)Foxp3(+) Tregs.
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- 2008
12. Functional Th1 Cells Are Required for Surgical Adhesion Formation in a Murine Model1
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Tzianabos, Arthur O., Holsti, Matthew A., Zheng, Xin-Xiao, Stucchi, Arthur F., Kuchroo, Vijay K., Strom, Terry B., Glimcher, Laurie H., and Cruikshank, William W.
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Interleukin-16 ,Enzyme-Linked Immunosorbent Assay ,Tissue Adhesions ,Th1 Cells ,Article ,Disease Models, Animal ,Interferon-gamma ,Mice ,Postoperative Complications ,Animals ,Cytokines ,Receptors, Virus ,T-Box Domain Proteins ,Hepatitis A Virus Cellular Receptor 2 - Abstract
Tissue trauma in the peritoneal and pelvic cavities following surgery or bacterial infection results in adhesions that are a debilitating cause of intestinal obstruction, chronic pelvic pain, and infertility in women. We recently demonstrated that CD4(+) alphabeta T cells are essential for development of this process. Using a murine model of experimental adhesion formation, we now demonstrate that adhesion formation is characterized by the selective recruitment of Tim-3(+), CCR5(+), CXCR3(+), IFN-gamma(+) cells, indicating the presence of a Th1 phenotype. We further demonstrate that adhesion formation is critically dependent on the function of Th1 cells because mice genetically deficient for IFN-gamma, T-bet, or treated with Abs to the Th1-selective chemoattractant IL-16 show significantly less adhesion formation than wild-type mice. In addition, disrupting the interaction of the Th1-specific regulatory molecule Tim-3, with its ligand, significantly exacerbates adhesion formation. This enhanced response is associated with increases in the level of neutrophil-attracting chemokines KC and MIP-2, known to play a role in adhesiogenesis. These data demonstrate that the CD4(+) T cells orchestrating adhesion formation are of the Th1 phenotype and delineate the central role of T-bet, Tim-3, IFN-gamma, and IL-16 in mediating this pathogenic tissue response.
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- 2008
13. 'Tim-4 expressed on antigen-presenting cells induces T cell expansion and survival'
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Rodriguez-Manzanet, Roselynn, Meyers, Jennifer Hartt, Balasubramanian, Savithri, Slavik, Jacqueline, Kassam, Nasim, Dardalhon, Valerie, Greenfield, Edward A., Anderson, Ana C., Sobel, Raymond A., Hafler, David A., Strom, Terry B., and Kuchroo, Vijay K.
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Cell Survival ,T-Lymphocytes ,Antigen-Presenting Cells ,Membrane Proteins ,Cell Differentiation ,Article ,Antibodies ,Cell Line ,Rats ,Mice ,Cricetinae ,Animals ,Female ,Signal Transduction - Abstract
TIM (T-cell, immunoglobulin, mucin) proteins can regulate T cell immune responses. Tim-4 mRNA is not expressed in T cells, but exclusively in antigen-presenting cells. Tim-4 is a ligand for Tim-1 and Tim-4.Ig fusion protein was shown to either inhibit or expand T cells. However, the molecular basis for such opposite effects was not defined. By generating monoclonal antibodies, we show that expression of Tim-4 protein is restricted to CD11c+ and CD11b+ cells and is upregulated upon activation. We show that Tim-4 specifically phosphorylates Tim-1 and induces T cell expansion by enhancing cell division and reducing apoptosis. Tim-4 also induces the phosphorylation of signaling molecules LAT, Akt, and ERK1/2 in T cells. Tim-4, expressed on antigen-presenting cells, is a costimulatory molecule that promotes T cell expansion and survival by crosslinking Tim-1 on T cells.
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- 2008
14. Targeting the IL-15 Receptor with an Antagonist IL-15 Mutant/Fcγ2a Protein Blocks Delayed-Type Hypersensitivity1
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Kim, Yon Su, Maslinski, Wlodzimierz, Zheng, Xin Xiao, Stevens, A. Christopher, Li, Xian Chang, Tesch, Gregory H., Kelley, Vicki R., and Strom, Terry B.
