PMSG、E_2、PGF_(2α)和hCG组合处理对初情前蓝狐卵巢和子宫的影响

为了完善提高狐狸繁殖效率的超排技术,探讨了用PMSG、E2、PGF2α和hCG的不同组合处理对诱发初情前雌性蓝狐发情及其对卵巢和子宫发育的影响.EPP组(E2、PMSG和PGF2α组合)和EPPh组(E2、PMSG、PGF2α和hCG组合)分别有2只和3只发情,而对照组未见发情;EPP和EPPh组卵巢指数和有腔卵泡百分率显著高于对照组(P<0.05),而初级卵泡所占百分率则显著低于对照组.此外,EPPh组次级卵泡所占百分率与对照组相比显著降低(P<0.05);当用EPP和EPPh法处理雌性蓝狐后,子宫指数、子宫壁和子宫内膜厚度显著高于对照组(P<0.05).结果 表明,EPP和EPPh处理不仅具有诱发雌性蓝狐发情的功效,而且能够提高初情前雌性蓝狐卵巢指数和增加有腔卵泡数量.     

PMSG或FSH同期发情处理对小鼠卵巢、输卵管和子宫中孕激素受体分布的影响

目的探讨孕马血清促性腺激素（pregnant mare serum gonadotropin,PMSG）和促卵泡激素（folliclestimulating hormone,FSH）同期发情处理的小鼠卵巢、输卵管和子宫中孕激素受体（progesterone receptor,PR）分布的差异。方法 10只8周龄KM系雌鼠,随机分为PMSG和FSH两个组,第一次处理后48 h取其卵巢、输卵管、子宫进行固定,免疫组织化学法观察各组织中PR的分布。结果两组小鼠卵巢、输卵管和子宫内膜中均有PR表达;其中PMSG组初级卵泡、次级卵泡和输卵管的阳性率均显著高于FSH处理组（P〈0.05）;PMSG组各级卵泡的平均吸光度值均显著高于FSH处理组（P〈0.05）;PMSG处理组子宫内膜上皮与腺上皮中的阳性率显著高于FSH组（P〈0.05）,而基质和子宫内膜上皮中的平均吸光度值显著低于FSH组（P〈0.05）。结论 PMSG和FSH同期发情处理不同程度影响小鼠卵巢、输卵管和子宫中PR的表达分布;其中PMSG处理组小鼠卵巢、输卵管和子宫上皮中PR表达普遍显著高于FSH处理组。     

血管紧张素Ⅱ在小鼠卵泡闭锁中的作用

应用幼年小鼠经孕马血清促性腺激素（pregnant mares serum gonadotropin,PMSG)处理的动物模型,研究了卵泡从发育到闭锁动态变化过程中血管紧张素Ⅱ（AngⅡ）的作用。结果表明：（1）24日龄小鼠给予PMSG（10IU/只）后6d时,卵巢中出现大量闭锁卵泡,颗粒细胞DNA琼脂糖电泳显示了梯形条带;（2）随卵泡闭锁发生,卵巢AngⅡ含量增加;（3）AngⅡ显著拮抗FSH刺激颗粒细胞雌二醇生成的作用。我们认为,AngⅡ参与了对小鼠卵泡闭锁的调节。     

PMSG和FSH同期发情处理对小鼠子宫、卵巢和输卵管中雌激素α受体分布的影响

目的从雌激素α受体（estrogen receptorα,ERα）的角度探讨孕马血清促性腺激素（pregnant mareserum gonadotropin,PMSG）和促卵泡激素（follicle-stimulating hormone,FSH）处理小鼠的卵巢、输卵管和子宫中,ERα分布是否有显著性差异。方法 10只8周龄母鼠,随机分为处理方式不同的两个组：PMSG组和FSH组,两组均在处理第48小时取其卵巢、输卵管和子宫样固定,采用免疫组织化学法分别观察组织中ERα分布情况。结果免疫组化结果显示,两个处理组小鼠卵巢、输卵管和子宫内膜的细胞中都有ERα表达;PMSG处理组卵巢中的初级卵泡和成熟卵泡上ERα阳性率和平均吸光度均显著高于FSH处理组;FSH处理组的输卵管中ERα阳性率和平均吸光度均高于PMSG处理组;FSH处理组子宫基质和腺上皮细胞中ERα的阳性率显著高于PMSG组,其中PMSG组基质中的平均吸光度显著高于FSH组,而子宫内膜上皮细胞的阳性率和平均吸光度两处理组间差异无显著性。结论 PMSG和FSH同期发情诱导由于其特性可不同程度地影响小鼠卵巢、输卵管和子宫中ERα的分布,使之在不同组织中产生差异性变化。     

