Estrogen,Progesterone and Epithelial Ovarian Cancer

Ovarian carcinoma (OCa) continues to be the leading cause of death due to gynecologic malignancies and the vast majority of OCa is derived from the ovarian surface epithelium (OSE) and its cystic derivatives. Epidemiological evidence strongly suggests that steroid hormones, primarily estrogens and progesterone, are implicated in ovarian carcinogenesis. However, it has proved difficult to fully understand their mechanisms of action on the tumorigenic process. New convincing data have indicated that estrogens favor neoplastic transformation of the OSE while progesterone offers protection against OCa development. Specifically, estrogens, particularly those present in ovulatory follicles, are both genotoxic and mitogenic to OSE cells. In contrast, pregnancy-equivalent levels progesterone are highly effective as apoptosis inducers for OSE and OCa cells. In this regard, high-dose progestin may exert an exfoliation effect and rid an aged OSE of pre-malignant cells. A limited number of clinical studies has demonstrated efficacies of antiestrogens, aromatase inhibitors, and progestins alone or in combination with chemotherapeutic drugs in the treatment of OCa. As a result of increased life expectancy in most countries, the number of women taking hormone replacement therapies (HRT) continues to grow. Thus, knowledge of the mechanism of action of steroid hormones on the OSE and OCa is of paramount significance to HRT risk assessment and to the development of novel therapies for the prevention and treatment of OCa.     

Bovine Uterine,Cervical and Ovarian Cytosol Estrogen and Progesterone Receptor Concentrations in Cystic Ovarian Disease

Bovine cytosol estrogen (ERC) and progesterone receptor (PRC) concentrations were measured simultaneously in various regions of the uterus and in ovarian stromal tissue in cows with cystic ovarian disease (follicular cysts), arid the concentrations compared with those in animals with normal cycles. In cystic ovarian disease, ERC concentrations in endometrium (550 fmol/mg cytosol protein (c.p.)) and in myometrium (405) were significantly higher than in control animals. Very high PRC contents were measured in the endometrium (3115) and myometrium (2761) of cows with cystic ovarian disease. In control animals, PRC concentrations in the endometrium and myometrium were significantly lower than in diseased animals. No statistical differences were observed in ERC or PRC contents between the endometrium and the myometrium in cows with cystic ovarian disease. ERC and PRC concentrations in the uterine cervix and ovaries were low compared to those detected in the uterus. Bovine serum estradiol-17ß concentrations were higher (p<0.001) in cows with cystic ovarian disease than in control animals in postpartum anestrus or during the normal estrous cycle. Serum sex hormone-binding globulin (SHBG) concentrations were of the same magnitude as in control cows during their estrous cycles. These findings show that long standing low endogenous progesterone and elevated estradiol concentrations in serum are associated with elevated ERC and PRC concentrations in bovine uterus.     

被动吸烟下调大鼠卵巢雌、孕激素及其受体的表达

目的利用Wistar大鼠烟雾吸入模型,观察被动吸烟对Wistar大鼠卵巢结构的影响,检测生殖激素水平,分析生殖内分泌的变化,为提倡生育期妇女避免被动吸烟提供新的理论依据。方法建立大鼠烟雾吸入模型。32只健康雌性Wistar大鼠,鼠龄(60±5)d,每只体重200～250g,随机分为空白对照组和实验组,每组16只。实验组吸烟3个月,对照组正常饲养。3个月后处死两组大鼠。酶联免疫吸附试验方法 (enzyme linkedimmunosorbent assay,ELISA)检测雌鼠血清中雌激素(estrogen,E2)、孕激素(progesterone,P4)的水平;常规石蜡切片,免疫组织化学SP法检测各组雌鼠卵巢雌激素受体(estrogen receptor,ER)、孕激素受体(progesterone receptor,PR)的表达情况。所得数据采用SPSS软件作统计学处理分析,比较各组间差异程度。结果①酶联免疫吸附试验结果 :吸烟3个月大鼠血清E2水平比空白对照组显著降低,其浓度值比较差异有显著性;吸烟3个月大鼠血清P4水平比空白对照组显著降低,其浓度值比较差异有显著性。②免疫组织化学结果 :ER主要表达在大鼠卵巢组织的各级生长卵泡的颗粒细胞的细胞核内,呈棕黄色颗粒状分布,卵泡膜细胞和间质细胞也有少量表达。吸烟3个月的大鼠卵巢组织中ER的表达显著低于空白对照组。PR主要表达在大鼠卵巢组织卵泡的颗粒细胞的细胞质和细胞核中,呈棕黄色颗粒状分布,吸烟3个月的大鼠卵巢组织中PR的表达显著低于空白对照组。结论①成功的建立了大鼠被动吸烟模型。②被动吸烟可使大鼠血清中E2及P4水平明显降低,使大鼠卵巢中ER及PR的表达减少,提示被动吸烟可破坏卵巢的功能,引起生殖内分泌失调。     