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Interleukin-15 ,STAT3 Transcription Factor ,Mice, Inbred BALB C ,Receptors, Interleukin-15 ,Recombinant Fusion Proteins ,Receptors, IgG ,Receptors, Interleukin-2 ,Milk Proteins ,Article ,DNA-Binding Proteins ,Mice ,STAT5 Transcription Factor ,Trans-Activators ,Animals ,Humans ,Tyrosine ,Hypersensitivity, Delayed ,Phosphorylation ,Cell Division ,Half-Life - Abstract
Owing to shared receptor components, the biologic activities of IL-15 are similar to those of IL-2. However, the patterns of tissue expression of IL-2/IL-2R alpha and IL-15/IL-15R alpha differ. The development of agents targeting the receptor and signaling elements of IL-15 may provide a new perspective for treatment of diseases associated with expression of IL-15/IL-15R. We designed, genetically constructed, and expressed a receptor site-specific IL-15 antagonist by mutating glutamine residues within the C terminus of IL-15 to aspartic acid and genetically linked this mutant IL-15 to murine Fc gamma2a. These mutant IL-15 proteins specifically bind to the IL-15R, competitively inhibit IL-15-triggered cell proliferation, and do not activate the STAT-signaling pathway. Because the receptor site-specific antagonist IL-15 mutant/Fc gamma2a fusion proteins had a prolonged t(1/2) in vivo and the potential for destruction of IL-15R+ leukocytes, we examined the immunosuppressive activity of this agent. An IL-15 mutant/Fc gamma2a fusion protein markedly attenuated Ag-specific delayed-type hypersensitivity responses and decreased leukocyte infiltration within the delayed-type hypersensitivity sites. These findings suggest that 1) IL-15/IL-15R+ cells are crucial to these T cell-dependent immune responses, and 2) treatment with IL-15 mutant/Fc gamma2a protein may ameliorate T cell-dependent immune/inflammatory diseases.
- Published
- 1998
15. Cyclosporine therapy of rat heart allograft recipients and release of interleukins (IL 1, IL 2, IL 3): a role for IL 3 in graft tolerance?
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Mario Abbud-Filho, Kupiec-Weglinski, J. W., Araujo, J. L., Heidecke, C. D., Tilney, N. L., and Strom, T. B.
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Immunology ,Immunology and Allergy - Abstract
LEW rat recipients of (LEW X BN)F1 strain heterotopic cardiac transplants treated with cyclosporine A (CsA) (15 mg/kg/day intramuscularly, 7 days) retain grafts indefinitely despite drug withdrawal. Donor-specific suppressor T cells that are active in passive transfer experiments have been harvested from long-term CsA-treated hosts. Although CsA is known to inhibit in vitro cytokine release, the in vivo effects of the CsA on the lymphokine cascade are not known. We investigated the action of the drug upon spontaneous and mitogen-induced interleukin 1 (IL 1), interleukin 2 (IL 2), and interleukin 3 (IL 3) release by spleen cells obtained from the following groups of rats: 1) normal, i.e., untreated and ungrafted; 2) grafted, acutely rejecting; 3) grafted, actively treated; and 4) under CsA-induced state of "tolerance." The results demonstrate that in vivo CsA therapy inhibits monocyte (IL 1 release) as well as lymphocyte function (IL 2 and IL 3 release) only during the inductive phase (the 7 days of treatment). During the "tolerant" phase, mitogen (Con A and LPS)-induced release of interleukins was quantitatively similar to that noted in normal animals. In contrast, a remarkable increase in the spontaneous production of IL 3 was observed in the "tolerant" group. Because cytokine release is not inhibited in the "tolerant" state, our data strongly support the concept that maintenance of the state of unresponsiveness is governed by the emergence of suppressor cells. The correlation of increased spontaneous production of IL 3 during this period leads us to postulate that this interleukin may be implicated in the activation or clonal expansion of suppressor cells, and hence may play a role in graft tolerance.
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- 1984
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16. Routes to Transplant Tolerance versus Rejection The Role of Cytokines
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Walsh, Patrick T., Strom, Terry B., and Turka, Laurence A.
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Graft Rejection ,surgical procedures, operative ,Graft Survival ,Immune Tolerance ,Animals ,Cytokines ,Humans ,Article ,Signal Transduction - Abstract
The alloimmune response can be divided into specific junctures where critical decisions between tolerance and immunity are made which define the outcome of the transplant. At these “decision nodes” various cytokines direct alloresponsive T cells to develop either a proinflammatory response aimed at graft destruction or an immunoregulatory response facilitating graft acceptance. This review will focus on the role of these cytokines in influencing the progression of an alloimmune response leading ultimately to either allograft survival or rejection.
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17. Immunologic enhancement of rat renal allografts. III. Immunopathologic lesions and rejection in long-surviving passively enhanced grafts
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Abbas, A. K., Corson, J. M., Carpenter, C. B., Strom, T. B., Merrill, J. P., and Dammin, G. J.
