复方辣木颗粒剂影响雄性小鼠性功能的实验研究

目的观察复方辣木颗粒剂对雄性小鼠性功能的影响。方法建立醋酸铅致雄性小鼠生精障碍模型。将60只实验小鼠分为正常组、模型组、阳性对照组和复方辣木颗粒剂高、中、低剂量组,每组10只。给药后,观察小鼠体重、脏器指数、附睾精子活力、精子活率及睾丸的病理形态等。结果复方辣木颗粒剂对醋酸铅致少弱精子症小鼠体重无明显影响,各给药组小鼠附睾系数、睾丸系数、精子活力、精子活率均有所上升,生精细胞和间质细胞数量增多、排列更紧密。各剂量间比较,高剂量效果更显著(均P0.05)。结论复方辣木颗粒剂可显著改善小鼠性功能,为临床合理应用提供有利参考。     

一种改进的阴茎电刺激采精法和猕猴藏酋猴及熊猴的采精及其精液特征的初步研究

本文报道了一种改进的阴茎电刺激采精法,用脱脂棉和铝箔作为电极,以避免直接用金属电极可能对阴茎的损伤,并运用这一方法对猕猴（Ｍａｃａｃａｍｕｌａｔｔａ）、藏酋猴（Ｍ．ｔｈｉｂｅｔａｎａ）和熊猴（Ｍ．ａｓｓａｍｅｎｓｉｓ）进行了电刺激采精及其精液特征研究。电刺激采精模式为连续刺激和间断刺激方式。在采精过程中没有发生阴茎损伤。对初次接受电刺激采精的动物以间断刺激模式效果较好。猕猴、藏酋猴和熊猴的射精体积分别为２．０±０．１、６．３±１．１和３．２±０．６ｍｌ;液化体积分别为０．７±０．６、２．１±０．４和１．７±０．３ｍｌ;精子浓度分别为１２．６±１．２×１０~８、４５．６±５．６×１０~８和１１．５±０．９×１０~８／ｍｌ。３种动物精液的液化率分别为：猕猴３６．２±０．９％,藏酋猴３４．０±１．４％;熊猴５１．８±１．２％。３种动物的精子总数与射精体积和凝块体积没有相关性（ｒ~２＝０．０７９;０．０１６;０．０９４和ｒ~２＝０．０６４;０．０２０;０．０７２）。上述结果表明：１）改进的阴茎电刺激采精法适用于猕猴,特别是阴茎表面较为粗糙的藏酋猴和熊猴;２）藏酋猴的射精体积和精子总数是迄今已报道的非人灵长类中最大的,可能     

小鼠发情周期卵泡发育动态及其对超数排卵的影响

该文探讨了小鼠发情周期中阴门状态、阴道脱落细胞类型变化规律、卵泡发育规律及其相互关系,并比较了发情周期不同阶段的超排效果。结果表明,采用阴门状态观察法和阴道脱落细胞涂片法,能有效判断小鼠发情周期阶段。卵巢组织切片观察结果表明,在发情周期不同阶段,小鼠的卵泡发育和黄体的生成与消退存在明显的规律性变化;小鼠发情周期中,其阴门状态、阴道脱落细胞种类及卵泡发育动态之间存在相关关系;发情周期不同阶段开始超排的小鼠,其配种见栓率和回收胚胎平均数均存在明显差异,发情前期显著优于发情后期与间情期(P<0.05),并高于发情期,但差异不显著(P>0.05),即阴门状态观察法与阴道脱落细胞涂片法均可用于小鼠发情周期阶段的判断,发情前期为最适宜的小鼠超排时期。     

动物直肠电刺激采精试验

采集动物精液是人工授精的重要环节之一。假阴道釆精法是目前动物人工采精的最常用的方法。近来,动物直肠电刺激采精技术亦日益广泛地应用于珍贵野生动物的人工繁殖研究。我们从1976年开始,与广东省科学院实验工厂协作,研制成功动物直肠电刺激采精器,对多种动物进行了电采精试验。     

