c-erbB_2对大鼠黄体细胞hCG诱导的孕酮分泌的影响

采用离体细胞体外孵育法 ,研究反义c erbB2 寡脱氧核苷酸 (antisensec erbB2 ODN)对大鼠黄体细胞hCG诱导的孕酮分泌的影响 ,及其与外源性cAMP和Ca2 以及蛋白抑制剂放线菌酮 (CYX)之间的关系。结果表明 ,反义c erbB2 以剂量相关方式抑制黄体细胞hCG诱导的孕酮的产生 ,同时使c erbB2 蛋白染色阳性的黄体细胞百分数下降 ,无义tatODN没有相应的作用。10 -4 mol/L的二丁酰cAMP能明显反转反义c erbB2 ODN对孕酮产生和c erbB2 表达的抑制作用 ,钙离子通道阻断剂维拉帕米和蛋白抑制剂CYX对此抑制作用有协同效应。该实验说明c erbB2 参于hCG诱导黄体细胞生孕酮作用     

反义c—fos寡脱氧核苷酸对hCG诱导大鼠黄体细胞孕酮和雌二醇生成的 …

采用离体孵育大鼠黄体细胞的方法,观察了反义ｃ－ｆｏｓ寡脱氧核苷酸（反义ｃ－ｆｏｓＯＤＮ）对ｈＣＧ诱导的黄体细胞孕酮（Ｐ）和雌二醇（Ｅ２）产生的影响,同时观察了外源性ｃＡＭＰ和钙离子通道阻断剂维拉帕米对黄体细胞中ｃ－ｆｏｓ蛋白的影响。结果发现,反义ｃ－ｆｏｓＯＤＮ能呈剂量相关方式抑制ｈＣＧ诱导的黄体细胞Ｐ和Ｅ２的产生,同时使ｃ－ｆｏｓ蛋白染色阳性的黄体细胞百分数下降;而无义ｔａｔ ＯＤＮ没有相应的作     

c—erbB2对大鼠黄体细胞hCG诱导的孕酮分泌的影响

采用离体细胞体外孵育法,研究反义ｃ－ｅｒｂＢ２寡脱氧核苷酸（ａｎｔｉｓｅｎｓｅ ｃ－ｅｒｂＢ２ ＯＤＮ）对大鼠黄体细胞ｈＣＧ诱导的孕酮分泌的影响,及其与外源性ｃＡＭＰ和Ｃａ＾２＋以及蛋白抑制剂放线菌酮（ＣＹＸ）之间的关系。结果表明,反义ｃ－ｅｒｂＢ２以剂量相关方式抑制黄体细胞ｈＣＧ诱导的孕酮的产生,同时使ｃ－ｅｒｂＢ２蛋白染色阳性的黄体细胞百分数下降,无义ｔａｔ ＯＤＮ没有相应的作用。１０＾－４     

c-fos、c-myb和c-erbB-2与大鼠卵巢颗粒细胞生孕酮调控关系的研究

目的和方法:用离体细胞体外孵育法,观察反义c-fos、c-myb和c-erbB-2 寡脱氧核苷酸(c-fos ODN、c-myb ODN和c-erbB-2 ODN)对hCG诱导大鼠颗粒细胞孕酮产生的影响,同时观察内皮素-1、γ-氨基丁酸和钙离子通道阻断剂维拉帕米对颗粒细胞中c -fos、c-myb和c-erbB-2蛋白的影响.结果:反义c-fos、c-myb和c-erbB -2 ODN均明显抑制hCG诱导颗粒细胞孕酮的产生,并伴有各自癌基因蛋白染色阳性的颗粒细胞百分率下降;而无义tat ODN没有相应的作用.2×10-7mol/L内皮素-1和5×10 -6mol/L γ-氨基丁酸能显著抑制hCG诱导颗粒细胞孕酮的产生,同时使c-fos、c-my b和c-erbB-2蛋白染色阳性的颗粒细胞百分率下降;而1×10-6mol/L维拉帕米对hCG 诱导颗粒细胞孕酮的产生和c-fos、c-myb和c-erbB-2蛋白染色阳性的颗粒细胞百分率均无明显影响.结论:c-fos、c-myb和c-erbB-2与hCG诱导颗粒细胞孕酮的产生密切相关;内皮素-1、γ-氢基丁酸能通过调节这些癌基因在颗粒细胞中的表达而影响hCG诱导颗粒细胞孕酮的产生;而Ca2+无相应的作用.     

