Effects of Erythropoietin on Neuronal Activity

Abstract

Recently, erythropoietin (EPO) receptors and synthesis of EPO have been identified in the brain. To clarify the effects of EPO on neuronal cells, we investigated the effects of EPO on Ca²⁺ uptake, intracellular Ca²⁺ concentration, membrane potential, cell survival, release and biosynthesis of dopamine, and nitric oxide (NO) production in differentiated PC12 cells, which possess EPO receptors. EPO (10^‐12‐10^‐10M) increased ⁴⁵Ca²⁺ uptake and intracellular Ca²⁺ concentration in PC12 cells in a dose‐related manner; these increases were inhibited by nicardipine (1 μM) or anti‐EPO antibody (1:100 dilution). EPO induced membrane depolarization in PC12 cells. After a 5‐day culture without serum and nerve growth factor (NGF), viable cell number decreased to 50% of that of the control cells cultured with serum and NGF. EPO (10^‐13‐10^‐10M) increased the number of viable cells cultured without serum and NGF; this increase was blunted by nicardipine or anti‐EPO antibody. Incubation with EPO (10^‐13‐10^‐10M) stimulated mitogen‐activated protein kinase activity in PC12 cells. EPO (10^‐13‐10^‐10M) increased dopamine release from PC12 cells and tyrosine hydroxylase activity; these increases were sensitive to nicardipine or anti‐EPO antibody. Following a 4‐h incubation with EPO (10^‐14‐10^‐10M), NO production was increased, which was blunted by nicardipine and anti‐EPO antibody. In contrast, maximal NO synthase activity was not changed by EPO. These results suggest that EPO stimulates neuronal function and viability via activation of Ca²⁺ channels.