小鼠胚胎卵巢卵泡体外无血清培养体系的建立(英文)

调节原始卵泡形成、起始生长的信号目前仍知之甚少。一个重要的原因就是缺乏一个良好的研究模型。我们以妊娠１３天昆明白小鼠胚胎卵巢为研究材料,经过５天的贴壁培养后,分别用牛血清（ＦＢＳ）、无血清（ＩＴＳ）和含有人卵泡刺激素（ＦＳＨ－ＩＴＳ）培养液继续体外培养到第１９天,发现ＩＴＳ组培养的胚胎卵巢卵泡发育要显著优于ＦＢＳ组（Ｐ＜０．０１）,如：培养至第７天时（Ｐ１,相当于出生日）,卵泡数分别为２９５±１８和 ２０６±１７;培养至第１３天时（Ｐ７）,卵泡数分别为 ５９４±３１和 ２６２±２８;培养至第１９天时（Ｐ１３）,卵泡数分别为 ３７１±２５和 ５０±１１（Ｆｉｇ．１,２＆４）。ＩＴＳ处理组的绝大部分卵巢在培养早期（如：Ｐ５前）都形成了皮质－髓质样的卵泡生长模式,而ＦＢＳ处理组超过半数卵巢不能形成皮质一髓质样的卵泡生长模式;ＦＳＨ－ＩＴＳ处理组和ＩＴＳ处理组的胚胎卵巢卵泡发育并无显著差异（Ｆｉｇ．２,４＆５）。 结果提示所建立的以ＩＴＳ为血清替代物的无血清培养模型更益于小鼠胚胎卵巢卵泡的体外发育;ｈＦＳＨ不是小鼠胚胎卵巢早期发生发育所必须的。     

不同剂量孕马血清促性腺激素超排处理对家兔卵巢组织形态和胚胎发育的影响

为了研究不同剂量的孕马血清促性腺激素（PMSG）对家兔（Oryctolagus cuniculus f. domesticus）超排后,卵巢组织形态和PMSG对早期胚胎体外发育的影响。将24只家兔分为对照组、50 IU、70 IU和90 IU组,每组6只,对照组不做处理,后3组分别注射50 IU、70 IU和90 IU PMSG和定量100 IU人绒毛膜促性腺激素（HCG）对家兔进行超排处理。解剖后测定卵巢形态和组织参数。利用注射器抽取5ml冲卵液,分别从左右输卵管冲取胚胎至培养皿中,转至细胞培养室对胚胎进行体外培养观察。结果显示,PMSG处理组与对照组相比,随着PMSG注射剂量的增大,家兔卵巢重及宽度和厚度均极显著增大（P<0.01）,卵巢长度显著增长（P<0.05）,卵巢表面充血,卵泡数增多;另外,随PMSG注射剂量的增大,次级卵泡及其卵母细胞直径、三级卵泡直径均呈减小趋势（P <0.01）,三级卵泡中卵母细胞直径呈增大趋势,与对照组相比差异显著（P <0.05）;三级卵泡的直径和卵泡的优势化率,70 IU组显著高于对照组及50 IU和90 IU组（P &l...     

