共查询到20条相似文献,搜索用时 15 毫秒
1.
[目的] 进一步探讨牛磺鹅去氧胆酸(taurochenodeoxycholic acid,TCDCA)在抗炎免疫方面的潜在调节作用。[方法] 以AA大鼠成纤维样滑膜细胞作为研究对象,采用ELISA方法检测TCDCA和IL-1β作用下AA大鼠成纤维样滑膜细胞上清液中PGE2的含量,分析TCDCA对IL-1β刺激下AA大鼠成纤维样滑膜细胞中PGE2分泌情况的影响。[结果] TCDCA能够对IL-1β刺激下AA大鼠纤维样滑膜细胞PGE2的分泌产生下调作用(P<0.05)。[结论] TCDCA对IL-1β刺激下AA大鼠成纤维样滑膜细胞中PGE2的分泌具有抑制作用,为TCDCA在兽医临床应用提供依据。 相似文献
2.
To determine the absorption and metabolism of 17β-estradiol (E2) by the rectum of the pig, 10 mg of crystalline E2 was placed in the rectum of prepubertal gilts in Experiment 1. Blood samples were subsequently obtained from hepatic portal and jugular veins and plasma was assayed for E2, estrone (E1), 17β-estradiol-glucuronide (E2G), estrone-glucuronide (E1G) and estrone-sulfate (E1S). Concentration of E2, E1, E2G, E1G, and E1S rose in the hepatic portal vein within 30 min and remained elevated for several hr. Concentrations of E2 in the hepatic portal vein represented 3% of the total estrogen detected in the hepatic portal vein during the 5 hr sampling period, indicating that most of the E2 was metabolized prior to entering the hepatic portal vein after absorption by the rectal mucosa. Concentrations of E2, E1, E2G, E1G, and E1S rose in the jugular vein and remained elevated for several hr. The rise in E2 and E1 in the jugular vein may have come from E2 and E1 in venous circulation from the rectum that entered the inferior vena cava bypassing the hepatic portal vein and liver. The net result of absorption of E2 from the rectum of gilts was a large rise in unconjugated and conjugated E2 and E1 in the peripheral circulation. In Experiment 2 prepubertal gilts fitted with jugular, hepatic portal, duodenal, and gall bladder catheters were infused into the duodenum with bile from pregnant gilts. Concentrations of E2, E1, E2G, and E1G were determined in gallbladder bile of gilts before infusion and at 470 min. Concentrations of E2G and E1G were determined in hepatic portal and jugular plasma before and after infusion of bile. A cholagogue was given at 480 min and E2G and E1G were measured in plasma from 490 min to 960 min. Concentrations of E2 and E1 in gallbladder bile rose at 470 min and fell to basal concentrations at 970 min. In gilts given the cholagogue, E2G and E1G in both the jugular and hepatic portal veins rose significantly over those in gilts not given the cholagogue. Bile estrogens circulate via the enterohepatic route and factors that influence secretion of estrogens in bile can influence concentrations of circulating estrogens. 相似文献
3.
Roberto da Costa RP Ferreira-Dias G Mateus L Korzekwa A Andronowska A Platek R Skarzynski DJ 《Domestic animal endocrinology》2007,32(4):287-302
Nitric oxide (NO) plays an important role in angiogenesis and in the regulation of the blood flow. This study was carried out to investigate (i) the effects of endogenous estrogens and progestins and exogenous progesterone (P4) (5 ng/ml or 1 μg/ml) or estradiol 17β (E2β) (50 pg/ml or 1 μg/ml) on in vitro endometrial NO synthesis; (ii) the presence of different isoforms of NO synthase; (iii) and their relationship to microvascular density in the equine endometrium during the estrous cycle. NOS expression was also evaluated in the myometrium. Expression of endothelial and inducible forms of NOS in the uterus was assessed by Western blot and immunocytochemistry. Vascular density in endometrial tissue was determined on histologic sections. In the luteal phase, compared to the follicular phase, endometrial NO production increased without exogenous hormones and with exogenous E2β (1 μg/ml). Although immunocytochemistry revealed iNOS and eNOS expression in the endometrium, no positive signal for iNOS was detected by Western blot. Endothelial NOS was observed in endometrial glands, endothelial cells, fibroblasts, blood and lymphatic vessels. Endometrial eNOS expression was the highest in the follicular and mid-luteal phases while it was found to be the lowest in the early luteal phase. In the follicular phase, hyperplasia of endometrial tissue with respect to myometrium was detected. No difference in vascular density was present between phases. All together, NO may play some roles in both proliferative and secretory phases of endometrial development in the mare. 相似文献
4.