一种改进的阴茎电刺激精法和猕猴藏酋猴及熊猴的采精及其精液特征…

本文报道了一种改进的阴茎电刺激采精法,用脱脂棉和铝箔作为电极,以避免直接用金属电极可能对阴茎的损伤,并运用这一方法对猕猴（Ｍａｃａｃａ ｍｕｌａｔｔａ）、藏酋猴（Ｍ．ｔｈｉｂｅｔａｎａ）和熊猴（Ｍ．ａｓｓａｍｅｎｓｉｓ）进行了电刺激采精及其精液特征研究。电刺激采精模式为连续刺激和间断刺激方式。在采精过程中没有发生阴茎损伤。对初次接受电刺激采精的动物以间断刺激模式效果较好。猕猴、藏酋猴和熊猴的射精体     

动物直肠电刺激采精简报

电刺激采精是一种较为简便又安全的人工采精方法,它对于开展某些动物的人工繁殖、杂交等方面都有一定的意义。我们采用直肠电刺激法,对梅花鹿、马鹿、绵羊、家猫等不同动物,共进行了16次采精试验,效果良好,其精液品质符合输精要求。 一、电刺激采精器 电刺激采精器包括电刺激器和直肠探子两个部分     

济元阳口服液主要药效实验研究

以济元阳口服液7g/kg、14g/kg灌胃,使小鼠性器官、副性器官重量显著增加,去势大鼠副性器官亦有增加;小鼠附睾精子数量增加,精子活率提高,并能对抗环磷酰胺所致精子数量与活力下降,雄性小鼠及去势大鼠交配能力均有增强;肾阳虚小鼠体重、胸腺指数上升,自由活动、游泳耐力及耐寒能力均有所增强,以上实验结果表明,济元阳口服液有补肾壮阳、生精长力之功效。     

精子和卵母细胞质量控制对山羊卵胞质内精子注射(ICSI)受精的影响

以体外成熟卵母细胞为材料研究了精子来源及制动处理方法、卵母细胞质量及注射后激活等因素对山羊ICSI效果的影响.结果说明,附睾头、体和尾精子ICSI后的受精率、卵裂率和桑椹胚/囊胚发育率与射出的鲜精精子都没有明显差异(p＞0.05),但带下注射时附睾头和体精子的受精和发育率显著低于附睾尾和射精精子.在以4种不同方法致死的精子中,室温保存24h的死精子ICSI受精、卵裂和桑椹/囊胚率虽然低于对照组,但是明显高于其它方式致死的精子;5℃保存15天的死精子受精和发育效果最差.0.0005%Triton X-100处理精子的受精率、卵裂率和桑椹/囊胚率显著(p＜0.05)高于制动对照组、不制动对照组和其它浓度组.经高渗处理法检测质量好的卵母细胞ICSI受精和胚胎发育效果显著好于质量差的卵母细胞.与对照组相比,A23187和Ionomycin/6-DMAP激活处理均显著(p＜0.05)提高ICSI的受精率、卵裂率和桑椹/囊胚发育率.因此,精子在附睾内的成熟过程主要与其获得与卵质膜融合能力有关;精液保存方法对精子受精能力的损伤程度有很大差异;适当浓度的Triton X-100处理可模仿精子制动;卵母细胞质量是影响ICSI效果的重要因素;注射精子后激活卵母细胞能保证山羊ICSI的受精效果.     

不同稀释液对圈养黑熊精液品质的影响

对23头圈养黑熊进行63次电刺激采精,并在对精液进行品质检查的基础上,通过对3种稀释液4℃保存精液结果的筛选比较试验,得出以下结果:圈养黑熊采精量平均为1.06±0.93ml,pH值为6.71±0.44,精子密度为(3.23±1.68)×108个/ml,精子畸形率为(23.48±7.95)%,顶体完整率为(88.58±3.86)%,精子活率和活力分别为(76.30±13.91)%和(63.91±18.53)%;Tris-柠-果-葡-卵稀释液保存圈养黑熊精液效果最好,可作为进一步研究优化的首选。     

DNA—处理的精子作为基因转移载体

继１９８９年首次报道成功地利用精细胞作为载体把ＤＮＡ转入小鼠胚胎及随后ＤＮＡ整合入小鼠基因组后,现又取得了一些进展和新的发现。据报道,ＤＮＡ可结合或掺入不同种类的动物和昆虫的精子中,包括小鼠、猪、山羊、绵羊、牛、鸡、鲤鱼、海胆、蜜蜂和丽蝇类等。通常,人们用脂质体或电激法来促进ＤＮＡ进入精细胞。这些研究出现的一个意外结果是质粒转基因作为染色体外遗传因子的持久性。１９９５年,澳大利亚研究人员在《动物生物技术》杂志上曾发表了一篇用ＤＮＡ处理的精子人工授精生产转基因牛的报道。经Ｓｏｕｔｈｅｍ印迹分析表明…     

