We have explored the possibility that estrogens and progesterone could have different target uterine cell populations according to their cell cycle stage and localization in glands vs. lumen. Experiments were carried out in which rabbits were injected with [3H]thymidine for 3 days to label nuclei of dividing cells, then either 17 beta-estradiol, progesterone, or vehicle were administered. 17 beta-Estradiol induced a decrease in the percentage of cells with labeled nuclei or labeling index of either luminal or glandular epithelium. Since this steroid has been shown to have a significant proliferative effect on glands, the data suggest that its effect is exerted on unlabeled quiescent cells, which are then recruited into the cell cycle. Progesterone, on the other hand, was found to induce a significant increase in labeling index of both luminal and glandular epithelium. Therefore, it is concluded that dividing cells are a target for this hormone. Analysis of the number of nuclear grains according to cell location in luminal vs. glandular epithelia and the effect of hormone administration confirmed that each ovarian hormone acts on different target cell populations. Short and long term administration of estrogens resulted in a larger internal circumference of the uterus due to an increase in the number of luminal cells, whereas the number of glands and glandular cells per section did not appear to change. These findings, in combination with previous research, suggest that endometrial gland cells migrate towards the lumen and estrogen administration decreases the rate of cell loss in the luminal epithelium. The concept of cell migration is supported by experiments in which single administration of [3H]thymidine to rabbits was followed by determination at different times of the geographical distribution of cells with labeled nuclei. There was observed, as a function of time, a decrease in the number of labeled cells in the bottom of the glands with a concomitant increase in the same parameter in the upper part of the glands and luminal epithelia. Estradiol administration changed these kinetics.
[1]
L. Gerschenson,et al.
Inhibition of estrogen-induced proliferation of cultured rabbit uterine epithelial cells by a cell density-dependent factor produced by the same cells.
,
1981,
Journal of steroid biochemistry.
[2]
L. Gerschenson,et al.
Regulation of ciliogenesis and proliferation of uterine epithelium by 20 alpha-hydroxy-pregn-4-en-3-one administration and withdrawal in ovariectomized rabbits.
,
1981,
Biology of reproduction.
[3]
L. Gerschenson,et al.
Temporal relationship between rabbit uterine epithelium proliferation and uteroglobin production.
,
1981,
Biology of reproduction.
[4]
L. Gerschenson,et al.
Differential effects of estradiol-17 beta and progesterone on the proliferation of glandular and luminal cells of rabbit uterine epithelium.
,
1981,
Biology of reproduction.
[5]
P. Galand,et al.
REGENERATION OF UTERINE EPITHELIUM AFTER EXPERIMENTAL ABLATION IN THE RAT
,
1981,
Cell and tissue kinetics.
[6]
S. Glasser,et al.
Differential response of individual uterine cell types from immature rats treated with estradiol.
,
1980,
Endocrinology.
[7]
L. Gerschenson,et al.
Hormonal regulation of proliferation in two populations of rabbit endometrial cells in culture.
,
1979,
Life sciences.
[8]
F. Nogales,et al.
THE NORMAL MENSTRUAL CYCLE. CHRONOLOGY AND MECHANISM OF ENDOMETRIAL DESQUAMATION
,
1978,
Obstetrics and gynecology.
[9]
J. Gorski,et al.
Stimulatory and inhibitory effects of estrogen on uterine DNA synthesis.
,
1976,
Endocrinology.
[10]
J. Pollard,et al.
Oestriol, oestradiol-17beta and the proliferation and death of uterine cells.
,
1976,
The Journal of endocrinology.