20 results on '"Brenner, R M"'
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2. Testosterone Synthesis in Rhesus Fetal Testes: Comparison Between Middle and Late Gestation1
- Author
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Ellinwood, W. E., Brenner, R. M., Hess, D. L., and Resko, J. A.
- Abstract
Several aspects of testosterone synthesis were examined in fetal testes of rhesus monkeys at middle (Days 79 to 82) and late gestation (Days 140 to 149). Histological examination of fetal testes revealed that Leydig cells are smaller at late gestation and that there are approximately one-third as many Leydig cells per unit area compared with midgestation. The concentration of testosterone in umbilical arterial serum, however, was not significantly lower at late gestation. In vitro synthesis of testosterone and cyclic AMP (cAMP) was stimulated by human chorionic gonadotropin (hCG) in tissues collected at both stages of gestation. The testosterone concentration of testicular tissue and testosterone synthesis in the absence of hCG were ∿2-fold greater at midgestation (P<0.05), but the rate of testosterone synthesis in the presence of hCG did not differ between the two stages. In contrast, cAMP synthesis was 4-fold greater in the absence of hCG and 9-fold greater in the presence of hCG in tissues collected at midgestation (P<0.01). Concentrations of biologically active luteinizing hormone (LH) in the fetal circulation were found to be 2-fold greater at late gestation than at midgestation (P<0.01).The data indicate that fetal testes of the rhesus monkey are steroidogenically active and capable of responding to gonadotropin in vitro at both middle and late gestation. The testicular adenylate cyclase system appears to be more active and more responsive to exogenous gonadotropin at midgestation, but Leydig cells at late gestation secrete testosterone at a rate that is as great as or greater than at midgestation. The greater concentrations of biologically active LH in the fetal circulation at late gestation may be the reason fewer Leydig cells are able to maintain high serum testosterone levels.
- Published
- 1980
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3. Effects of Estradiol-17βand Progesterone on Cyclic Nucleotide Metabolism in Myometrium of Macaques
- Author
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Beatty, C. H., Bocek, R. M., Herrington, P. T., Young, M. K., and Brenner, R. M.
- Abstract
We determined the activities of the adenylate (homogenate) and guanylate cyclases (100,000 × g supernatant) and the cyclic nucleotide phosphodiesterases (PDEs) (100,000 × g supernatant and particulate) of myometria from: 1) rhesus monkeys spayed for at least 6 months and treated either with estradiol-17β(E2) for 14 days or with E2for 14 days and then treated for 5–14 additional days with E2plus progesterone (P); and 2) cynomolgus monkeys during the follicular and luteal phases of natural menstrual cycles. Plasma levels of E2and P were similar in the spayed rhesus monkeys treated with hormones and the naturally cycling cynomolgus monkeys. The specific activities of the guanylate cyclase and the cAMP- and cGMP-PDE enzymes/mg nitrogen or DNA were decreased in myometria from monkeys in the luteal compared with the follicular phase of both natural and induced menstrual cycles; no difference was observed in adenylate cyclase activity. There was also no difference in the concentrations of nitrogen and of DNA in the follicular and luteal phase myometrium. The average cAMP/cGMP ratio was more than twice as high in the follicular compared with the luteal phase (8.5 vs 3.7). This decrease in the cyclic nucleotide ratio was due mainly to an increase in cGMP levels and suggests that in vivo the activity of the guanylate cyclase enzyme decreased less than did the activity of the cGMP-PDE. These data strongly suggest that it is P that causes the decrease in the activities of the guanylate cyclase and cyclic nucleotide PDE, because enzyme activity is significantly higher in the myometrium during the follicular phases of both the induced and natural menstrual cycles. It appears that cyclic nucleotide metabolism in nonhuman primate myometrium varies during the menstrual cycle.
- Published
- 1979
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4. Estradiol-Induced Differentiation of the Oviductal Epithelium in Ovariectomized Cats
- Author
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Verhage, H. G. and Brenner, R. M.