小鼠卵巢几个重要发育事件的初步研究

选定多个阶段小鼠卵巢进行切片染色和生殖细胞计数统计等分析,以发现该阶段小鼠卵巢的发育特点。结果显示在胚胎发育第12.5 d的生殖嵴中,大部分的生殖细胞正进行有丝分裂增殖,并以生殖包囊的形式存在;在出生后第2 d的小鼠卵巢中,有大量紧密接触的原始卵泡,表明生殖包囊刚完成重组形成原始卵泡;在第5 d的小鼠卵巢中,原始卵泡仍占有大部分比例,但也有大量的初级卵泡处于发育之中;在出生后第10 d的卵巢中同时有原始卵泡、初级卵泡和次级卵泡的发育;老年小鼠(16个月大)卵巢中已基本没有卵母细胞。     

小鼠卵巢冷冻移植后卵泡发育和卵母细胞成熟的研究

本研究探讨了冷冻保存的1日龄小鼠卵巢异体异位移植后,其原始卵泡重新启动生长发育的能力。一日龄B6C2F．小鼠卵巢分离冷冻后置液氮中保存,保存1周。6个月后解冻,并将卵巢移植到8-12周龄B6C2F．受体鼠。肾脏包膜下,移植至少14d。每侧肾囊移植2枚卵巢的40只受体鼠中卵巢的回收率为45．00％（72／160）,而每侧。肾囊移植l枚卵巢的20只受体鼠的回收率为82．50％（33／40）。移植卵巢上卵泡的发育基本与体外自然生长鼠的卵巢卵泡发育情况一致。对卵巢移植19d的受体鼠用孕马血清促性腺激素（pregnant mare serum gonadotrophin,PMSG）处理后,从移植卵巢上发育成熟卵泡中获得的卵母细胞在MEM0c培养基中培养16-17h,有40．90％的卵母细胞发生生发泡破裂（germinal vesicle breakdown,GVBD）,其中89．02％的卵母细胞发育到第二次减数分裂中期（metaphaseⅡ,MⅡ）。将剩余的卵母细胞继续培养到20～21h,又有50．83％的卵母细胞发生生发泡破裂,但其中只有21．40％的卵母细胞能够发育到MII期。以上结果说明,小鼠早期卵巢经过冷冻．解冻并异体异位移植后,其原始卵泡能够重新启动生长发育,发育后的卵泡卵母细胞能够在体外培养成熟。这些结果意味着原始卵泡或卵巢冷冻一移植技术有可能充分利用雌性生殖细胞用于濒危动物保种、建立动物基因库和人类辅助生殖等。     

妊娠期腹腔注射多氯联苯对大鼠生长发育的影响

将50只同期怀孕的大鼠分为5组,在怀孕第7—18d,每天给两组大鼠腹腔分别注射1和20mg／kg体重2,2’,4,4’-四氯联苯(PCB47);给另两组分别注射0．25和1mg／kg体重3,3’,4,4’-四氯联苯(PCB77);对照组注射0．1mL芝麻油。幼鼠出生时记录每窝产仔数和性比;出生后每隔7d称体重直到第119d;出生后第15天时检查幼鼠的睁眼率。与对照组相比,PCB47和PCB77所有剂量组每窝产仔数和性比无显著差异;PCB47(20g／kg体重组)和PCB77(两个剂量组)雌幼鼠肛门一生殖孔距离显著增加,出生后15d幼鼠的睁眼率显著降低;PCB77(1mg／kg体重组)雄幼鼠从出生后第35至119天体重显著降低。提示PCB77主要影响雄鼠的生长发育。     