Ultrastructure of Bovine Ovarian Follicles Induced to Extended Growth by Perioestrous Suprabasal Progesterone Levels

The present study was undertaken to determine if a short-term prolonged growth of the ovulatory follicle (12 to 18 h after expected time of ovulation), induced by progesterone implants, would cause ultrastructural changes in the follicular wall. Oestrous behaviour, follicular growth, follicular and blood plasma levels of oestradiol-17ß, progesterone and plasma luteinizing hormone (LH) were monitored in heifers oophorectomized at 9 to 12 h (controls) or 36 h after the onset of oestrus, in order to sample the pre-ovulatory follicle present. The suprabasal plasma progesterone concentrations (approximately 1.2 nmol L−1) allowed expression of oestrus at the expected time, but ovulation was delayed owing to the absence of a LH-surge. The resulting prolongation of follicle growth was associated with mild degenerative changes in the follicle wall, i.e. both granulosa and thecal cells presented increased electron density, higher amounts of secondary lysosomes and lipid droplets, increased intercellular spaces with presence of debris. No signs of luteinization were seen.     

Preovulatory endocrinology and oocyte maturation in superovulated cattle

Preovulatory follicular and oocyte nuclear maturation was studied in donor cattle induced to superovulate with a PMSG- or FSH-prostaglandin regimen. Plasma concentrations of progesterone (P4) and luteinizing hormone (LH) and follicular fluid levels of progesterone and estradiol-17β were measured and related to the oocyte nuclear maturation stages. The oocyte donors could be divided into two distinct groups. Group I had entirely normal periovulatory P4 and LH concentrations, and the majority of follicles and oocytes followed a characteristic pattern, clearly time-related to the LH peak. Group II had deviating levels of P4 and/or LH in the pre- and periovulatory period, and a majority of their follicles and oocytes had disturbed maturation, such as abnormal P4:E2 ratio in follicles and prematurely activated or meiotically arrested oocytes. It is concluded that a certain proportion of superovulated cows and heifers develop abnormal follicular/oocyte maturation and constitute poor oocyte, and probably also embryo, donors.     

Preovulatory evaluation of the superovulatory response in donor cattle

Dairy cows and heifers (n = 134) were induced to superovulate with exogenous gonadotrophins. In 103 animals, peripheral plasma concentrations of progesterone (P4) and luteinizing hormone (LH) were measured during the preovulatory period. On the basis of these measurements, normal and deviating profiles of P4 and LH were defined. A high degree of correlation existed between the normality of the two profiles; when the P4 profile was normal, the probability for the LH profile also to be normal was greater than 10:1. This relationship was utilized to evaluate donors based on four preovulatory measurements of P4. When used on 31 animals used for collection of eggs, a superior superovulatory response was encountered in animals with normal vs deviating P4 profiles (eggs recovered: 7.2 +/- 1.1 vs 0.5 +/- 0.3, P < 0.001; transferable embryos: 4.4 +/- 0.9 vs 0.3 +/- 0.2, P < 0.01). It is concluded that evaluation of donors by measurements of progesterone in plasma at four preovulatory sampling points allows for the early exclusion of donors with inferior embryo yield.     