Prostaglandin E2 (PGE2) and stromelysin are produced by equine chondrocytes and synovial cells in vitro in response to recombinant human (rh) interleukin-1 (IL-1) alpha and beta, and equine mononuclear cell supernatants (MCS) containing IL-1. However, culture conditions are important. PGE2 concentrations increase in proportion to the concentration of fetal calf serum (FCS) in the culture medium, whereas stromelysin concentrations are inversely proportional to the concentration of FCS. Equine MCS, containing a lower concentration of IL-1 than the concentration of rhIL-1 used in these experiments, stimulated production of much higher levels of PGE2 than rhIL-1. In addition, equine MCS induced the production of broadly similar levels of PGE2 by both chondrocytes and synovial cells, whereas rhIL-1 was more active on equine synovial cells than equine chondrocytes. Although equine MCS induced both stromelysin and PGE2 production by equine articular cells, on the whole rhIL-1 failed to induce stromelysin production. This supports previous observations of species restrictions in the activity of human IL-1 on equine cells. Therefore, experiments using mammalian cells and heterologous IL-1 should be interpreted with caution. 相似文献
5.
Three experiments were performed to study effects of decreased concentrations of estradiol-17β (E2) on lifespan and function of ensuing ovine corpora lutea (CL). In experiment 1, 52 follicles were collected from 10 ewes and placed into individual culture with 0 or .01 μCi 3H-androstenedione (10 ng; 3H-A) and 0, 10−11, 10−9, 10−7, or 10−5 M of a nonsteroidal aromatase inhibitor, CGS16949A (CGS). Concentrations of E2 secreted into the medium, and synthesis of estrogens as estimated by formation of 3H-water from 3H-A were decreased by 10−5 and 10−7 (P<.01), but not 10−9 or 10−11 M CGS. In experiment 2, luteolysis was induced in 24 ewes by injection of PGF2 on days 5 to 10 of the estrous cycle (0 hr). Ewes received 0, 0.5, 1.0, 2.0 or 4.0 mg CGS per kg BW i.v. at −12, 0, 12 and 24 hr, and an ovulatory dose of hCG at 36 hr. Jugular (P<.001) and vena caval (P<.001) concentrations of E2 were decreased by CGS at all doses tested for 8 to 10 hr, but had returned to levels similar to control ewes by the time of the next injection. Concentrations of E2 around the time of the LH surge were similar in control and treated ewes. During the subsequent luteal phase, concentrations of progesterone (P4) were similar in control and treated ewes. Thus, transient decreases in E2 during the follicular phase were not deleterious to the subsequent luteal phase. In experiment 3, luteolysis was induced in 18 ewes by injection of PGF2 on days 6 or 7 (0 hr) of the estrous cycle. Ewes received 0 or 1 mg CGS per kg BW i.v. every 8 hr from 0 to 40 hr. Ovulation was induced with hCG at 36 hr. CGS reduced jugular (P<.001) and vena caval (P<.001) concentrations of E2, prevented an endogenous surge of LH (P<.05) and increased (P<.001) concentrations of FSH. All ewes had ovulated a marked follicle by 72 hr, but onset of the luteal phase, as assessed by concentrations of P4, was delayed (P<.01) in ewes receiving CGS. Delayed luteal phases were not solely attributable to the presence of new CL or to luteinization of follicular cysts. When data were aligned according to the day ewes were observed in estrus, profiles of P4 did not differ with treatment. Therefore, normal luteal function ensued following estrus whether or not ewes re-ovulated. In conclusion, decreased secretion of E2 by the preovulatory follicle was not involved in the ontogeny of CL of short lifespan or subnormal function. Instead, adequate production of E2 or precisely timed E2 secretion may be required during follicular development for subsequent functional luteinization. 相似文献
6.