大鼠卵巢不同功能阶段时c-fos表达的动态变化

目的和方法：本文用免疫组织化学方法检测了成年大鼠卵巢于不同的功能阶段和未成年大鼠外源性激素诱导的卵巢于不同的功能阶段c-fos表达的变化以及与血清E2和P含量的相关关系。结果：在成年大鼠动情前期、动情期卵巢的间质腺和基质中及动情间期和妊娠期卵巢的黄体细胞和基质中有c-fos表达,c-fos蛋白阳性信号的表达范围和表达强度在动情前期卵巢较大,动情间期和动情期卵巢较低,妊娠期卵巢最大,这种变化与血清E2和P含量的变化呈明显的正相关关系。未成年大鼠,用DES使卵泡发育至窦前期时,在卵巢中未检测到有c-fos蛋白的表达,用PMSG使贸泡发育至排卵前期时在卵巢的间质腺和基质中有c-fos表达,用PMSG和hCG后4天形成的早期黄体化卵巢c-fos在黄体细胞和基质中的表达明显升高,而于用hCG后9天形成的晚期黄体化卵巢c-fos表达明显下降,这种变化也与血清E2和P含量的变化呈明显的正相关关系。结论：c-fos与卵泡发育、排卵、黄体形成和退化等功能密切相关。     

血小板活化因子对大鼠黄体细胞孕酮分泌及血管内皮生长因子表达的作用

本文旨在研究血小板活化因子(platelet-activating factor,PAF)对大鼠黄体细胞孕酮分泌及血管内皮生长因子(vascularendothelial growth factor,VEGF)mRNA表达的作用.将未成年(25～28 d)Sprague-Dawley雌性大鼠颈部皮下注射50 IU孕马血清促性腺激素(pregnant mare serum gonadotrophin,PMSG),48 h后注射25 IU人绒毛膜促性腺激素(human chorionicgonadotrophin.hCG)诱导卵泡发育和黄体生成,第6天(hCG注射日为第1天)收集卵巢黄体细胞,体外培养24 h后,不加或加入不同剂量(0.1 μg/mL、1 μg/mL、10 μg/mL)PAF,37℃、5%CO2培养箱内培养24 h.用放射免疫方法测定培养液中孕酮的含量,流式细胞仪和RT-PCR方法检测黄体细胞凋亡以及VEGF mRNA的表达.结果显示,PAF促进黄体细胞孕酮分泌,1 μg/mL PAF作用最强(P<0.05);PAF促进黄体细胞凋亡无明显剂量依赖性,但10 μg/mL PAF显著促进大鼠黄体细胞凋亡(P<0.05):PAF刺激黄体细胞VEGF mRNA表达,1 μg/mL PAF效果最显著(P<0.01).结果提示,PAF可通过调节黄体细胞孕酮的分泌和VEGF mRNA的表达来促进黄体形成.     

血管活性肠肽对肺表面活性物质结合蛋白A表达的影响

目的:研究血管活性肠肽(VIP)对肺表面活性物质结合蛋白A(SP-A)表达的影响以及VIP调控SP-A表达的细胞内信号转导途径.方法:运用免疫组织化学和RT-PCR技术研究VIP对SP-A表达的影响;并进一步运用受体拮抗、蛋白激酶抑制、反义寡核苷酸阻断等手段探讨VIP促进SP-A表达的信号转导途径.结果:①VIP(10-8mol/L)促进肺泡Ⅱ型细胞(ATⅡ)细胞中的SP-A蛋白表达和提高肺组织SP-AmRNA含量:②VIP受体拮抗剂(10-6mol/L)可取消VIP(10-8mol/L)促进SP-A表达的效应;③蛋白激酶C抑制剂H7(10-5mol/L)和c-fos基因的反义寡核苷酸(9×10 6mol/L)均可阻断VIP促进SP-A表达的作用.结论:VIP通过其受体促进SP-A的表达,PKC及c-fos蛋白在介导VIP促进SP-A表达的细胞内信号转导过程中起重要作用.     