Estrogen-Inducible Progesterone Receptors in the Rat Lumbar Spinal Cord: Regulation by Ovarian Steroids and Fluctuation across the Estrous Cycle

Ovarian hormones influence the physiology of the spinal cord through incompletely understood cellular mechanisms. To date, there has been little compelling evidence for progesterone receptors in spinal cord neurons. Using two antibodies specific for progesterone receptors in an immunohistochemical investigation, we now report the presence of estrogen-inducible progesterone receptors in the spinal cord. Estrogen-inducible progesterone receptors were observed in the neurons of lamina X and the interomedialateral cell column, which are also known to express estrogen receptors. Estrogen-inducible progesterone receptors similar to those observed in females were also apparent in lamina X and interomediolateral cell column neurons in the spinal cords of males treated with estradiol. Furthermore, the density of progesterone receptors in lamina X was observed to fluctuate across the estrous cycle in female rats, with the highest progesterone receptor expression levels occurring late in proestrus, following the estradiol surge and coincident with high circulating progesterone levels. The lowest progesterone receptor expression levels were observed late in estrus following the progesterone surge. Together, these results demonstrate that estrogen-sensitive progestin targets exist in the spinal cord, and their possible role in the nervous control of reproduction and ovarian steroid modulation of nociception is discussed.     

Preovulatory LH profiles of superovulated cows and progesterone concentrations at embryo recovery

Forty-two Holstein cows were randomly assigned to three superovulatory treatment groups of 14 cows each. Cows in Group I received follicle stimulating hormone (FSH; 50 mg i.m.); those in Group II received FSH (50. mg i.m.) along with GnRH (250 ug in 2 % carboxymethylcellulose s.c.) on the day of estrus; and cows in Group III were infused FSH (49 mg) via osmotic pump implants. FSH was administered over a 5-d period for cows in Groups I and II (twice daily in declining doses). Cows in Group III received FSH over a 7-d period (constantly at a rate of 7 mg/day). All cows received 25 mg PGF(2)alpha (prostaglandin F(2)alpha) 48 hours after initiation of the FSH treatment. Blood samples were collected from seven cows from each group at 2 hour intervals on the fifth day of superovulation for serum luteinizing hormone (LH) concentration analysis by radioimmunoassay, and blood samples were collected from all cows on the day of embryo recovery for plasma progesterone determination. The LH profile was not altered (P>0.05) by either GnRH administration or by the constant infusion of FSH as compared to FSH treatment alone. Plasma progesterone concentrations were highly correlated with the number of corpora lutea (CL) palpated (r=0.92; P<0.01) and with the number of ova and/or embryos recovered (r=0.88; P<0.01). The accuracy of predicting the number of recoverable ova and/or embryos by the concentration of plasma progesterone was 86%.     

Effect of Monochromatic Light on Expression of Estrogen Receptor (ER) and Progesterone Receptor (PR) in Ovarian Follicles of Chicken

Artificial illumination is widely used in modern poultry houses and different wavelengths of light affect poultry production and behaviour. In this study, we measure mRNA and protein abundance of estrogen receptors (ERs) and progesterone receptors (PRs) in order to investigate the effect of monochromatic light on egg production traits and gonadal hormone function in chicken ovarian follicles. Five hundred and fifty-two 19-wk-old laying hens were exposed to three monochromatic lights: red (RL; 660 nm), green (GL; 560 nm), blue (BL; 480 nm) and control cool white (400–760 nm) light with an LED (light-emitting diode). There were 4 identical light-controlled rooms (n = 138) each containing 3 replicate pens (46 birds per pen). Water was supplied ad libitum and daily rations were determined according to the nutrient suggestions for poultry. Results showed that under BL conditions there was an increase in the total number of eggs at 300 days of age and egg-laying rate during the peak laying period. The BL and GL extended the duration of the peak laying period. Plasma melatonin was lowest in birds reared under BL. Plasma estradiol was elevated in the GL-exposed laying hens, and GL and BL increased progesterone at 28 wk of age. In the granulosa layers of the fifth largest preovulatory follicle (F5), the third largest preovulatory follicle (F3) and the largest preovulatory follicle (F1), ERα mRNA was increased by BL and GL. Treatment with BL increased ERβ mRNA in granulosa layers of F5, F3 and F1, while GL increased ERβ mRNA in F5 and F3. There was a corresponding increase in abundance of the proteins in the granulosa layers of F5, with an increase in PR-B, generated via an alternative splice site, relative to PR-A. Treatment with BL also increased expression of PR mRNA in all of the granulosa layers of follicles, while treatment with GL increased expression of PR mRNA in granulosa layers of SYF(small yellow follicle), F5 and F1. These results indicate that blue and green monochromatic lights promote egg production traits via stimulating gonadal hormone secretion and up-regulating expression of ERs and PRs. Changes in PR-B protein suggest that this form of the progesterone receptor is predominant for progesterone action in the granulosa layers of preovulatory follicles in chickens during light stimulation.