Inhibition of spermiation in the syrian hamster using dibutyryl cyclic-AMP

Summary Young adult male Syrian hamsters were given intraperitoneal injections of 50 mg dibutyryl cyclic AMP twice daily for a period of three days. On the fourth day the animals were sacrificed and their testes were processed for light and electron microscopy. The results indicate that the mature spermatozoa were retained within the seminiferous epithelium after the stage in the seminiferous cycle in which spermiation normally occurs. The unreleased spermatozoa were ultrastructurally normal. Typical Sertoli-spermatid junctional specializations remained associated with the retained spermatozoa. These findings indicate that normally spermiation is initiated by the disappearance of the junctional specializations. In addition, the present results demonstrate that spermiation can be controlled.Supported in part by NIH Grant RR05654 and by NIH Grant P 30 HD 10202 (Morphology Core)The skillful technical assistance of Pam Duke is gratefully acknowledged     

Pattern of loss of spermatozoa from the vagina of the ewe

In a series of experiments spermatozoa were inseminated blindly into the vagina of ewes and then recovered at varying times after insemination. Most of the spermatozoa inseminated were lost by drainage through the vulva. The rate of loss was not affected by the motility of spermatozoa or oestrous state of the ewe. Initially after insemination the loss was not rapid with 82% of the insemination 18% of spermatozoa remained and by 12 h 10% remained. Spermatozoa were removed from the vagina during withdrawal of the penis after intromission and the extent of this loss varied between rams and with the volume of semen already in the vagina. Up to half the inseminate was lost in this way when there was 0.5 ml of semen in the vagina but only 11% was lost when the volume of inseminate was 0.1 ml. The unavoidable loss of spermatozoa may influence the quantity available for fertilizing ova.     

Ultrastructural observations on spermatozoa retained within the seminiferous epithelium after treatment with dibutyryl cyclic AMP

Spermiation was inhibited in the Syrian hamster by administering large doses of dibutyryl cyclic AMP. After treatment with dibutyryl cyclic AMP most stage VIII, IX, and X seminiferous tubules contained some mature spermatozoa within the seminiferous epithelium. The acrosomal membranes and plasma membranes of the unreleased spermatozoa remained intact, indicating that the spermatozoa had not been phagocytized by the Sertoli cells. Sertoli-spermatid junctional specializations were usually applied to the heads of the mature spermatozoa. The unreleased spermatozoa often appeared swollen with accumulated fluid located in the subacrosomal space. The accumulation of subacrosomal fluid in the unreleased spermatozoa seems to result from the absence of tubulobulbar complexes. That is, when tubulobular complexes fail to form the normal flow of cytoplasm into the tubulobular complexes is blocked resulting in an accumulation of fluid around the nucleus. Inhibition of spermiation may result from the absence of tubulobulbar complex formation. It is postulated that the tubulobulbar complex functions to transfer a chemical trigger from the maturing spermatid into the Sertoli cell. This chemical trigger may initiate the disappearance of the Sertoli-spermatid junctional specialization and induce spermiation.     

Characteristics and seasonal variations in the semen of Alpine, Saanen and Damascus goat bucks born and raised in Greece

Twenty-three purebred Alpine (n=8), Saanen (n=7) and Damascus (n=8) goat bucks raised at the Institute of Reproduction and Artificial Insemination in Thessaloniki, Greece (40 degrees 37 minutes N, 22 degrees 58 minutes E and altitude 32 m above sea level), were used to study the effect of photoperiod on semen production. Samples were collected with an artificial vagina and examined immediately after collection. In spite of the variation in nearly all semen characteristics studied among the 3 breeds of bucks, there was significant seasonal variation in both semen quantity (volume, concentration and total number of spermatozoa per ejaculate) and quality (percentage of motile spermatozoa, percentage of abnormal spermatozoa and rate of progressive motility). The best semen was produced during the breeding season (late summer and autumn). However, the magnitude of these seasonal effects was not sufficient to prevent bucks from being used for breeding throughout the year. Nevertheless, individual differences in the semen quantity and quality among bucks within a breed make individual evaluation of semen necessary to select the most fertile males for breeding.     