反义c－fos和c－jun抑制IL－1诱导阿片肽分泌

白细胞介素-1(IL-1)及阿片肽作为神经调质参与了神经细胞兴奋性毒性作用.以大鼠大脑皮层神经细胞为研究对象,探讨了IL-1、阿片肽和c-fos、c-jun表达产物之间的关系.结果表明,IL-1β能诱导大脑皮层神经细胞c-fos、c-jun mRNA瞬时短暂表达,15min增高,30min达高峰,c-fos mKNA 2h回至基线水平,c-jun mRNA 8h回至基线水平;联合应用c-fos、c-jun反义寡核苷酸能部分抑制IL-1诱导的大脑皮层神经细胞脑啡肽及β-内啡肽分泌增加,呈一定量效关系,相应意义寡核苷酸无抑制作用.提示IL-1促进大脑皮层神经细胞脑啡肽及β-内啡肽分泌作用部分受Fos和Jun蛋白调控.     

~3H-酪氨酸与大鼠离体黄体细胞的结合

用孕马血清促性腺激素和hCG处理25—28d龄未成年雌性大鼠,造成超排卵并形成黄体,取hCG处理后7d的黄体制备黄体细胞。将黄体细胞与~3H-酪氨酸一起孵育(24℃,45min)后,~3H-酪氨酸能与黄体细胞特异结合,~3H-酪氨酸浓度为7.5μmol/L时达到饱和,在4℃孵育10min条件下仍有~3H-酪氨酸的结合。用哇巴因抑制酪氨酸向细胞内的转运后,~3H-酪氨酸的特异结合依然存在,放线菌酮也不能影响~3H-酪氨酸结合。这些结果证明,酪氨酸能与黄体细胞特异结合,并提示酪氨酸的结合位点存在于细胞膜上。     

Na~+、K~+离子通道阻滞剂对离体大鼠黄体细胞孕酮生成的影响

本工作用二种离子通道阻断剂四乙胺(TEA)和河豚毒素(TTX)来研究 Na~+、K~+通道的改变对大鼠黄体细胞孕酮生成的影响。10~(-3)mol/L 的 TEA 或 TTX 均使孕酮分泌量显著增加,而这种促进效应可被酪氨酸(Tyr)完全阻断。Tyr 对 TEA 或 TTX 与 hCG 联合所引起的孕酮分泌也有抑制作用。上述实验说明跨黄体细胞内外的 K~+和 Na~+浓度差与孕酮分泌有关。     

c-myb对人绒毛膜促性腺激素诱导的大鼠睾丸间质细胞睾酮分泌的影响

采用离体细胞体外孵育法,观察反义c-myb寡脱氧核苷酸(oligodeoxynucletides,ODN)对人绒毛膜促性隙激素(humanchorionic-gonadotropin hormone,hCG)诱导的人鼠间质细胞睾酮分泌的影响,并进一步探讨了外源性二丁酰cAMP(dbcAMP)、Ca^2 以及蛋白质抑制剂放线菌酮(cycloheximide,CYX)对间质细胞中c-Myb蛋白表达和睾酮分泌的作用。结果表明,反义c-myb ODN呈剂量依赖性地抑制hCG诱导的离体间质细胞的睾酮分泌,同时使间质细胞中c-Myb蛋白免疫组化染色下降：而无义tat ODN没有相应的作用。100μmol／L的dbc AMP可进一步促使hCG秀导的间质细胞分泌睾酮,并且使间质细胞中c-Myb蛋白免疫组化染色IOD值升高,与hCG组相比,具有统计学意义。钙离子通道阻断剂维拉帕米(10μmol／L)和蛋白质抑制剂放线菌酮(50μg／ml)可使hCG诱导的大鼠间质细胞的睾酮分泌下降,并使间质细胞的c-Myb蛋白免疫组化染色降低。该结果说明c-myb参与hCG诱导的大鼠间质细胞睾酮分泌作用。     