Yoon MJ Boime I Colgin M Niswender KD King SS Alvarenga M Jablonka-Shariff A Pearl CA Roser JF 《Domestic animal endocrinology》2007,33(4):470-479
The objectives of this study were to determine the efficacy of recombinant equine luteinizing hormone (reLH) in shortening the time to ovulation in cycling mares and to determine the effects of treatment on endogenous hormones and inter-ovulatory intervals. In study 1, mares of light horse breeds (3–20 years) were treated with either a vehicle, various doses of reLH, or human chorionic gonadotropin (hCG). Cycling mares were examined by palpation and ultrasound per rectum daily or every 12 h from the time of treatment to ovulation. In studies 2 and 3, jugular blood samples were collected daily or every 12 h from the time of treatment to ovulation for analysis of LH, follicle stimulating hormone (FSH), estradiol-17β (E2), and progesterone (P4) by radioimmunoassays (RIA). Increasing doses of reLH (0.3, 0.6, 0.75, and 0.9 mg) showed increasing effectiveness at inducing ovulation within 48 h of treatment. Treatments with the 0.75 and 0.9 mg doses of reLH resulted in 90% and 80% ovulation rates, which were similar to hCG treatment (85.7%). Except for the early rise in LH after treatment with 0.5, 0.65, and 1.0 mg of reLH, hormone profiles appeared to be similar between control and treated cycles. Inter-ovulatory intervals were similar between control and treatment cycles. In conclusion, reLH is a reliable and effective ovulatory agent that does not significantly alter endogenous hormone profiles or affect inter-ovulatory intervals. 相似文献
7.
为研究胸腺上皮细胞(thymic epithelial cells,TECs)中雌激素(estradiol,E2)对长链非编码RNA(long non-coding RNA,lncRNA)表达的调节作用,本研究首先培养小鼠胸腺髓质上皮细胞系1(medullary thymic epithelial cell line 1,MTEC1),经50 nmol/L E2作用24 h后,观察对细胞表型变化的影响,并用CCK-8试剂盒检测细胞活力;提取细胞总RNA,运用实时荧光定量PCR技术验证E2对lncRNA-2410006H16Rik表达的调节作用;最后运用RT-PCR技术扩增其目的基因,构建pEGFP-N1-lncRNA-2410006H16Rik重组过表达载体。结果显示,50 nmol/L E2能够明显抑制MTEC1的增殖,且相较于对照组细胞,50 nmol/L E2处理组细胞的D450 nm值极显著降低(P<0.01),表明其细胞活力极显著下降。实时荧光定量PCR结果显示,在E2作用下,lncRNA-2410006H16Rik在MTEC1细胞中的表达极显著上调(P<0.01),约是对照组的2倍,与高通量测序结果一致。经RT-PCR、双酶切及测序结果分析显示,试验成功构建pEGFP-N1-lncRNA-2410006H16Rik表达载体。结果表明,TECs中lncRNA-2410006H16Rik的表达与E2作用密切相关,为后续在细胞水平上进一步验证lncRNA-2410006H16Rik的调节功能奠定了基础。 相似文献
8.
