Abstract
Epidermal growth factor (EGF) at nanomolar concentrations stimulated DNA synthesis in confluent, serum‐starved cultures of calf aorta and human uterine smooth muscle cells. Stimulation of DNA synthesis in lens epithelial cells was studied for comparison. L and D‐ascorbic acid potentiated the effect of serum and EGF on DNA synthesis in calf aorta cells. In contrast L‐ascorbic acid had minimal potentiating effect with serum and no effect with EFG present along with serum on DNA synthesis in human uterine smooth muscle and rabbit lens epithelial cells. EGF and ascorbic acid increased cell number when added to stationary phase cultures. Specific binding of ^125^I‐labelled EGF to smooth muscle cells was demonstrated. Receptor concentration in calf‐aorta smooth muscle cells was higher in dense cultures compared to sparse cultures. The time course of binding and dissociation of ^125^I‐labelled EGF was similar in “dense” and “sparse” cultures.
Human uterine smooth muscle cells in culture exhibited a finite lifespan. There was no stimulation of DNA synthesis in response to serum and EGF in cells of high population doubling level (PDL); although ^125^I‐labeled EGF binding was higher in old cells (high PDL) compared to young cells (low PDL). This increase in binding was shown to be due to changes in the concentration of receptors without changes in their affinity for EGF.