排卵前期卵泡颗粒细胞端粒酶的表达及其影响因素

用端粒酶重复扩增酶联免疫吸附分析法（telomeric repeat amplification protocol-enzyme linked immunoadsordent assay,TRAP-ELISA）观察体外培养的大鼠排卵前期卵巢颗粒细胞中端粒酶活性的表达及其影响因素,并用放射免疫分析法（radioimmunoassay,RIA）同步测定培养液中雌二醇（estradiol,E2）、孕西阿（progesterone,P0）含量的变化及MTT（四甲基偶氮唑盐）法测定颗粒细胞增殖指数,分析颗粒细胞中端粒酶活性的表达以及端粒酶活性表达的影响因素。本实验中大鼠排卵前期卵巢颗粒细胞中有端粒酶活性表达,且在人绒毛膜促性腺激素（human chorionic gonadotropin,HCG）、卵泡刺激素（follicle-stimu1ating hormone,FSH）、二丁酰环磷腺苷（dbcAMP）及维拉帕米（verapamil）作用下活性明显升高,而在反义c-myb作用下活性明显降低。RIA测定培养液中雌激素及孕激素含量发现,在verapamil及FSH作用下E2与P0分泌量明显升高,在dbcAMP及HCG作用下分泌量无明显改变,而在反义c-myb作用下分泌量明显降低,在不同作用因素下的端粒酶活性与它相对应的E2及P0分泌量无相关性。MTT法测定显示,反义hTERT能明显抑制颗粒细胞的增殖。由此可以证实,排卵前期卵巢的颗粒细胞中表达有端粒酶活性,其活性受FSH、HCG、verapamil、dbcAMP及癌基因的影响,并且端粒酶活性与颗粒细胞增殖功能相关。     

Steroidogenic response of rat and pig luteal cells to estradiol-17 beta and catecholestrogens in vitro.

The corpora lutea of several species contain estrogen receptors, but the role of estrogens in luteal function is unclear in most species. In this study, we investigated the direct effect of estradiol-17 beta (E2) and catecholestrogens (2-OHE2 or 4-OHE2) on rat and pig luteal steroidogenesis using in vitro cultures of small (SLC) and large (LLC) luteal cells prepared by elutriation. SLC and LLC were cultured at 37 degrees C for 36 h in serum-free media and treated with E2, 2-OHE2, or 4-OHE2; LH; forskolin (FORS); dibutyryl cAMP (dbcAMP); or combinations thereof. In the rat, E2 (2.5-10 micrograms/ml) inhibited progesterone (P4) production by both cell types dose-dependently. P4 production by rat SLC increased with increasing dose of 4-OHE2 up to the 2.5-microgram dose, then decreased to near control level at the 10-microgram dose. In LLC, P4 production in the presence of 4-OHE2 decreased initially (up to 2.5 micrograms/ml 4-OHE2), then increased at the 10-microgram dose. LH, FORS, and dbcAMP stimulated P4 production by SLC and LLC. For SLC, the stimulatory effects of LH and 4-OHE2 (2.5 micrograms) were comparable but lower than those of FORS and dbcAMP. For LLC, the effects of 4-OHE2 (10 micrograms), LH, and FORS were comparable but lower than those of dbcAMP. In time-course experiments, E2 inhibition of P4 production was observed at 36 and 72 h but not 6 h of culture for SLC and at all time points for LLC.(ABSTRACT TRUNCATED AT 250 WORDS)     

Effects of cholesterol and cAMP on progesterone production in cultured luteal cells isolated from pseudopregnant cat ovaries