Effect of the collection method on semen characteristics of Zebu and European type cattle in the tropics

The effect of the collection method on the characteristics of fresh semen and the recovery of spermatozoa after thawing was studied in 30 Zebu bulls (Bos indicus ) and in 30 Brown Swiss (Bos taurus ) bulls. Semen was collected by using an artificial vagina and by electroejaculation; the ejaculates were individually evaluated. Semen was diluted for freezing in skimmed milk and stored in 0.5-ml French straws, at a concentration of 30 x 10(6) spermatozoa. Data were evaluated by analysis of variance using a factorial model which included collection method, breed effect, and interaction between method and breed, with each bull as a block. Higher volume and pH of the semen was obtained following electroejaculation. Conversely, higher concentration prior to freezing and better progressive motility after thawing was observed in semen collected with an artificial vagina. No differences in motility were obtained in fresh semen between methods. Better post-thaw recovery occurred when the semen was collected by an artificial vagina, independently of the breed type.     

Effect of semen collection method (artificial vagina vs. electroejaculation), extender and centrifugation on post-thaw sperm quality of Blanca-Celtibérica buck ejaculates

The aim of this study was to evaluate the effect of semen collection method (artificial vagina compared to electroejaculation), season in which the semen was collected (breeding season compared to non-breeding season), freezing extender (Biladyl(?), Andromed(?) and skim milk based extender) and pre-treatment procedure (washing compared to non-washing) on post-thaw semen quality in buck. Ejaculates from seven bucks of the Blanca-Celtibérica breed were collected by artificial vagina and electroejaculation during the breeding (July to December) and non-breeding season (January to June). Samples were split in two aliquots and one of them was washed. Three freezing extenders were evaluated on washing and non-washing sperm samples. Ejaculates collected by artificial vagina had a greater sperm quality after thawing, with greater values (P≤0.05) for SM (sperm motility), NAR (acrosome intact), YO-PRO-1-/PI- (intact spermatozoa), and Mitotracker+/YO-PRO-1- (spermatozoa with active mitochondria) and lower % DFI (DNA fragmentation index). Thawed sperm samples which were collected during the breeding season had greater values (P≤0.05) for NAR, intact spermatozoa and spermatozoa with active mitochondria, than those semen samples obtained during the non-breeding season. Semen freezing with Biladyl(?) and Andromed(?) resulted in a greater sperm quality (P≤0.05) after thawing in relation to milk-based extender. Washing procedure had no effect on sperm parameters assessed at thawing. Results from the present study suggest that the success of semen cryopreservation in Blanca-Celtibérica goat depends on semen collection method and season, as well as on the extender used. Thus, the post-thaw sperm quality will be greater (P≤0.05) when samples are collected by artificial vagina during the breeding season and when Biladyl(?) or Andromed(?) are used as freezing extenders.     

Time required for spermatozoa to remain in the vagina of the ewe to ensure conception

Oestrous ewes (N = 202) were inseminated with 0.1 ml of semen containing 500 X 10(6) motile spermatozoa and the spermatozoa were flushed from their vagina either immediately or 0.25, 0.5, 1, 2, 4 and 8 h after insemination. Pregnancy was determined by returns to service and laparoscopy. Some ewes became pregnant (10.71%) after spermatozoa had been flushed from the vagina only seconds after insemination and about 40% of ewes became pregnant after spermatozoa had been in the vagina for 15 min. Maximum conception (55%) was achieved when spermatozoa had been in the vagina for at least 2 h. It was concluded that the losses of spermatozoa that occur from the vagina will not influence the chance of a ewe conceiving because sufficient spermatozoa to ensure a normal conception move up the reproductive tract before large losses from the vagina take effect.     