Nielsen MO Nyborg S Jakobsen K Fleet IR Nørgaard J 《Domestic animal endocrinology》2004,27(4):345-362
Mammary arterious − venous differences (A − V) and excretion into milk of four prostanoids were related to changes in milk yield and milk vein blood velocity (MBV) in goats at different stages of pregnancy and lactation, and during somatotropin (ST) treatment in mid-lactation. Arterial concentrations and mammary A − V for the vasodilators prostacyclin (PGI2) and prostaglandin (PG) E2 (measured as 6-keto-PGF1 and bicyclic PGE2, respectively) decreased from late pregnancy to lactation. A − V were negatively correlated to MBV (r = −0.32 to −0.34). Arterial concentrations of the vasoconstrictors PGF2 and TXA2 (measured as TXB2) changed similarly, but no A − V across the mammary gland were found. The vasodilator to vasoconstrictor ratio in plasma was around 1:1, and in skimmed milk around 0.29–0.49 due to significantly higher TXB2 levels in milk compared to plasma. Close linear correlations were established between milk yield and excretion of TXB2 into milk (r = 0.80, P < 0.001), and between MBV and PGE2 excretion into milk (r = 0.69, P < 0.001). ST treatment stimulated MBV and mammary prostanoid supply, and decreased prostanoid concentration in milk vein plasma. The high arterial levels of prostaglandins during pregnancy most likely reflected uterine synthesis. Our results support a role for PGI2 and PGE2 in local mammary blood flow regulation during lactation. Increased mammary uptake of these two prostanoids may be involved in the mammary blood flow response to ST. TXA2 may be synthesized by mammary epithelial as well as vascular cells, and TXA2 may be an important factor in regulation of mammary function. 相似文献
9.
Two experiments were conducted in order to determine the effects of estradiol (E2) on the development of the hypothalamic-pituitary-testicular axis in bull calves. In experiment 1, calves were assigned randomly to one of the following groups: 1) intact, 2) intact E2-treated, 3) castrated, or 4) castrated E2-treated. Treatments began when the calves were 7.5 wk of age and continued for 16.5 wk. Samples of blood were collected once a week from 3 to 14 wk of age and every 10 min for 6 hr at 8, 12 and 16 wk of age. Concentrations of E2 in plasma decreased between 3 and 4 wk of age and were further reduced by castration. Maximum concentrations of E2 (24.3 pg/ml) were observed 72 hr after insertion of E2 implants, however, plasma E2 stablized at 5–9 pg/ml by 2 wk after insertion of implants. Treatment with E2 eliminated the pulsatile secretion of LH in intact and castrated calves and retarded testicular growth. In experiment 2, calves were assigned to a control (n=4) or E2-treated (n=6) group. Implants of E2 were inserted at 7.5 wk of age. At 24 wk of age, calves were bled and then sacrificed to collect hypothalamic and pituitary tissues. Age-related changes in testicular weight and secretion of LH were blocked by E2. Neither the morphology nor the intensity of immunostaining of GnRH nerve cell bodies in the preoptic area (POA) were affected by E2. However, the density of GnRH fibers and beads in the stalk median eminence (SME), and concentrations of pituitary GnRH receptors were greater (P<.01) in E2-treated compared to control calves. In addition, concentrations of norepinephrine (NE) in the SME were lower in E2-treated calves when compared to controls. Based on these observations, it is concluded that administration of E2 at 7.5 wk of age causes profound alterations in hypothalamic function including, changes in metabolism of NE and suppression of GnRH release. 相似文献
10.
J.E. Kinder M. Garcia-Winder K. Imakawa M.L. Day D.D. Zalesky M.L. D''Occhio T.T. Stumpf R.J. Kittok B.D. Schanbacher 《Domestic animal endocrinology》1991,8(4):463-469
The objective of the research was to determine the relationship between circulating 17β-estradiol (E2) and secretion of luteinizing hormone (LH) in cows. A second objective was to determine if response to E2 was influenced by interval between ovariectomy and the start of E2 treatment. Thirty-one nulliparous cows 3 yr of age were randomly assigned to a 2 × 4 factorial arrangement of treatments. Sixteen cows were ovariectomized at 18 mo of age (long term), and the other 15 cows were ovariectomized at 36 mo of age (short term). At the time of ovariectomy of cows in the short term group, 11 cows in the short term group and 12 cows in the long term group were implanted subcutaneously with 1, 2 or 4 polydimethylsiloxane capsules containing E2. The other eight cows served as non-implanted controls (n=4-short term, n=4-long term). All cows were fitted with jugular vein catheters on day 29 of treatment, and on day 30 blood samples were collected at 12-min intervals for 6 hr. At the end of 6 hr, luteinizing hormone-releasing hormone (LHRH) was administered and blood sampling continued at 12-min intervals for an additional hour. Serum was analyzed for LH and E2. Variables of LH secretion analyzed were mean concentration, frequency of pulses, amplitude of pulses and maximum concentration after LHRH. There were no significant interactions for any of the variables of LH among cows ovariectomized for the long and short term. There was a significant linear increase in mean concentration of LH with increased circulating concentration of E2. Frequency of LH pulses was not affected by circulating concentration of E2. As circulating concentration of E2 increased, amplitude of LH pulses increased and response to LHRH increased - resulting in an increase in mean LH. Interval from time of ovariectomy to the start of E2 treatment only had a minor influence on mean concentration of LH and profile of LH concentrations in circulation. 相似文献
11.
