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JBC, Vol. 251, Issue 18, 5694-5702, Sep, 1976
S. Strickland and W. H. Beers
A quantitative method is described for measuring the amount of plasminogen
activator produced by rat ovarian granulosa cells following exposure to
hormones in vivo or in vitro. The results confirm the previously reported
observation (Beers, W. H., Strickland, S., and Reich, E. (1975) Cell 6,
(387-394) that granulosa cells in vivo produce increasing amounts of
plasminogen activator as the time of ovulation approaches and that the
enzyme is produced only be cells obtained from follicles destined to
ovulate. Inactive cells can be stimulated in vitro by gonadotropins to
produce plasminogen activator. This response is time- and dose-dependent,
and results in an increase of intracellular and extracellular enzyme.
Studies of the specificity of this response indicate that preparations of
follicle-stimulating hormone are much more effective than corresponding
preparations of luteinizing hormone. The effect of other pituitary hormones
is also presented. Molecules other than gonadotropins are also capable of
stimulating the cells to produce the enzyme. Prostaglandins E1 and E2 and
analogues of cAMP effectively stimulated the cells to produce plasminogen
activator, cGMP and its analogues and prostaglandins F1a and F2a were
without effect as were the six steroids studied. The inactive compounds
also did not inhibit the response of the cells to gonadotropins. The
granulosa cell plasminogen activator has been analyzed by sodium dodecyl
sulfate-polyacrylamide gel electrophoresis and has an apparent molecular
weight of 75,000. By this and other criteria, the granulosa cell enzyme is
similar to one of the species of plasminogen activators obtained from
cultures of simian virus 40-transformed rat embryo fibroblasts.
Studies on the role of plasminogen activator in ovulation. In vitro response of granulosa cells to gonadotropins, cyclic nucleotides, and prostaglandins
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