- Abstract
The effect of 17β-estradiol on the oviductal epithelium of ovariectomized cats was studied by light and electron microscopy. Estradiol was administered by implantation of a silastic capsule containing crystalline 17β-estradiol. Two months after ovariectomy the epithelial cells were atrophied and nonciliated. Estradiol treatment resulted in hypertrophy, mitotic activity and partial differentiation of both the nucleus and cytoplasm during days one to three. This differentiation included the conversion of chromatin from a condensed to a dispersed state along with the appearance of a distinct nucleolus, and an increase in the amount of polyribosomes, mitochondria, Golgi apparatus and short profiles of smooth endoplasmic reticulum. Ciliogenesis was found to be a multiphase process which occurred primarily on days two through five of estrogen treatment. Fibrogranular aggregates and patches of fibrous granules were evident in the apices of the future ciliated cells on day two. Procentrioles and basal bodies in various stages of development were found associated with either deuterosomes or diplosomal centrioles on days three and four. On day four mature basal bodies were either arranged in linear fashion at the apical border or were already aligned giving rise to ciliary buds and short cilia. After seven days of estrogen treatment 60 percent of the epithelial cells were ciliated. The remaining cells possessed abundant cisternae of endoplasmic reticulum and appeared to be differentiating into secretory cells. After 10 to 14 days, these cells possessed a large Golgi apparatus, dilated cisternae of endoplasmic reticulum and scattered apical secretory granules. This study clearly demonstrates that 17β-estradiol can restore the oviductal epithelium of the ovariectomized cat to a fully differentiated state, and that the mode of basal body and cilia formation is essentially the same as in the oviducts of various other species.
- Published
- 1975
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5. A Delayed Antagonistic Effect of Progesterone on the Estradiol-Induced Differentiation of the Oviductal Epithelium in Spayed Cats
- Author
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Verhage, H. G. and Brenner, R. M.
- Abstract
We have shown previously (West et al., 1976) that progesterone (P) antagonizes the effect of estradiol (E2) on the oviducts of cats when E2and P are administered sequentially (E2first, then E2+ P). To determine whether P could completely block the effects of E2on the oviduct with reversal of the sequential treatment pattern, we treated two groups of spayed cats with silastic implants of P (12 cm) and E2(0.5 cm) as follows. Group A: P (7 days); P + E2(14 days). Group B: blank implant (7 days); E2(14 days).Oviducts were collected and fixed at closely spaced intervals for morphologic and cytomorphometric determinations. The mean plasma levels of E2in Groups A and B were similar (16.8 and 19.7 pg/ml, respectively) whereas the mean level of P was 14.1 ng/ml in Group A and 0.3 ng/ml in Group B animals. After two days of E2treatment, cells from both treatment groups showed identical patterns of mitosis and hypertrophy. On Days 3–5, combined E2-P treatment had prevented further cell hypertrophy (Fimbriae: 21.9 μm[A], 26.6 μm[B]; Ampulla 21.3 μm[A], 28.9 μm[B]), but ciliogenesis was evident in cells from both groups. By Day 7, combined E2-P treatment had somewhat reduced the number of ciliated cells in the fimbriae (Group A: 46 percent; Group B: 67 percent) and more dramatically in the ampulla (Group A: 22 percent; Group B: 63 percent). By 14 days the combined E2-P treatment had led to further atrophy and extensive deciliation (Fimbriae: 15.5 μm and 22 percent [A], 24.3 μm and 57 percent [B]; Ampulla: 16.5μm and 13 percent [A], 27 μm and 48 percent [B]). In the presence of P, the nonciliated cells never became functional secretory cells.These data suggest that in cats a period of E2-induced differentiation must occur before P can antagonize the E2effect, that P antagonism develops gradually, and that the rate at which P antagonism develops differs from region of the oviduct to another.
- Published
- 1976
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6. Plasma Levels of Estradiol and Progesterone in the Cat During Polyestrus, Pregnancy and Pseudopregnancy
- Author
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Verhage, H. G., Beamer, N. B., and Brenner, R. M.
- Abstract
The levels of estradiol and progesterone in the systemic plasma of four domestic cats during pregnancy, pseudopregnancy and polyestrus were determined by radioimmunoassay. During polyestrus, estradiol values fluctuated between peaks (59.5 ± 13.4 (SD) pg/ml; n = 13) and troughs (8.1 ± 3.8 (SD) pg/ml; n=12) with an interpeak period of 15.8 ± 3.8 days (n=9). After the animals had been mated to either intact or vasectomized males, their estradiol levels declined sharply from peak values and remained low (6–12 pg/ml) during pseudopregnancy and pregnancy except for a slight rise just before parturition. Essentially no progesterone could be detected during polyestrus and for 2 to 3 days after copulation with either intact or vasectomized males, but by Day 21 of pregnancy or pseudopregnancy progesterone rose to a peak of either ∿35 or ∿24 ng/ml respectively. After Day 21 of pregnancy, progesterone gradually declined to ∿10 ng/ml by Day 60, ∿5 ng/ml just before parturition, and <1 ng/ml just after parturition. After Day 21 of pseudopregnancy, progesterone levels declined rapidly to ∿4 ng/ml by Day 40, ∿2 ng/ml by Day 50 and <1 ng/ml by Day63–65. Estrone was measured throughout pregnancy, pseudopregnancy and polyestrus in one animals; no major elevations were detected.
