Title of article
Kinetics of expression and subset distribution of the TNF superfamily members CD40 ligand and Fas ligand on T lymphocytes in cattle
Author/Authors
Hirano، نويسنده , , Ayumi and Brown، نويسنده , , Wendy C and Trigona، نويسنده , , Wendy and Tuo، نويسنده , , Wenbin and Estes، نويسنده , , D.Mark، نويسنده ,
Issue Information
سالنامه با شماره پیاپی سال 1998
Pages
13
From page
251
To page
263
Abstract
CD40 and Fas are members of the tumor necrosis factor receptor (TNFR) superfamily. CD40 and Fas play key roles in T cell–B cell interactions. Cross linkage of these molecules induces cell activation and cell death, respectively. The interaction of CD40 with its ligand (CD40L), which is expressed on activated T cells, plays a pivotal role in the generation of the T-dependent (TD) immune response, and FasL-bearing T cells, which have been shown to be predominantly of either the TH0 or TH1 type, have the potential to induce the apoptotic death of Fas expressing B cells. We investigated bovine CD40L mRNA expression in established T cell clones by RT-PCR and Southern blotting. T cells analyzed included CD4+ TH0 and TH1 cell subpopulations, CD8+, and γ/δ T cells stimulated with either specific antigen or Con A. All CD4+ clones but not all CD8+ or γ/δ T cell receptor (TCR)-bearing clones expressed mRNA for CD40L. To determine the activation requirements for CD40L expression in cattle, we examined the kinetics and induction requirements for CD40L transcription in peripheral blood T cells using a phorbol ester and/or ionomycin, immobilized mouse anti-bovine CD3, or Con A. Our results demonstrate that CD40L mRNA appears relatively early after activation (1 h) and peaks at 2–4 h poststimulation. A rise in intracellular calcium concentration mediated by ionomycin treatment alone was sufficient to induce CD40L mRNA expression at relatively high levels. Ionomycin treatment in combination with other agonists (anti-CD3, PMA) did not enhance CD40L mRNA expression above levels obtained with ionomycin alone. The bovine Fas ligand gene was partially cloned and mRNA expression determined by RT-PCR in a panel of T cell clones. Our results demonstrate that TH0 and TH1 bovine T cell clones expressed Fas ligand transcripts although only one γ/δ T cell clone did. This expression was upregulated within 3 h after mitogen stimulation and reduced by 24 h.
Keywords
Bovine CD40 ligand , Bovine Fas ligand , TNF superfamily , Kinetics , T cell subsets , T cell clones
Journal title
Veterinary Immunology and Immunopathology
Serial Year
1998
Journal title
Veterinary Immunology and Immunopathology
Record number
2160720
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