Fig. 4.
Fig. 4. TCR-Ras-Erk signaling and agonist-induced IL-2 secretion in Jurkat T cells overexpressing RasGRP. / (A) Jurkat cells transformed with either the empty vector pBMGNeo (Neo) or the same vector containing full-length human RasGRP (GRP) were induced with 5.0 μmol/L CdCl2 for 24 hours, as indicated, then examined for RasGRP expression by immunoblotting using the H176 antibody. (B) Cells expressing BMGNeo or RasGRP were induced with CdCl2 for 24 hours then stimulated with either 50 ng/mL PMA for 10 minutes or 0.156 μg/mL OKT3 for various periods. Cells were then harvested, lysed, and assayed for Ras-GTP, phospho-Erk and total Erk. (C) Cells from the same cultures as in (A) were stimulated with various concentrations of OKT3 for 15 minutes at 37°C and then directly lysed in SDS sample buffer. The lysates were then probed for phospho-Erk. The bands representing phospho-Erk were quantified by densitometry and plotted versus the concentration of OKT3. Samples were also probed with an anti-Erk antibody to verify that similar amounts of total Erk protein were present (data not shown). (D) Cells were induced with CdCl2 as indicated for 24 hours then stimulated for 48 hours with the calcium ionophore A23187 (A, 0.5 μmol/L) and either PMA (24 nmol/L) or bryostatin-1 (Bryo, 10 nmol/L). IL-2 in the medium was then measured. Values are the average of quadruplicate samples, with the standard error of the mean indicated.

TCR-Ras-Erk signaling and agonist-induced IL-2 secretion in Jurkat T cells overexpressing RasGRP.

(A) Jurkat cells transformed with either the empty vector pBMGNeo (Neo) or the same vector containing full-length human RasGRP (GRP) were induced with 5.0 μmol/L CdCl2 for 24 hours, as indicated, then examined for RasGRP expression by immunoblotting using the H176 antibody. (B) Cells expressing BMGNeo or RasGRP were induced with CdCl2 for 24 hours then stimulated with either 50 ng/mL PMA for 10 minutes or 0.156 μg/mL OKT3 for various periods. Cells were then harvested, lysed, and assayed for Ras-GTP, phospho-Erk and total Erk. (C) Cells from the same cultures as in (A) were stimulated with various concentrations of OKT3 for 15 minutes at 37°C and then directly lysed in SDS sample buffer. The lysates were then probed for phospho-Erk. The bands representing phospho-Erk were quantified by densitometry and plotted versus the concentration of OKT3. Samples were also probed with an anti-Erk antibody to verify that similar amounts of total Erk protein were present (data not shown). (D) Cells were induced with CdCl2 as indicated for 24 hours then stimulated for 48 hours with the calcium ionophore A23187 (A, 0.5 μmol/L) and either PMA (24 nmol/L) or bryostatin-1 (Bryo, 10 nmol/L). IL-2 in the medium was then measured. Values are the average of quadruplicate samples, with the standard error of the mean indicated.

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