The Role of JNK, ERK and p38 Mitogen Activated Protein Kinases in the Response of Jurkat T Cells as a Model for T Cell Activation

Authors

  • Eduardo Parra Laboratory of Experimental Biomedicine, School of Medicine, FACSAL, University of Tarapacá, Avenida Senador Luis Valente Rossi, Arica, Chile.
  • Pedro Hecht Laboratory of Experimental Biomedicine, School of Medicine, FACSAL, University of Tarapacá, Avenida Senador Luis Valente Rossi, Arica, Chile.

DOI:

https://doi.org/10.9734/bpi/rdmmr/v10/9770D

Keywords:

CD28 response element, Staphylococcal Enterotoxin A-E, Extracellular signal regulated kinase, c-Jun N-terminal kinase, Interleukin-2

Abstract

Activation of T lymphocytes requires at least two distinct signals for full cellular response. Signal one involves the engagement of the T cell receptor (TCR) by antigen specific peptide-MHC complexes.  The signal two is provided by the interaction of costimulatory molecules on the antigen presenting cells (APC) and the corresponding counter receptors on the T cells. In this way, to mimic the two-signal requirements for T cell activation mediated by ligands, we exposed the superantigens SEA or SEE (signal 1) to T cells incubated with HLA-DR/LFA-3 or HLA-DR/B7-1-CHO transfected cells (signal 2). LFA-3 costimulation was able to induce T cell proliferation as well as IFN-\(\gamma\) and IL-4 production at similar levels as in cells induced by B7-1. Analysis of the CD28RE of the IL-2 promoter showed specific transcription factor recruitment at the CD28RE element upon induction by B7 1/SEE. Further functional studies with an IL-2 enhancer-promoter carrying either wild type or mutated versions of the CD28RE site revealed that this element is necessary for full activation upon B7-1 costimulation. While both CD28/B7-1 and CD2/LFA-3 costimulation resulted in the up-regulation of IL-4 and IFN-\(\gamma\) promoters, IL-2 promoter activity and production of IL-2 were only seen after B7-1 costimulation. However, contrary to what has been previously proposed, we show that costimulation with either B7-1 or LFA-3 further enhanced the ERK-2 activity and strongly activated the p38 MAPK pathway, but only B7-1 costimulation induced high levels of JNK-1 activity. These data suggest that the differential effect of CD28 vs. CD2 can be related to the difference in the ability of the two pathways to induce JNK-1 activity.

Published

2021-10-30

How to Cite

Eduardo Parra, & Pedro Hecht. (2021). The Role of JNK, ERK and p38 Mitogen Activated Protein Kinases in the Response of Jurkat T Cells as a Model for T Cell Activation. Recent Developments in Medicine and Medical Research Vol. 10, 1–14. https://doi.org/10.9734/bpi/rdmmr/v10/9770D