外源激素组合控制青春期前奶山羊卵泡超数同步发育及其卵母细胞发育潜能的评价

本研究的目的是探索自青春期前奶山羊获取大量可用于体细胞核移植的卵母细胞的可能性。为此,本研究比较了几种不同组合的激素处理方法(对照、FSH、E2-P4和E2-P4-FSH)对出生39-60日龄的奶山羊卵巢大小、卵泡数量和卵泡大小的影响:同时将出生39-120日龄奶山羊按年龄分成三组来研究年龄对激素处理时招募起始生长卵泡数量的影响:然后,比较了来自E2-P4- FSH和FSH处理的早青春期前奶山羊卵巢上直径大于3mm卵泡中卵母细胞减数分裂能力;最后,通过SCNT方法验证E2-P4-FSH处理的早青春期前奶山羊卵巢上直径大于3mm卵泡中卵母细胞的发育能力。在四组激素处理的早青春期前奶山羊中,E2-P4-FSH处理组的卵巢最大、卵泡(直径大于3 mm)数量最多。在不同的年龄组中,39-60天组奶山羊卵巢上直径大于3mm的卵泡数量显著多于61-90天和91-120天组的。卵母细胞减数分裂能力的分析结果表明,来自E2-P4-FSH处理组的卵母细胞减数分裂能力显著高于FSH处理组的卵母细胞。与E2-P4-FSH处理后的成年奶山羊卵母细胞相比,早青春期前奶山羊卵母细胞发育能力较低:卵母细胞成熟后,作为受体用于体细胞核移植后的克隆囊胚发育率低于成年奶山羊(15.3%versus 22.1%,P<0.01)。然而,早青春期前的奶山羊经E2-P4-FSH处理后,自每头羊卵巢上直径大于3mm的卵泡数显著高于成年奶山羊(108±10.3 versus 28±5.0),因此,每头早青春期前奶山羊产生的克隆囊胚绝对数量显著高于成年奶山羊(7.1±2.7 versus 4.2±1.4)。由此,从本研究可以得出结论:E2-P4-FSH处理的早青春期前奶山羊能够为体细胞核移植研究提供相对多数量的具备一定发育能力的成熟卵。     

In utero exposure of mice to diethylstilbestrol alters neonatal ovarian follicle growth and development

The prenatal exposure of mice to diethylstilbestrol (DES, 10 micrograms/kg on day 15 of gestation) caused both quantitative and structural alterations in ovarian follicles within the neonatal ovary. At birth, control ovaries consisted of small type 1 and 2 ovarian follicles located in the ovarian cortex. By postnatal day 7, ovarian follicle development had advanced to the type 4 stage with larger follicles located within the ovarian medulla. In DES-exposed animals, ovarian follicle maturation was advanced with type 3b and 4 follicles appearing 24 h prior to their appearance in control animals. Also, type 5 ovarian follicles were present on postnatal day 6 in experimental animals but were never seen in control animals. In addition to an alteration in ovarian follicle dynamics, the diameter of individual ovarian follicles was transit time between the various stages of follicular development which results in a greater number of developmentally advanced ovarian follicles being present during neonatal ovarian development. The mechanism by which prenatal exposure to DES alters ovarian follicle dynamics during neonatal development is not known.     

Effects of FGA and PMSG on follicular growth and LH secretion in Suffolk ewes

The effects of fluorogestone acetate (FGA) and/or pregnant mare serum gonadotrophin (PMSG) on follicular growth and LH secretion in cyclic ewes were determined. Suffolk ewes (n = 40), previously synchronized with cloprostenol were divided into 4 experimental groups (n = 10 ewes per group). Group I served as the control, while groups II, III and IV received FGA, PMSG, FGA and PMSG respectively. Four ewes of each group underwent daily laparascopy for 17 d. All the ovarian follicles >/= 2 mm were measured, and their relative locations were recorded on an ovarian map in order to follow the sequential development of each individual follicle. Comparisons were made of the mean day of emergence and the mean number of small, medium and large follicles, the atresia rate and the ovulation rate. For each group, 3 waves of follicular growth and atresia were observed during the cycle. During luteal phase, FGA treatment accelerated the mechanisms of follicular growth but reduced the number of large follicles and increased the atresia rate. In the follicular phase, FGA treatment was detrimental to both the number of large follicles and the ovulation rate. By contrast, PMSG enhanced recruitment of small follicles and the ovulation rate. Serial blood samples were collected during the luteal and follicular phases to study LH secretion. None of the treatments had any effect on LH secretion patterns.     