12.
For optimizing in vitro maturation system of bovine oocytes,we firstly examined the influence of four different hormonal regimes(FSH+LH,HMG,FSH+LH+E2 and HMG+E2) on oocyte maturation rates.Then we studied the effects of epidermal growth factor (EGF) in the above defined medium on bovine oocyte maturation,in vitro development and quality of parthenogenetic embryos.The cell apoptotic index of parthenogenetic blastocysts was detected by TUNEL.No significant difference was observed in maturation rates in four groups supplemented with different hormones.However,human menopausal gonadotropin (HMG) provided steady maturation results in replicates.Maturation of oocytes was promoted by supplementation with 17β-estradiol (E2).Combination of HMG and E2 gave rise to steady and efficient mature results.The presence of EGF at 30 ng/mL concentration significantly increased maturation rate and blastocyst rate and reduced apoptotic cells in parthenogenetic blastocysts.Therefore,the optimal oocyte maturation solution could be supplemented with 0.075 IU/mL HMG,1 μg/mL E2 and 30 ng/mL EGF. 相似文献
13.
为建立敏感、特异、快速的雌二醇(estradiol,E2)残留免疫检测方法,本研究利用雌二醇人工抗原(E2-BSA)免疫BALB/c小鼠,应用淋巴细胞杂交瘤技术制备特异性雌二醇单克隆抗体,利用高效价、高特异性单克隆抗体建立间接竞争ELISA(icELISA)方法。结果显示,试验成功筛选获得一株稳定分泌抗雌二醇抗体的杂交瘤细胞株(3H3),抗体效价可达1∶320 000,利用3H3腹水抗体优化间接竞争icELISA反应条件,检测抗体的敏感度,IC50为1.636 ng/mL,IC20~IC80线性范围为0.202~13.281 ng/mL。雌二醇腹水抗体与雌三醇、乙炔雌二醇的交叉反应率分别达0.31%和0.25%,而与雌酮、戊酸雌二醇、苯甲酸雌二醇、炔雌醚、己烯雌酚、壬基酚的交叉反应率均<0.1%。结果表明,利用本研究制备的单克隆抗体建立雌二醇间接竞争ELISA检测方法,可满足食品中雌二醇残留高灵敏度的检测要求。 相似文献
14.
BAI Yu HU Jing-yan XU Yong-peng HE Jie JIN Jun-jie LI Pei-de LIU Su-zhen 《中国畜牧兽医》2017,44(10):3100-3105
In order to establish a sensitive,specific and rapid method for the detection of estradiol (E2) residues, an indirect competitive enzyme-linked immunosorbent assay (icELISA) based on monoclonal antibody (MAb) for E2 was developed. BALB/c mice were immunized by E2-BSA and cell fusion technology was employed to screen hybridoma cell lines. One hybridoma cell line (3H3) was isolated, which produced monoclonal antibody that could binding E2. Under the optimized conditions, the icELISA based on 3H3 for E2 showed a half maximum inhibition concentration (IC50) values of 1.636 ng/mL and detection ranges of 0.202 to 13.281 ng/mL with cross-reactivities for estriol and ethinyloestradiol of 0.31% and 0.25%, respectively, and negligible cross-reactivities with other E2 analogs including estrone, estradiol valerate, estradiol benzoate, quinestrol, diethylstilbestrol and nonylphenol. The results demonstrated that the developed method could meet the requirements of high sensitivity detection of E2 residue in food samples. 相似文献
15.