The present study was designed to incubate luteal cells isolated from pseudopregnant cats and to investigate the effects of cholesterol and cAMP on luteal progesterone production. Corpora lutea were collected from the cats on days 10 and 15 of pseudopregnancy. Luteal cells were isolated from the ovaries by collagenase digestion. Steroidogenic luteal cells were stained for 3β-hydroxysteroid dehydrogenase (3β-HSD) activity. Cells (2 × 10⁴) staining positive for 3β-HSD were cultured for up to 7 days. The cells were treated with 22(R)-hydroxycholesterol (22R-HC) and dibutyryl cyclic AMP (dbcAMP) on days 1, 3 and 7.Treatment of cells with 22R-HC resulted in a dose-dependent increase (p < 0.001) in progesterone production. When 22R-HC was used at a concentration of 10 μg/ml, it resulted in 2.7- and 5.1-fold increases in progesterone production on days 3 and 5, respectively. When the dose was doubled (20 μg/ml), treated cells produced four times more progesterone on days 3 and 7, and three times more on day 5. By day 7, progesterone production increased up to 9.1 times more than the control.Incubation of cells with both concentrations of dbcAMP (0.1 mM and 1 mM) resulted in significant stimulations of progesterone on days 5 and 7 (p < 0.001). However, on day 3, only higher doses of dbcAMP (1 mM) resulted in significant stimulation (p < 0.05). Progesterone production was increased up to 2- and 2.9-fold of the control when cells were treated with lower concentration of dbcAMP (0.1 mM) on days 5 and 7, respectively. Incubation of cells with 1 mM concentrations of dbcAMP induced a 3.2-fold increase on day 5 and a 5-fold increase on day 7.In conclusion, a successful incubation was performed for long-life culturing of luteal cells collected from pseudopregnant cats. The method works well and allows for optimal growth and development of cells in the culture. The present study also demonstrated that incubating cat luteal cells with 22R-HC and dbcAMP induces a significant increase in luteal progesterone synthesis.     

细胞内外钙浓度变化不影响酪氨酸抗hCG致孕酮生成作用

实验取经ＰＭＳＧ－ｈＣＧ处理的未成年雌性大鼠卵巢,用胶原酶－ＤＮＡ酶消化,制得黄体细胞悬浮液,预孵育１ｈ后加入各种处理因素,继续孵育２ｈ,用放射免疫方法测孵育液中孕酮的量。结果：孵育液中含有高钙或高钾或加入Ａ２３１８７时均可增加黄体细胞基础及ｈＣＧ诱导的孕酮生成量。相反,减少钙的浓度或加入ＥＧＡＴ或戊脉胺,孕酮生成量则明显减少。酪氨酸抑制ｈＣＧ刺激的孕酮生成,但对高钙、高钾和Ａ２３１８７增加孕酮的作用没有影响,并对上述三者分别与ｈＣＧ同时作用所致孕酮生成增加也没有影响。提示：大鼠黄体细胞孕酮生成依赖于细胞内外的钙;细胞内外钙浓度的变化不影响酪氨酸抗ｈＣＧ致孕酮生成作用;钙与ｈＣＧ使孕酮增加的作用可能是通过不同机制。     

Modulation of cyclic AMP formation and progesterone secretion by human chorionic gonadotropin, epinephrine, buserelin and prostaglandins in normal or human chorionic gonadotropin desensitized rat immature luteal cells in monolayer culture

It is now well recognized that hCG-induced luteolysis is associated with hCG-induced desensitization, but the physiological significance of luteal cell GnRH, PGs and beta-receptors is still undefined. Therefore, we intend in this study to observe the effects of prostaglandin F2 alpha and prostaglandin E2 and the interactions between epinephrine, a potent LHRH agonist [(D-Ser-(TBu)6, des-Gly-NH10(2) LHRH ethylamide: Buserelin] and hCG in normal and in vitro hCG-desensitized rat immature luteal cells in monolayer culture, on basal, hCG or cholera toxin stimulated intracellular and extracellular cAMP and progesterone secretion. The present report shows that incubation of immature rat luteal cells in monolayer culture with Buserelin, led to 25-50% inhibition of the epinephrine-as well as PGE2-induced cAMP and progesterone responses. The LHRH agonist can also reverse the stimulatory effects of cholera toxin in the presence of hCG and led with PGF2 alpha, to additive inhibitory effects on extracellular cAMP accumulation induced by cholera toxin. Both Buserelin and PGF2 alpha can reverse the hCG-induced cAMP and progesterone release but no effect could be observed when the incubation was carried out with either substance in the absence of hCG. Prostaglandin E2, in acute conditions of incubation, seems to share agonist properties with hCG when both were incubated with luteal cells. Buserelin reversed the stimulatory effects of PGE2, hCG, epinephrine and cholera toxin on cAMP and progesterone responses to these substances. These results suggest that Buserelin and PGF2 alpha have luteolytic-like effects and that there may be a complementary action for the two substances. Preincubation of rat luteal cells in monolayer culture with 1 nM hCG for a 24 h period led to the inhibition of cAMP and progesterone responses after a subsequent exposure to hCG and epinephrine. Luteal cells were no longer responsive to hCG while the presence of epinephrine in hCG-desensitized cells led to a 40% stimulation of cAMP and progesterone production. These observations suggest that occurred a partial alteration of the N component activity of the adenylyl cyclase system.     