- Published
- 1976
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7. Effects of Estradiol-17β and Progesterone on Cyclic Nucleotide Metabolism in Myometrium of Macaques
- Author
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Beatty, C. H., primary, Bocek, R. M., additional, Herrington, P. T., additional, Young, M. K., additional, and Brenner, R. M., additional
- Published
- 1979
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8. Matrix metalloproteinase expression in Macaca mulatta endometrium: evidence for zone-specific regulatory tissue gradients.
- Author
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Rudolph-Owen LA, Slayden OD, Matrisian LM, and Brenner RM
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- Animals, Blotting, Northern, Endometrium anatomy & histology, Endometrium drug effects, Estradiol administration & dosage, Estradiol pharmacology, Female, Follicular Phase, Macaca mulatta, Matrix Metalloproteinase 3 metabolism, Matrix Metalloproteinase 7, Menstruation, Metalloendopeptidases analysis, Metalloendopeptidases metabolism, Ovariectomy, Progesterone administration & dosage, Progesterone pharmacology, RNA, Messenger metabolism, Tissue Inhibitor of Metalloproteinase-1 metabolism, Endometrium enzymology, Gene Expression Regulation, Enzymologic, Metalloendopeptidases genetics
- Abstract
Matrix metalloproteinases (MMPs) are highly expressed in the human endometrium during menstruation, and these enzymes participate in the cyclic destruction and regeneration characteristic of the primate endometrium. To examine hormonal regulation of MMPs in vivo, we evaluated MMP expression and localization in the endometrium of ovariectomized rhesus macaques under various hormonal conditions. Although all MMPs were up-regulated by progesterone (P4) withdrawal, their expression declined spontaneously after menstruation in the absence of P4. Of 7 MMPs examined, only matrilysin and stromelysin-3 were suppressed any further when P4 levels were experimentally re-elevated. MMP expression was confined to the upper functionalis zone during menstruation, but after menstrual breakdown was complete, matrilysin and the tissue inhibitor of MMPs, TIMP-1, shifted expression from the functionalis to the basalis zone in the absence of both estradiol and P4. The spiral arteries in the functionalis, but not the basalis, were intense foci of MMP and TIMP-1 expression. Menstruation and MMP expression after P4 withdrawal were similar in both the presence and absence of estradiol. In sum, endometrial MMPs in vivo are strongly up-regulated by P4 withdrawal, but zone-specific tissue gradients greatly influence the pattern and degree of MMP expression.
- Published
- 1998
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9. Oviduct physiology and sperm/oviduct interactions: an introduction.
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Brenner RM
- Subjects
- Animals, Female, Humans, Male, Pregnancy, Fallopian Tubes physiology, Fertilization physiology, Spermatozoa physiology
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- 1998
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10. Androgen receptor and 5 alpha-reductase activity in the ductuli efferentes and epididymis of adult rhesus macaques.
- Author
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Roselli CE, West NB, and Brenner RM
- Subjects
- Animals, Cholestenone 5 alpha-Reductase, Immunohistochemistry, Kinetics, Macaca mulatta, Male, Rete Testis metabolism, Epididymis metabolism, Oxidoreductases metabolism, Receptors, Androgen metabolism
- Abstract
We measured androgen receptors (AR) and 5 alpha-reductase activity (5 alpha RA) in the ductuli efferentes and epididymides from adult rhesus macaques. Tissue samples were either assayed biochemically for AR or stained immunocytochemically (ICC) with a monoclonal antibody against AR. To estimate 5 alpha RA, tissue microsomes were incubated with [1 alpha,2 alpha-3H]testosterone, and the [3H]dihydrotestosterone formed was quantified. We found significant regional differences in the levels of both 5 alpha RA and AR in the excurrent ducts. In general, both enzyme activity and AR levels were higher in the caput and corpus epididymis than in ductuli efferentes and cauda epididymis. With ICC, positive nuclear AR staining was detected in all epithelial cell types, whereas variable numbers of stromal cells were positively stained. Our data demonstrate that there are segmental differences in the concentrations of 5 alpha RA and AR in epididymis and suggest that there may be regional differences in the regulation of epididymal functions by androgen.