Development of infantile rat ovaries autotransplanted after cryopreservation by vitrification

We cryopreserved infantile rat ovaries by vitrification and assessed their viability by autotransplantation. Hemilateral ovarian transplantation was performed on rats on postnatal Days 10 to 12. The left ovary of each rat was dissected out, cryopreserved by vitrification using a modified vitrification solution (VS1), and then autotransplanted under the capsule of the right kidney. The right ovary of each rat was removed. For the control, the left ovary was dissected out from each rat and was immediately transplanted by the same procedure, without cryopreservation. Rats were nursed until weaning, and then the day of vaginal opening, estrous cyclicity from the day of vaginal opening until postnatal Day 84, and histology of ovarian grafts at postnatal Day 84 were examined. The time course of development of endocrine function of cryopreserved grafts was similar to that of fresh grafts. In ovarian transplants recovered on postnatal Day 84, antral follicles and corpora lutea (CL) were observed in addition to small follicles, although the number of antral follicles in cryopreserved grafts was smaller than in the fresh grafts. These results indicate that cryopreservation of ovarian tissue by vitrification can be used for the preservation of fertility and endocrine function of ovaries.     

Cellular localization of ovarian proopiomelanocortin messenger RNA during follicular and luteal development in the rat

Opioid peptides are expressed in the reproductive system and have been reported to regulate reproductive function. The present study used in situ hybridization to selectively localize ovarian cells containing high levels of proopiomelanocortin (POMC) mRNA, an opioid precursor, during different stages of ovarian development. Prepubertal rats were primed with PMSG to stimulate follicular development, followed by hCG to induce ovulation. Treatment groups consisted of control (no treatment), PMSG (2 days post-PMSG), 1 day corpus luteum (CL; 1 day post-hCG), and 8 day CL (8 days post-hCG). POMC mRNA-containing cells were present in antral follicles, CL, and the interstitial compartment. With gonadotropin treatment, the percentage of follicles containing heavily labeled cells increased in the PMSG and 1 day CL groups. The number of POMC mRNA-containing cells per follicle also increased in the 1 day CL group. In the CL, no difference was observed in the percentage of CL exhibiting labeled cells between the 1 day CL and 8 day CL groups; however, more labeled luteal cells per CL were present in the 1 day CL group. A marked increase in POMC mRNA-containing cells was observed in the interstitial compartment of the 1 day CL group. These results indicate that the number of POMC mRNA-containing cells increases with follicular development and CL formation; however, the ovarian distribution suggests that the labeled cells could be nonendocrine cells, possibly white blood cells. The in situ hybridization findings are indicative of low total concentrations of ovarian POMC mRNA, suggesting mainly an autocrine or paracrine role for POMC or POMC-derived peptides.(ABSTRACT TRUNCATED AT 250 WORDS)     

Ovarian response to exogenous hormones in six-week-old lambs.

Crossbred lambs 5--6 weeks old were treated with human chorionic gonadotrophin (hCG) (500 or 1500 i.u.) alone, hCG plus pregnant mare serum gonadotrophin (PMSG) (1000 or 2000 i.u.), 1000 i.u. PMSG alone, or were untreated. PMSG alone and PMSG + hCG increased ovarian weight and uterine weight. PMSG alone stimulated growth and luteinization of follicles but PMSG + hCG induced ovulations and formation of corpora lutea. hCG alone did not change any of the characteristics which were measured. PMSG had a significant effect on the number of vesicular follicles but none of the treatments affected the number of growing follicles.     

噬菌蛭弧菌代谢产物活性成分对小鼠免疫功能的影响

目的研究噬菌蛭弧菌代谢产物活性成分对小鼠免疫功能的影响。方法将噬菌蛭弧菌代谢产物的3种有机溶剂（石油醚、三氯甲烷、乙酸乙酯）提取物和提取后的剩余液体分别腹腔注射实验小鼠,分两次注射,共注射0.5 mL,注射后连续饲养28 d,每隔7 d小鼠采血检测离体白细胞吞噬活性（phagocytic activity）、吞噬细胞杀菌活性（bactericidal activity）、超氧化物歧化酶（superoxide dismutase,SOD）活性、血清凝集抗体效价、血红蛋白值和红细胞数的变化,以研究不同提取物对小鼠免疫功能的影响。结果石油醚提取物组和三氯甲烷提取物组小鼠血清SOD活性、血清凝集抗体效价、离体白细胞吞噬活性和吞噬细胞杀菌活性增强与对照组相比差异极显著（P〈0.01）;乙酸乙酯提取物组SOD活性和血清凝集抗体效价增强与对照组相比差异极显著（P〈0.01）,离体白细胞吞噬活性和吞噬细胞杀菌活性增强与对照组相比差异显著（P〈0.05）;石油醚提取物组的血红蛋白值（12.64 g/100 mL）和红细胞数（11.32×106/mL）最高。各项指标的峰值均出现在第7天~第21天。结论噬菌蛭弧菌代谢产物3种有机溶剂提取的活性物质具有增强小鼠免疫功能的作用。     