细胞渗透性神经酰胺可抑制大鼠离体黄体细胞甾体激素生成并诱导细胞凋亡

本文旨在观察神经酰胺对离体孵育的大鼠黄体细胞孕酮分泌及细胞凋亡的影响,以PMSG－hCG处理的雌性Wistar大鼠为模型,分离制备黄体细胞,将外源性细胞渗透性神经酰胺与黄体细胞共同孵育,分别用放免法和流式细胞仪分析神经酰胺对黄体细胞孕酮生成和凋亡的影响,同时还检测了一氧化氮合酶（NOS）活性和一氧化氮（NO）水平的变化,结果显示,神经酰胺可以剂量相关方式抑制hCG－诱导的孕酮分泌,而对基础孕酮没有显著影响,离体孵育12h的大鼠黄体细胞存在自发性凋亡,5umol/L神经酰胺能显著增加亡率（P＜0．05）,流式细胞仪分析可见增强的凋亡蜂,实验还发现,50umol/L神经酰胺能明显促进NOS活性（P＜0．01）和NO生成（P＜0．01）,结果提示,神经酰胺可能通过调节甾体激素生成和细胞凋亡而作为一种重要的信息分子参与黄体退化等卵巢的生理过程。     

Effects of high density lipoprotein containing high or low beta-carotene concentrations on progesterone production and beta-carotene uptake and depletion by bovine luteal cells

Luteal cells were isolated from mid-luteal heifer ovaries by collagenase digestion. Cells were cultured with DMEM/Ham's F12 medium in serum pre-treated plastic culture dishes for periods of up to 11 days. As beta-carotene is almost completely insoluble in all polar solvents, it was added to cultures in either dimethyl sulphoxide (DMSO), tetrahydrofuran (THF) or as high-density lipoprotein (HDL) containing high or low beta-carotene concentrations. Medium was replaced after 24 h, thereafter medium was changed every 48 h. Treatment of cells with DMSO alone or with beta-carotene (5 micromol/l) in DMSO both resulted in significant (P<0.01) stimulation of progesterone production. beta-Carotene (5 micromol/l) in THF did not alter progesterone production but 50 micromol/l beta-carotene in THF resulted in significant inhibition (P<0.02) of progesterone production on days 3 and 7. Cultures were also supplemented with bovine HDL preparations containing equal concentrations of cholesterol (25 microg/ml) but high or low beta-carotene (12.4 or 0.44 microg/mg of cholesterol). Both HDL preparations significantly stimulated progesterone production (P<0. 001) but the high beta-carotene HDL was significantly (P<0.02) more effective than the low beta-carotene HDL. However, when given together with bovine luteinizing hormone (bLH) or dibutyryl cAMP (dbcAMP), the high beta-carotene HDL stimulated progesterone production less than did the low HDL (P<0.01). Uptake and depletion of beta-carotene by luteal cells were also examined in culture. beta-Carotene supplementation increased luteal cell beta-carotene from an initial level of 373 ng per 10(6) cells to 2030 ng per 10(6) cells by day 6. In contrast, the levels in control cells decreased to 14% of starting values during the same period. Cells treated with HDL containing high beta-carotene on day 1 or days 1 and 3 were then incubated with or without bLH or dbcAMP for a further 2 days to investigate the effect of bLH and dbcAMP on depletion of beta-carotene by luteal cells. beta-Carotene depletion in the luteal cells was significantly higher (P<0.05) in LH- and dbcAMP-treated cells than in the control cells in both groups. These results indicate that the use of solvents such as DMSO or THF may have undesirable effects due to alteration of cell membrane permeability. Supplementation with bLH or dbcAMP may increase the metabolism of beta-carotene in luteal cells. bLH or dbcAMP together with high beta-carotene HDL may, when combined with the effect of increased beta-carotene metabolism, give less stimulation than with low beta-carotene HDL.