- Published
- 1991
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11. Localization of androgen receptor in the follicle and corpus luteum of the primate ovary during the menstrual cycle.
- Author
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Hild-Petito S, West NB, Brenner RM, and Stouffer RL
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- Animals, Corpus Luteum metabolism, Female, Immunohistochemistry, Macaca fascicularis, Macaca mulatta, Ovarian Follicle metabolism, Menstrual Cycle metabolism, Ovary metabolism, Receptors, Androgen metabolism
- Abstract
Ovarian androgens may act locally to modulate follicular and luteal function in various species. This study examined the distribution of androgen receptors within the primate ovary throughout the menstrual cycle. Ovaries were collected from rhesus and cynomolgus monkeys during the early, mid-, and late (n = 3-5 per stage) follicular and luteal phases of the cycle. The tissues were processed for indirect immunocytochemical localization of androgen receptors with a specific monoclonal antibody against human androgen receptor (AN1-15). In addition, ovaries (n = 3) were collected from rhesus monkeys for biochemical detection of androgen receptor using 3H-androgen and AN1-15. Specific immunocytochemical staining, as determined by comparing adjacent tissue sections incubated with either AN1-15 or a nonspecific control antibody, was exclusively nuclear. Androgen receptor was detected in the germinal epithelium and ovarian stroma at all stages of the cycle. The thecal and granulosa cells of growing follicles, and of many but not all atretic follicles, contained androgen receptors. Luteinizing granulosa cells of the periovulatory follicle and luteal cells from the early and midluteal phase stained intensely for androgen receptor. Regressing corpora lutea of the late luteal phase also stained for androgen receptor; however, fully regressed corpora lutea in the early follicular phase of the next cycle did not exhibit receptor staining. Luteal cells that were androgen receptor-positive also stained histochemically for the presence of 3 beta-hydroxysteroid dehydrogenase. Sucrose gradient analysis with radiolabeled androgen demonstrated a shift in the androgen receptor peak in monkey ovarian tissue upon addition of AN1-15, confirming the presence of androgen receptor.(ABSTRACT TRUNCATED AT 250 WORDS)
- Published
- 1991
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12. Estrogen receptor in the ductuli efferentes, epididymis, and testis of rhesus and cynomolgus macaques.
- Author
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West NB and Brenner RM
- Subjects
- Animals, Antibodies analysis, Centrifugation, Density Gradient, Epididymis cytology, Epididymis metabolism, Male, Receptors, Estrogen immunology, Testis cytology, Testis metabolism, Vas Deferens cytology, Vas Deferens metabolism, Epididymis ultrastructure, Macaca metabolism, Macaca fascicularis metabolism, Macaca mulatta metabolism, Receptors, Estrogen metabolism, Testis ultrastructure, Vas Deferens ultrastructure
- Abstract
We obtained the testes, ductuli efferentes, and epididymides from adult rhesus and cynomolgus macaques and examined these tissues for estrogen receptors (ER) with immunocytochemistry (ICC) and a sucrose gradient assay. Both techniques employed monoclonal antibodies prepared against ER, and both showed that high concentrations of ER were present OFFy in the ductuli efferentes. Moreover, all specific staining was confined to the nuclei of the nonciliated, absorptive epithelial cells. The quantity of salt-extractable ER in the ductuli efferentes (834 +/- 161 [SEM] fmol/mg DNA [n = 8]) did not differ significantly from the amounts measured with the identical assay in oviducts and endometrium of estrogenized female macaques. Testes and epididymides of macaques had no specific staining by ICC and barely detectable amounts by biochemical analysis (7 +/- 4 [n = 3], 8 +/- 2 [n = 5], 33 +/- 16 [n = 3], and 6 +/- 3 [n = 8] fmol/mg DNA for testis and caput, corpus, and cauda epididymis, respectively). The functional significance of the high levels of ER in the ductuli efferentes of macaques remains to be determined.
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- 1990
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13. Estrogen and progestin receptors in the reproductive tract of male and female primates.