试验旨在研究不同激素配比及表皮生长因子(EGF)浓度对牛卵母细胞体外成熟及卵母细胞质量的影响。将随机分组的卵丘-卵母细胞复合体于添加FSH+LH、HMG、FSH+LH+E2、HMG+E2 4种不同激素组合配比的成熟基础液中培养,对比其体外成熟率,比较了EGF对牛卵母细胞体外成熟率和孤雌胚胎体外发育的影响,并采用TUNEL法检测添加不同浓度EGF的牛孤雌激活囊胚细胞凋亡情况。结果表明,添加HMG的成熟试验结果稳定,E2对牛卵母细胞成熟有一定的促进作用,HMG+E2联合使用可以得到高效稳定的成熟结果;在此基础上,在成熟液中添加30 ng/mL EGF对牛卵母细胞的成熟质量、胚胎发育及降低胚胎细胞凋亡都有明显的促进作用。因此,在体外成熟培养液中添加0.075 IU/mL HMG、1 μg/mL E2和30 ng/mL EGF对牛卵母细胞的成熟和质量较为有益。 相似文献
17.
18.
旨在探究双氢睾酮(dihydrotestosterone,DHT)是否通过调节孕酮(progesterone,P4)、雌二醇(oestrogen,E2)和细胞凋亡参与影响绵羊子宫功能,以揭示其在绵羊生殖生理中的潜在作用。本试验以1.5岁左右的雌性小尾寒羊为试验动物,检测卵泡期、黄体期和妊娠期子宫中DHT合成酶和雄激素受体(androgen receptor,AR)的表达变化。随后,体外培养绵羊子宫内膜上皮细胞,并用DHT (10-10~10-7 mol·L-1)和AR拮抗剂氟他胺(Flu,10-8 mol·L-1)处理(n=3)。通过酶联免疫吸附试验、细胞免疫荧光、蛋白质印迹法和实时荧光定量PCR检测P4和E2水平、合成酶和受体表达。此外,还检测经DHT和Flu处理后,绵羊子宫内膜上皮细胞中凋亡因子Bcl-2相关X蛋白(Bcl-2-associated X protein,Bax)、B细胞淋巴瘤蛋白2(B cell lymphoma protein 2,Bcl-2)、半胱天冬酶3(caspase 3,CASP3)和活化半胱天冬酶3(active-caspase 3,Act-CASP3)的表达变化。结果表明,绵羊子宫不同时期DHT的合成和AR的表达存在差异,妊娠期子宫DHT合成及AR表达显著低于卵泡期和黄体期(P<0.05)。10-10~10-7 mol·L-1DHT处理后,P4合成酶表达显著上调(P<0.05),在10-8~10-7 mol·L-1 DHT时P4合成显著增加(P<0.05),在10-10~10-8 mol·L-1 DHT时孕酮受体蛋白表达显著增加(P<0.05),但10-7mol·L-1 DHT时孕酮受体蛋白表达显著下降(P<0.05);在10-8~10-7 mol·L-1 DHT时E2相关合成酶显著减少,并且E2水平显著下降(P<0.05),在10-9和10-7 mol L-1 DHT时E2受体ERα蛋白显著下调(P<0.05),在10-10~10-7 mol·L-1 DHT时ERβ和GPER显著增加(P<0.05)。经Flu处理后部分解除DHT对P4和E2的调控。此外,10-10~10-7 mol·L-1 DHT显著促进子宫内膜上皮细胞凋亡(P<0.05)。本研究证实DHT至少部分通过AR调节P4和E2合成及受体表达,影响细胞凋亡,参与调节子宫功能,这为进一步阐明雄激素参与调节子宫功能提供了新的基础和相关数据。 相似文献
19.