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Graft Rejection ,Immunity, Cellular ,Kidney Cortex ,Kidney Glomerulus ,Fluorescent Antibody Technique ,Arteries ,Complement C3 ,Kidney ,Kidney Transplantation ,Blood Urea Nitrogen ,Rats ,Kidney Tubules ,Immunoglobulin G ,Animals ,Transplantation, Homologous ,Kidney Cortex Necrosis ,Atrophy ,Research Article - Abstract
Immunologic enhancement of renal allografts from (Lewis times Brown Norway) F1 to Lewis rats was achieved by administering a single dose of antidonor serum at the time of transplantation. A series of grafts functioning for 1 to 4 months after transplantation were examined by light and immunofluorescence microscopy to evaluate the long-term protective effects of the enhancing serum and to determine if previously unobserved lesions appeared in long survivors. Despite the absence of detectable circulating cytotoxic alloantibody, long-term allografts showed necrotizing glomerular and arterial lesions which resembled those seen in acutely rejecting grafts and were compatible with humoral rejection. Thus, in this model, there is a late decline in the ability of passive enhancement to inhibit humoral rejection. Long-term grafts also developed tubular lesions with deposition of immunoglobulin and complement on the tubular basement membranes (TBM). Anti-TBM antibodies were demonstrated in recipients' sera and found to be organ specific but not major histocompatibility antigen or species specific. This tubular lesion is therefore a unique form of allograft injury in which the immune response is directed against tissue antigen(s) which are distinct from the major histocompatibility antigens that induce rejection.
- Published
- 1975
18. Unmodified pancreatic islet allograft rejection results in the preferential expression of certain T cell activation transcripts
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O Connell, P. J., Pacheco-Silva, A., Peter Nickerson, Muggia, R. A., Bastos, M., Kelley, V. R., and Strom, T. B.
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Immunology ,Immunology and Allergy - Abstract
Polymerase chain reaction-assisted reverse transcription was used to study the temporal course of rejection in unmodified recipients of murine pancreatic islet cell allografts (DBA/2-->B6AF1) by using syngeneic tissues as controls. The histologic appearance of the grafts was analyzed in parallel. Preproinsulin and constant region of the TCR-beta chain transcripts were studied as markers of graft integrity and infiltrating T cell mass, respectively. The participation of certain cytokines and CTL were analyzed by the detection of IL-2, IFN-gamma, IL-4, and CTL-specific serine protease (granzyme B) transcripts. The time-related disappearance of intragraft preproinsulin transcripts correlated with graft destruction, whereas the intensity of intragraft TCR-beta chain transcript levels correlated with the magnitude of mononuclear leukocyte infiltration in allografts. In unmodified allografts, the magnitude of IL-2 and IFN-gamma intragraft mRNA levels correlated with the intense mononuclear leukocyte infiltrate found on histologic examination at day 8. Only after stable IL-2 gene transcription on day 8 does evidence of graft destruction become apparent, indicating that IL-2 gene activation is closely related to and probably required for expression of alloimmune cytopathic processes. In contrast, IL-4 transcripts were absent or detected in low copy number throughout this time course. Intragraft expression of granzyme B mRNA, a CTL-specific transcript, peaked from day 8 to day 12 in allografts compared with syngeneic grafts or normal tissue. In syngeneic grafts IL-2 and/or IL-4 mRNA was essentially not detected. Although IFN-gamma and granzyme B transcripts were detected in syngeneic grafts, after 4 days the levels of detected transcripts were far less than those noted in allografts. In vivo detection of intragraft IL-2 transcripts in the relative absence of detectable IL-4 transcripts strongly suggests IL-2-dependent immune effector mechanisms are associated with, and perhaps responsible, for allograft rejection. Apparently IL-4-dependent effector mechanisms are not necessary for allograft rejection.
19. The intragraft gene activation of markers reflecting T-cell-activation and -cytotoxicity analyzed by quantitative RT-PCR in renal transplantation
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Strehlau, J., Pavlakis, M., Llpman, M., Maslinski, W., Michael Shapiro, and Strom, T. B.