- Author
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Brenner RM, West NB, and McClellan MC
- Subjects
- Animals, Endometrium analysis, Fallopian Tubes analysis, Female, Macaca fascicularis, Macaca mulatta, Macaca nemestrina, Male, Prostate analysis, Seminal Vesicles analysis, Genitalia analysis, Receptors, Estrogen analysis, Receptors, Progesterone analysis
- Abstract
With the aid of monoclonal antibodies specific to the estrogen and progestin receptors, we have examined the cellular localization of these proteins in the reproductive tract of male and female macaques. Two striking findings have resulted from our work with these new reagents. First, these receptors are detectable only in cell nuclei, regardless of hormonal treatment, and second, they are often detectable in stromal, but not epithelial cells when the epithelial cells undergo various estrogen or progestin-dependent events. The latter observation has led us to conclude that stromal cell-epithelial cell interactions may play previously unappreciated roles in the hormonal control of the primate reproductive tract. The lines of evidence that have drawn us to this conclusion will be reviewed.
- Published
- 1990
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14. Hormonal regulation of sex skin in Macaca nemestrina.
- Author
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Carlisle KS, Brenner RM, and Montagna W
- Subjects
- Animals, Castration, Estradiol blood, Female, Genitalia, Female anatomy & histology, Progesterone blood, Skin anatomy & histology, Skin ultrastructure, Genitalia, Female physiology, Gonadal Steroid Hormones physiology, Macaca physiology, Macaca nemestrina physiology, Skin Physiological Phenomena
- Published
- 1981
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15. Estrogen receptor levels in the oviducts and endometria of cynomolgus macaques during the menstrual cycle.
- Author
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West NB and Brenner RM
- Subjects
- Animals, Cytoplasm analysis, Estradiol blood, Female, Follicular Phase, Luteal Phase, Macaca fascicularis, Progesterone blood, Endometrium analysis, Fallopian Tubes analysis, Menstruation, Receptors, Estrogen analysis
- Abstract
We sampled oviducts and endometria of 27 cynomolgus macaques during the menstrual cycle and measured the concentration of nuclear and cytoplasmic estrogen receptors in these tissues by exchange assay. We assessed the stage of the cycle by correlating serum estradiol (E2) and progesterone (P), as measured by radioimmunoassay, with the morphological condition of the ovaries, oviducts and endometrium of each animal. We have previously identified a series of oviductal stages that reflected the orderly sequence of cytological changes in the oviduct during the cycle, and we normalized receptor measurements to these stages. The amounts of nuclear and cytoplasmic estrogen receptor in both the oviduct and the endometrium were approximately twofold greater in the follicular phase than in the luteal phase. In the follicular phase, elevated receptor levels were associated with oviductal proliferation and differentiation, as well as with endometrial proliferation. During the luteal phase, lowered levels were correlated with atrophy and dedifferentiation in the oviduct, but with hypertrophy and progestational development in the endometrium. When the luteal phase of one cycle ends and the follicular phase of the next begins, it is a decline in serum P, not a rise in serum E2, that precedes the elevation in estrogen receptor level and the onset of proliferation in the oviduct and endometrium. Proliferation of the reproductive tract and elevations in nuclear estrogen receptor levels during the early follicular phase can therefore be viewed as consequences of the release of the system from antagonism by P.
- Published
- 1983
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16. Morphology of the oviducts and endometria of cynomolgus macaques during the menstrual cycle.
- Author
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Brenner RM, Carlisle KS, Hess DL, Sandow BA, and West NB
- Subjects
- Animals, Estradiol blood, Female, Macaca fascicularis, Progesterone blood, Endometrium cytology, Fallopian Tubes cytology, Menstruation
- Abstract
We sampled the reproductive tracts of 27 cynomolgus macaques during the menstrual cycle and correlated the cytologic changes in the oviductal epithelium with changes in the serum levels of estradiol (E2) and progesterone (P) and with the histology of the ovaries and the endometria. We identified an orderly sequence of changes in the oviductal epithelium from the early follicular to the late luteal phase, and we classified this sequence into eight stages, named as follows: preciliogenic, ciliogenic, ciliogenic-ciliated, ciliated-ciliogenic, ciliated-secretory, early regression, late regression and full regression. The preciliogenic and ciliogenic phases were coincident with menses and the early follicular phase. The ciliogenic-ciliated, ciliated-ciliogenic and ciliated-secretory phases during which the oviductal epithelium became progressively more differentiated were coincident, respectively, with the midfollicular, late follicular and periovulatory phases of the cycle. The early, late and full regression stages during which the epithelium became progressively more atrophied, deciliated and nonsecretory were coincident, respectively, with the early, mid and late luteal phases of the cycle. The cyclic changes in the endometrium of cynomolgus macaques were similar to those reported for the rhesus macaque.
