Kinetics of long‐term (72 hr) calcium content during mitogen activation of cultured human T lymphocytes

Abstract

In vitro stimulation of human blood lymphocytes with mitogen resulted in an increased intracellular content of Ca²⁺ per unit cell volume. This increase in Ca²⁺ content of lectin‐activated cells reached a maximum after 24 hr of culture and thereafter slowly declined. Brief treatment of cells at 24 hr of culture with the Ca²⁺ ionophore A23187 in combination with EGTA resulted in a larger release of Ca²⁺ from cells in mitogen‐stimulated cultures than from cells in control cultures. This indicates that the Ca²⁺ is accumulated intracellularly but is readily exchangeable. At 24 hr of culture the increase in cellular Ca²⁺ correlated well with the proliferative response as measured by ³H‐thymidine incorporation. Ca²⁺ influx at 24 and 48 hr of culture was markedly enhanced in the mitogenically stimulated cells as compared either to cells cultured for 1 and 72 hr or cells cultured without mitogen.