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Adult ,Cytotoxicity, Immunologic ,Graft Rejection ,Transcriptional Activation ,Biopsy ,T-Lymphocytes ,Lymphocyte Activation ,Kidney Transplantation ,Polymerase Chain Reaction ,Gene Expression Regulation ,Cytokines ,Humans ,RNA, Messenger ,Child ,Biomarkers ,T-Lymphocytes, Cytotoxic - Abstract
T-cell activation is the key event in the development of acute allograft rejection and precedes clinically apparent organ damage. We have performed competitive RT-PCR to quantify the intragraft gene expression for T-cell associated cytokines (IL-2, IL-4, IL-7, IL-15), CTLA4 and cytotoxic lymphocyte specific molecules to test their potential as rejection markers and to further elucidate mechanisms involved in graft rejection. RNA was isolated from snap-frozen portions of core biopsies obtained for the evaluation of graft dysfunction in 34 adults and 8 children. Reverse transcription derived cDNA was coamplified with a known amount of a competitor (a mutated target gene fragment) and normalized for the house keeping gene GAPDH. IL-2, the principal T-cell growth factor and IL-4 were not detectable in any biopsy at the time of histologically apparent rejection. Transcripts of the novel cytokine IL-15 were found in all dysfunctioning grafts and in two donor kidneys prior to reperfusion. CTLA-4, expressed in activated T-cells after costimulation by CD28 was uniformly present post transplantation, but not in the two donor kidneys. Transcripts for IL-7 (p0.001), IL-15 (p0.0005), CTLA4 (p = 0.04), granzyme B (p0.00015) and perforin (p0.0003) showed a significant correlation to acute rejection episodes. Heightened gene expression declined rapidly after initiation of rejection treatment. Fas-ligand mRNA gene expression was upregulated in both acute and chronic rejections. While this study shows that competitive RT-PCR is a reliable diagnostic tool to detect acute rejection in renal core biopsies, a future challenge will be to identify molecular markers of evolving rejections utilizing RT-PCR in sequential samples of fine needle aspirations, urine and blood.
20. Increased CD40 ligand gene expression during human renal and murine islet allograft rejection
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Zheng, X. X., Schachter, A. D., Vasconcellos, L., Strehlau, J., Tian, Y., Michael Shapiro, Harmon, W., and Strom, T. B.
21. A further analysis of primary cytomegalovirus disease prevention in renal transplant recipients with a cytomegalovirus immune globulin: Interim comparison of a randomized and an open-label trial
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David Snydman, Werner, B. G., Tilney, N. L., Kirkman, R. L., Milford, E. L., Cho, S. I., Bush Jr, H. L., Levey, A. S., Strom, T. B., Carpenter, C. B., Berardi, V. P., Levey, R. H., Harmon, W. E., Zimmerman Ii, C. E., Tenny, A., Heinze-Lacy, B., Shapiro, M. E., Steinman, T., and Logerfo, F.
22. Targeting the IL-15 receptor with an antagonist IL-15 mutant/Fcγ2a protein blocks delayed-type hypersensitivity
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Kim, Y. S., Maslinski, W., Zheng, X. X., Stevens, A. C., Li, X. C., Tesch, G. H., Kelley, V. R., and Strom, T. B.
23. Ex vivo coating of islet cell allografts with murine CTLA4/Fc promotes graft tolerance
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Steurer, W., Peter Nickerson, Steele, A. W., Steiger, J., Xin Xiao Zheng, and Strom, T. B.
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Immunology ,Immunology and Allergy - Abstract
To test the hypothesis that blockade of B7-triggered costimulation by donor cells could preclude allograft rejection, we coated crude islet allograft preparations in vitro for 1 h with a murine CTLA4/Fc fusion protein. Murine CTLA4/Fc blocks the proliferative response in primary mixed lymphocyte cultures (MLC) and Con A-stimulated murine spleen cell cultures by 85 to 95%. Responder cells from a primary MLC containing mCTLA4/Fc were hyporesponsive upon restimulation to the same stimulator cells in a secondary MLC lacking mCTLA4/Fc. Because of mutations in the Fc gamma RI and C'1q binding sites of the Fc portion of the murine CTLA4/Fc fusion protein, the molecule binds to, but does not target, cells for Ab-dependent cellular cytotoxicity or complement-directed cytolysis. Although systemic immunosuppression was not applied, 42% (10 of 24) of B6AF1 recipients of islet allografts pretreated with CTLA4/Fc were permanently engrafted. Further, 50% of hosts bearing functioning islet allografts more than 150 days post-transplant were formally proved to be tolerant to donor tissues. A persistent CD4+ and CD8+ T cell infiltrate surrounding, but not invading, islet grafts in tolerant hosts was discerned. In control experiments, 89% (8 of 9) of islet allografts coated with mIgG3, and 100% (n = 10) pretreated with media alone were rejected. Thus, we conclude that 1) B7-triggered costimulation by donor APCs is an important element of rejection, and 2) blockade of the B7 pathway by in vitro allograft manipulation is able to induce tolerance.