Effect of semen collection method on pre- and post-thaw Guirra ram spermatozoa

In this study, we evaluated the potential effect of the method of recovery (artificial vagina or electroejaculation) on the production and quality of Guirra ram spermatozoa cryopreserved for the possible constitution of a sperm bank. In order to address this question, we evaluated the effect of semen collection method on fresh semen quality parameters, including: volume, concentration, production, microscopic analysis (abnormal sperm and intact apical ridge) and sperm motility parameters determined by CASA system. For frozen-thawed semen, we evaluated motility parameters by CASA and intact apical ridge, acrosomal status, assessed by dual staining by IP and FITC-PNA and capacitation status, assessed by M540 and Yo-pro1, using flow cytometry. The main findings from this study were: (i) that electroejaculation resulted in a lower recovery efficiency (80% of the cases), as a consequence of contamination with urine or lack of response to the electrical stimulation; (ii) the fresh seminal quality was not significantly different between recovery methods, except for the concentration of spermatozoa, but total number of spermatozoa and the consequent number of possible seminal doses for artificial insemination were similar; and, (iii) a higher number of stable and functional spermatozoa (higher number of live non-capacitated cells, higher live acrosome intact cells and live acrosome reacted cells) were found for frozen-thawed spermatozoa collected by electro ejaculation than by artificial vagina. According to our results, we are able to develop both methodologies in the creation of the Guirra sperm bank. Assuming the advantages and limitations of both methodologies, in Guirra breed, would enable the rapid constitution of a sperm bank including samples from a large number of non-trained rams in a short period of time, which will increase the genetic variability, and so guarantee the conservation of this breed.     

Semen characteristics after vasectomy in the ram

The objective of this study was to monitor the changes in semen characteristics in vasectomized rams and to determine if infertility was present 14 days after vasectomy. Experiments were performed using five cross-breed rams, aged between 18 and 30 months. Semen was collected weekly by artificial vagina from 2 months before to 5 months after vasectomy. After sexual rest for 10 days, vasectomy was performed by the cranial midscrotal approach. In all ejaculates the volume, concentration, total sperm number, motility and morphology (normal spermatozoa, loose heads) were determined and sperm viability (SYBR-14/PI) was evaluated in all semen samples collected after vasectomy. In the first ejaculate obtained 14 days post vasectomy all rams showed a significant (P < 0.05) drop in mean volume (from 1.2 to 0.5 mL), total sperm count (from 5176.8 to 51.1 x 10(6)) and morphologically normal sperm (from 84.1 to 15.7%), when compared to the last prevasectomy collection. We could also demonstrate a positive correlation (r = 0.89) between the individual cumulative total number of spermatozoa after vasectomy and the scrotal circumference measured before vasectomy. Sperm motility and viability could never be demonstrated after vasectomy and normal spermatozoa continuously decreased concomitant with an increase in loose heads. On post mortem examination 5 months after surgery, spermatocele formation and multiple sperm granulomas were present in all five rams. Our results show that in the first ejaculate collected by artificial vagina 14 days after vasectomy, no motile and viable spermatozoa could be detected. Despite weekly collections during a 5-month period after sterilization, azoospermia could never be achieved.     

Observations of spermiogenesis and epididymal sperm maturation in the rufous hare wallaby, Lagorchestes hirsutus (Metatheria, Mammalia)

Acrosomal development in the early spermatid of the rufous hare wallaby shows evidence of formation of an acrosomal granule, similar to that found in eutherian mammals, the Phascolarctidae and Vombatidae. Unlike the other members of the Macropodidae so far examined, the acrosome of this species appears to be fully compacted at spermiation and extends evenly over 90% of the dorsal aspect of the nucleus. During spermiogenesis, the nucleus of the rufous hare wallaby spermatid showed evidence of uneven condensation of chromatin; this may also be related to the appearance of unusual nucleoplasm evaginations from the surface of the fully condensed spermatid. This study was unable to find evidence of the presence of Sertoli cell spurs or nuclear rotation during spermiogenesis in the rufous hare wallaby. The majority of spermatozoa immediately before spermiation had a nucleus that was essentially perpendicular to the long axis of the sperm tail. Nuclei of spermatozoa found in the process of being released or isolated in the lumen of the seminiferous tubule were rotated almost parallel to the long axis of the flagellum; complete parallel alignment occurred during epididymal maturation. At spermiation spermatozoa have characteristically small cytoplasmic remnants compared to those of other macropods. Unlike the majority of macropodid spermatozoa so far described, the spermatozoa of the rufous hare wallaby showed little evidence of morphological change during epididymal transit. There was no formation of a fibre network around the midpiece or of plasma membrane specializations in this region; the only notable change was a distinctive flattening of midpiece mitochondria and scalloping of the anterior mitochondrial sheath to accommodate the sperm head. Preliminary evidence from spermiogenesis and epididymal sperm maturation supports the classification of the rufous hare wallaby as a separate genus but also indicates that its higher taxonomic position may need to be re‐evaluated.