- Published
- 1983
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17. Changes in nuclear estradiol receptor and cell structure during estrous cycles and pregnancy in the oviduct and uterus of cats.
- Author
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West NB, Verhage HG, and Brenner RM
- Subjects
- Anestrus, Animals, Cats, Copulation, Endometrium cytology, Fallopian Tubes cytology, Female, Pregnancy, Proestrus, Receptors, Estrogen, Cell Nucleus metabolism, Endometrium metabolism, Estradiol metabolism, Estrus, Fallopian Tubes metabolism, Pregnancy, Animal
- Published
- 1977
- Full Text
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18. Sex steroids in reproductive tract tissues: regulation of estradiol concentrations by progesterone.
- Author
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Resko JA, Boling JL, Brenner RM, and Blandau RJ
- Subjects
- Animals, Estradiol pharmacology, Female, Haplorhini, Macaca mulatta, Muscles metabolism, Progesterone metabolism, Radioimmunoassay, Rats, Estradiol metabolism, Fallopian Tubes metabolism, Progesterone pharmacology, Uterus metabolism
- Published
- 1976
- Full Text
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19. Estradiol synthesis by fetal monkey ovaries correlates with antral follicle formation.
- Author
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Ellinwood WE, McClellan MC, Brenner RM, and Resko JA
- Subjects
- Androstenedione biosynthesis, Animals, Cyclic AMP biosynthesis, Dehydroepiandrosterone biosynthesis, Female, Gestational Age, In Vitro Techniques, Lipids analysis, Microscopy, Electron, Organoids ultrastructure, Ovary embryology, Ovary ultrastructure, Progesterone metabolism, Estradiol biosynthesis, Macaca embryology, Macaca mulatta embryology, Ovary metabolism
- Abstract
We compared the morphology of ovaries from fetal rhesus monkeys at two different stages of gestation with the ability of ovarian tissue to synthesize androgens and estrogens in vitro. Ovaries collected between 80 and 104 days of gestation contained single-layered primordial follicles but no multilayered or antral follicles. Within these ovaries we found theca-like interstitial cells which contained abundant smooth endoplasmic reticulum and lipid droplets. These ovaries produced androstenedione and dehydropiandrosterone (but not estradiol) in vitro in the absence of exogenous substrates. Ovaries collected between Days 124 and 153 of gestation, however, contained numerous, well-developed multilayered and antral follicles. The ultrastructural characteristics of the thecal and granulosa cell layers were similar to those of adult ovarian follicles. These ovaries synthesized large amounts of androstenedione, dehydroepiandrosterone, and estradiol in vitro. Identity of the estradiol was confirmed by incubating homogenates of late gestation ovaries with [14C]progesterone, by isolation of estradiol and formation of its derivative, and by recrystallization to constant specific activity. In vitro cyclic AMP synthesis was stimulated by Pergonal (luteinizing hormone [LH] + follicle stimulating hormone [FSH] ) only in ovaries which contained multilayered and antral follicles, an indication that fetal ovaries contain gonadotropin receptors during late stages of development. These data indicate that fetal ovaries of rhesus monkeys attain the capacity for de novo estrogen biosynthesis and to respond to gonadotropins during late gestation, when multilayered and antral follicles have developed.
- Published
- 1983
- Full Text
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20. Effects of estradiol-17 beta and progesterone on cyclic nucleotide metabolism in myometrium of macaques.
- Author
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Beatty CH, Bocek RM, Herrington PT, Young MK, and Brenner RM
- Subjects
- 2',3'-Cyclic-Nucleotide Phosphodiesterases analysis, Adenylyl Cyclases analysis, Animals, Castration, Collagen analysis, Cyclic AMP analysis, Cyclic GMP analysis, DNA analysis, Endometrium enzymology, Endometrium metabolism, Estradiol analysis, Female, Guanylate Cyclase analysis, Haplorhini, Myometrium drug effects, Myometrium enzymology, Nitrogen analysis, Progesterone analysis, Estradiol pharmacology, Macaca physiology, Macaca mulatta physiology, Menstruation drug effects, Myometrium metabolism, Nucleotides, Cyclic metabolism, Progesterone pharmacology, Uterus metabolism
- Published
- 1979
- Full Text
- View/download PDF
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