24. A Noncytolytic IL-10/Fc Fusion Protein Prevents Diabetes, Blocks Autoimmunity, and Promotes Suppressor Phenomena in NOD Mice
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Zheng, X. X., Steele, A. W., Hancock, W. W., Stevens, A. C., Peter Nickerson, Roy-Chaudhury, P., Tian, Y., and Strom, T. B.
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Immunology ,Immunology and Allergy - Abstract
We have been successful in our efforts to develop a long lived noncytolytic murine IL-10/Fc fusion protein. In the nonobese diabetic mouse (NOD) model, administration of IL-10/Fc from 5 to 25 wk of age completely prevented the occurrence of diabetes. Moreover, these mice remained disease-free long after cessation of IL-10/Fc therapy. Immunohistochemistry studies show that IL-10/Fc treatment inhibits expression of TNF-alpha, proinflammatory cytokine, as well as Th1-type cytokines, IL-2 and IFN-gamma, but promotes expression of IL-4 and IL-10, Th2-type cytokines, by islet-infiltrating leukocytes. In an adoptive transfer model of diabetes in NOD mice, we found that: 1) IL-10/Fc treated hosts bear leukocytes that block expression of diabetes and 2) these leukocytes persisted even 8 wk after cessation of IL-10/Fc treatment. The potent antidiabetogenic effects provided by IL-10/Fc in the NOD model, together with its apparent lack of systemic toxicity, are notable.
25. Use of cytomegalovirus immune globulin to prevent cytomegalovirus disease in renal-transplant recipients
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Snydman, D. R., Werner, B. G., Heinze-Lacey, B., Berardi, V. P., Tilney, L., Kirkman, R. L., Milford, E. L., Cho, S. I., Bush Jr, H. L., Levey, A. S., Strom, T. B., Carpenter, C. B., Levey, R. H., Harmon, W. E., Zimmerman Ii, C. E., Michael Shapiro, Steenman, T., Logerfo, F., Idelson, B., and Schroter, G. P. J.
26. CTLA4lg prevents lymphoproliferation and fatal multiorgan tissue destruction in CTLA-4-deficient mice
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Tivol, E. A., Boyd, S. D., Mckeon, S., Borriello, F., Peter Nickerson, Strom, T. B., and Sharpe, A. H.
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Immunology ,Immunology and Allergy - Abstract
Mice lacking CTLA-4 develop a fatal spontaneous lymphoproliferative disease with massive lymphocytic infiltrates and tissue destruction in many organs. CTLA-4-deficient (-/-) splenocytes and lymph node cells proliferate without added stimuli in vitro. We report here that CTLA4Ig treatment of CTLA-4 -/- mice prevents lymphoproliferation and fatal multiorgan tissue damage in vivo and proliferation of CTLA-4 -/- splenocytes and lymph node cells in vitro. Therefore, stimulation via CD28-B7 interactions appears necessary for CTLA-4 -/- T cell proliferation and the production of lymphoproliferative disease in vivo. When CTLA4Ig treatment is terminated, CTLA-4 -/- T cells become activated and lymphoproliferative disease develops. The lack of long term protective effects of CTLA4Ig treatment suggests that CTLA-4 is needed for the induction and or maintenance of tolerance.
27. Prolonged islet allograft acceptance in the absence of expression of interleukin-4
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Peter Nickerson, Zheng, X. X., Steiger, J., Steele, A. W., Steurer, W., Roy-Chaudhury, P., Müller, W., and Strom, T. B.
28. Leptin Modulation of Alloimmunity by Dendritic Cell Modulation of Regulatory T Cells and Th17 Cells Balance
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Pedro Vieira, Bassi, E. J., Larocca, R., Lepique, A. P., Quintana, F. J., Araujo, R., Basso, A. S., Strom, T. B., and Camara, N. O.
29. Expression of protective genes in human renal allografts: A regulatory response to injury associated with graft rejection
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Avihingsanon, Y., Ma, N., Csizmadia, E., Wang, C., Pavlakis, M., Giraldo, M., Strom, T. B., Miguel Soares, and Ferran, C.
30. IL-2 and IL-4 double knockout mice reject islet allografts: A role for novel T cell growth factors in allograft rejection
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Li, X. C., Roy-Chaudhury, P., Hancock, W. W., Manfro, R., Zand, M. S., Li, Y., Zheng, X. X., Peter Nickerson, Steiger, J., Malek, T. R., and Strom, T. B.
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