Mechanism of estrogen action: indirect effect of estradiol-17 beta on proliferation of quail oviduct cells

Experimental data were collected to test whether the effect of estrogens required a direct action of the steroid on their target cells for induction of (i) cell multiplication and (ii) celltype-specific protein synthesis. Ovariectomized quails were perfused for 24 hr with several doses of estradiol-...

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Bibliographic Details
Published in:Proceedings of the National Academy of Sciences - PNAS 1983-03, Vol.80 (6), p.1621-1625
Main Authors: Laugier, Christian, Pageaux, Jean-Francois, Soto, Ana M., Sonnenschein, Carlos
Format: Article
Language:English
Subjects:
Animals
Biological Sciences: Cell Biology
Birds
Carrier Proteins - metabolism
Castration
Cell Division - drug effects
Cell growth
Cell Nucleus - metabolism
Coturnix
DNA
Endocrinology
Estradiol - administration & dosage
Estradiol - pharmacology
Estrogens
Female
Jugular vein
Liver
Liver - physiology
Oviducts
Oviducts - cytology
Oviducts - drug effects
Perfusion
Portal vein
Receptors, Estrogen
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Summary:Experimental data were collected to test whether the effect of estrogens required a direct action of the steroid on their target cells for induction of (i) cell multiplication and (ii) celltype-specific protein synthesis. Ovariectomized quails were perfused for 24 hr with several doses of estradiol-17β (E2) (0.05-6.8 ng/min) through either the jugular vein or the portal vein. E2plasma concentrations increased progressively when the perfusion rate through the jugular vein was 0.5 ng/min and higher. With the portal vein, by contrast, E2plasma concentrations increased over the concentration in unperfused ovariectomized animals only when the perfusion rate was above 2 ng/min. An increase in DNA concentration per oviduct was observed regardless of the route of administration and the rate of perfusion, starting at 0.5 ng/min. Nuclear estrophilins increased when E2was perfused through the jugular vein at rates of 0.5 ng/min or greater. This same parameter was not increased in oviducts of quail perfused through the portal vein even at a perfusion rate of 2.0 ng/min. Progestophilins were induced in the oviducts of quail perfused through the jugular vein at rates of 2 ng/min and above; on the other hand, progestophilins were induced in birds perfused through the portal vein at rates above 2 ng/min. Ovalbumin was not induced in quail oviducts at any rate and route of perfusion. The induction of the synthesis of cell-type-specific protein (progestophilins, in this case) seems to require, however, the direct action of E2. The E2concentrations effecting the induction of progestophilins were higher than those necessary to effect the proliferation of oviduct cells. These results suggest that the E2effect on cell proliferation is indirect, it involves an intermediary step at the liver, and it does not require increased concentration of nuclear estrophilins.
ISSN:0027-8424
1091-6490
DOI:10.1073/pnas.80.6.1621