ZHAO Xi NURIBIYAMU&# Maimaitituoheti SONG Yukun AIRIXIATI&# Dilixiati ZHANG Bo AERMAN&# Haire ABULIZI&# Wusiman 《中国畜牧兽医》2007,47(10):3289-3296
The purpose of this study was to investigate the effect of growth differentiation factor 9 (GDF9) on the gene expression of cumulus cells expansion and hormone receptors as well as hormone secretion,in order to provide evidence for the role of GDF9 in the development of sheep cumulus cells.Sheep cumulus cells were used as the research object in this study,and were cultured for 48 h by adding different concentrations (0,50,100,200,400 ng/mL) GDF9 to low serum cell culture medium.Total RNA were extracted from the cells,using β-actin as the reference gene,Real-time quantitative PCR technology were used to detect the cumulus cells expansion related genes hyaluronic acid synthase gene 2 (HAS2),prostaglandin lead oxide synthase 2 (PTGS2),pentraxin 3 (PTX3) and hormone receptor genes follicle-stimulating hormone receptor (FSHR),luteinizing hormone receptor (LHR) and estrogen receptors (E2R).Using the enzyme-linked immunosorbent assay (ELISA) method to test the content of E2 and P4.The results showed that HAS2,PTX3,FSHR,E2R and LHR mRNA relative expression of 200 ng/mL GDF9 group was extremely significantly higher than the control group and other GDF9 groups (P<0.01),PTGS2 mRNA relative expression was extremely significantly higher than the control group and 50,400 ng/mL GDF9 groups (P<0.01),and significantly higher than 100 ng/mL GDF9 group (P<0.05).When added 400 ng/mL GDF9,the relative mRNA expression of all the mentioned-above genes were all extremely significantly lower than that of the 200 ng/mL GDF9 group.Moreover,the E2 secretion level was extremely significantly higher than that of the control group and 50 ng/mL GDF9 group (P<0.01),significantly higher than that of the 100 ng/mL GDF9 group(P<0.05),while had no significant difference from the 200 ng/mL GDF9 group (P>0.05).When added 100,200 and 400 ng/mL GDF9,the concentration of P4 was significantly higher than the control group (P<0.05),and there was no significant difference from the 50 ng/mL group (P>0.05),and there was no significant difference between 100,200 and 400 ng/mL GDF9 groups (P>0.05).To sum up,GDF9 could promote the expansion of sheep cumulus cells and participated in the regulation of hormone secretion of sheep cumulus cells. 相似文献
20.
本试验旨在探究生长分化因子9(GDF9)对卵丘细胞扩展相关基因和激素受体基因表达量及激素分泌的影响,为GDF9在绵羊卵泡发育中的作用提供依据。以绵羊卵丘细胞为研究对象,通过在低血清细胞培养液中添加不同浓度(0、50、100、200、400 ng/mL)的GDF9,培养绵羊卵丘细胞48 h后,提取细胞总RNA,利用实时荧光定量PCR技术,以β-actin为内参基因,检测卵丘细胞扩展相关基因透明质酸合酶2(HAS2)、前列腺素内过氧化物合酶2(PTGS2)、穿透素3(PTX3)及激素受体相关基因卵泡刺激素受体(FSHR)、促黄体生成素受体(LHR)和雌激素受体(E2R)的mRNA相对表达量;利用酶联免疫吸附法(ELISA)测定培养液中卵丘细胞分泌的雌二醇(E2)和孕酮(P4)含量。结果显示:在细胞培养液中添加200 ng/mL GDF9时,HAS2、PTX3、FSHR、E2R和LHR的mRNA相对表达量极显著高于对照组与其他处理组(P<0.01);PTGS2 mRNA相对表达量极显著高于对照组、50和400 ng/mL GDF9组(P<0.01),显著高于100 ng/mL GDF9组(P<0.05)。当添加400 ng/mL GDF9时,各基因mRNA相对表达量均极显著低于200 ng/mL GDF9组(P<0.01);E2分泌量极显著高于对照组与50 ng/mL GDF9组(P<0.01),显著高于100 ng/mL GDF9组,与200 ng/mL GDF9组差异不显著(P>0.05)。100、200和400 ng/mL GDF9组P4分泌量显著高于对照组(P<0.05),与50 ng/mL GDF9组没有显著差异(P>0.05),且3组之间差异不显著(P>0.05)。综上所述,GDF9能够促进绵羊卵丘细胞扩展,并参与绵羊卵丘细胞激素分泌的调控。 相似文献