The follicle-deplete mouse ovary produces androgen

The follicle-depleted postmenopausal ovary is enriched in interstitial cells that produce androgens. This study was designed to cause follicle depletion in mice using the industrial chemical, 4-vinylcyclohexene diepoxide (VCD), and characterize the steroidogenic capacity of cells in the residual ovarian tissue. From a dose-finding study, the optimal daily concentration of VCD was determined to be 160 mg/kg. Female B6C3F(1) immature mice were treated daily with vehicle control or VCD (160 mg kg(-1) day(-1), 15 days, i.p.). Ovaries were removed and processed for histological evaluation. On Day 15 following onset of treatment, primordial follicles were depleted and primary follicles were reduced to about 10% of controls. On Day 46, primary follicles were depleted and secondary and antral follicles were reduced to 0.7% and 2.6% of control, respectively. Seventy-five percent of treated mice displayed disruptions in estrous cyclicity. All treated mice were in persistent diestrus (acyclic) by Day 58. Plasma FSH levels were increased (P < 0.05) relative to controls on Day 37 and had plateaued by Day 100. Relative to age-matched cyclic controls, by Day 127, the significant differences in VCD-treated mice included reduced ovarian and uterine weights, elevated plasma LH and FSH, and reduced plasma progesterone and androstenedione. Furthermore, plasma 17beta-estradiol levels were nondetectable. Unlike controls, immunostaining for LH receptor, and the high density lipoprotein receptor (SR-BI), was diffuse in ovarian sections from VCD-treated animals. Ovaries from Day 120 control and VCD-treated animals were dissociated and dispersed cells were placed in culture. Cultured cells from ovaries of VCD-treated animals produced less LH-stimulated progesterone than control cells. Androstenedione production was nondetectable in cells from cyclic control animals. Conversely, cells from VCD-treated animals produced androstenedione that was doubled in the presence of insulin and LH (1 and 3 ng/ml). Collectively, these data demonstrate that VCD-mediated follicle depletion results in residual ovarian tissue that may be analogous to the follicle-deplete postmenopausal ovary. This may serve as a useful animal model to examine the dynamics of follicle loss in women as ovarian senescence ensues.     

Role of intrafollicular regulators and FSH in growth and development of large antral follicles in sheep

Manipulation of circulating concentrations of hormones and ovarian follicle status was carried out on Day 11-12 of the oestrous cycle in sheep. All follicles visible on the ovary were ablated by cautery and ewes were treated with oestradiol or ovine follicular fluid (oFF) to suppress FSH or with PMSG to increase circulating gonadotrophic activity. One group underwent unilateral ovariectomy which greatly increased endogenous FSH and was the only treatment which significantly affected LH pulse frequency. The size distribution of antral follicles, the extent of atresia and the mitotic index of granulosa cells of follicles on Day 15 showed that (a) treatment with oFF inhibited the growth of follicles beyond 2 mm diameter by suppressing the mitotic index of the granulosa cells and (b) the concentration of FSH in peripheral plasma was related to the ability of small antral follicles to grow during the late luteal-early follicular phase of the cycle. Subsequently, it was demonstrated that oFF inhibits, in a dose-dependent manner, folliculogenesis sustained by PMSG in ewes on Days 12-15. Inhibition of folliculogenesis was represented by a decrease in those follicles greater than 4 mm, an increase in the relative proportion of follicles less than 2 mm, and minimal change in the average number of follicles visible on the ovarian surface, and a decrease in the mitotic index of granulosa cells of follicles less than 2 mm. There was no change in the extent of atresia.(ABSTRACT TRUNCATED AT 250 WORDS)