Abstract

ABSTRACT: Clinical observation of patients with congenital growth hormone (GH) deficiency and Laron‐type dwarfism suggests that factors such as GH or insulin‐like growth factor 1 (IGF‐1) might, in addition to androgens, be needed for normal phallic growth. We speculated GH or IGF‐1 might have direct actions on genital tissues and performed the present study to evaluate the in vitro effects of GH and IGF‐1 on cultured neonatal foreskin fibroblasts. Cells derived from foreskins of normal newborns were studied between cell passages 6 and 15. Serum‐free media with and without 100 ng/ml GH, IGF‐1, or both were added 24 hours prior to and at the time of study. To determine the activity of 5‐alpha‐reductase (5‐α‐R), 3 H‐testosterone (T; 2 nM) was added, and 5‐α‐R activity was calculated as femtomoles 3 H‐dihydrotestosterone and 3 H‐androstanediol produced/microgram DNA/hour. Androgen receptor (AR) binding was determined by the addition of 3 H‐dihydrotestosterone (dHT; 0.03125–0.5 nM) in the presence and absence of a 200‐fold excess of unlabeled dHT. Specific binding was used in Scatchard analysis for determination of AR number ( B max ) and binding affinity ( K d ). The rate of DNA synthesis was determined by incorporation of 3 H‐thymidine ( 3 H‐Thy) into trichloroacetic acid‐insoluble material. DNA and protein content were determined on cell lysates. IGF‐1, but not GH, had proliferative effects (significant increases in the rate of 3 H‐Thy incorporation, DNA, and protein content) but no effect on 5‐α‐R activity, B max or K d . This suggests that IGF‐1 has direct, in vitro , proliferative effects on genital tissue that are not mediated by changes in 5‐α‐R or AR.