不同稀释液配方对牛冻精品质的影响

选用3种稀释液配方分别对6头种公牛精液进行稀释、封装、冷冻,并检查种公牛冻精解冻后的精子活力、畸形率、顶体完整率、冻后废弃率、存活时间及镜检感光度.结果表明：3种不同稀释液配方对种公牛精液冻后活力影响差异均显著（P＜0.05）,Ⅰ稀释液生产冻精的畸形率极显著高于Ⅱ稀释液和Ⅲ稀释液（P＜0.01）,3种稀释液冻精精子顶体完整率之间差异均极显著（P＜0.01）,Ⅲ稀释液与Ⅰ稀释液和Ⅱ稀释液间对牛精液所生产冻精的冻后废弃率影响均差异显著（P＜0.05）,Ⅰ稀释液与Ⅱ稀释液和Ⅲ稀释液间对牛精液所生产冻精的存活时间影响差异也显著（P＜0.05）,Ⅲ稀释液生产的冻精精子感光度优于Ⅰ稀释液和Ⅱ稀释液,其余各项指标差异均不显著（P＞0.05）.因此,可用自配Ⅱ稀释液替代进口专用Ⅲ稀释液.     

2种稀释液对公猪精液冷冻保存效果的影响

试验为探究2种不同冷冻稀释液对公猪精液稀释冷冻效果的影响。试验采用手握法采集同一头公猪精液,将采集的精液分为2组,进行液氮熏蒸制作细管冻精,分别使用Ⅰ号冷冻稀释液和Ⅱ号冷冻稀释液对猪精液进行冷冻保存,24 h后检测2种冷冻稀释液细管冻精的活力。结果显示,Ⅰ号冷冻稀释液冷冻解冻后的精子活力显著高于Ⅱ号冷冻稀释液(P0.05),同一种稀释液距液氮面5 cm进行熏蒸冷冻的效果较距液氮面4 cm冷冻效果好,但差异不显著(P0.05)。研究表明,利用Ⅰ号冷冻稀释液在距液氮面5 cm处进行液氮熏蒸冷冻可获得较好的公猪冷冻精液。     

不同稀释方法对小型宠物犬精液冷冻效果影响

为了研究Tris-果糖稀释液在不同稀释方法下对小型宠物犬精液冷冻的效果,选取常见的3个小型宠物犬品种共计6只犬进行试验,精液稀释过程分别采用一步稀释法和两步稀释法。结果表明:冷冻精液解冻后各组犬精液的同一剂型间的精子活力差异均不显著(P0.05);一步稀释法中的颗粒冻精与0.25 mL细管冻精和0.50 mL细管冻精相比,解冻后精子活力差异均显著(P0.05),而0.25 mL细管冻精与0.50 mL细管冻精的解冻后精子活力差异极显著(P0.01);采用两步稀释法的颗粒冻精、0.25mL细管冻精及0.50 mL细管冻精的解冻后精子活力组间差异均不显著(P0.05)。用Tris-果糖稀释液稀释精液时,使用两步稀释法对不同冻精剂型的精子活力影响不明显。     

不同浓度抗生素的稀释液对牛冷冻精液质量的影响

本试验用添加了不同浓度抗生素的稀释液对5头种公牛精液进行稀释、封装和冷冻,检查牛冻精解冻后的精子活力、畸形率和细菌数。结果表明,抗生素添加范围在1 000～2 000IU/mL内,冻精活力≥35%,细菌数控制在30个左右,冻精质量符合国家标准。     

不同配方稀释粉对公猪鲜精保存的效果分析

精液稀释液成本占人工授精整体成本费用很大的比例,因此研究出经济高效的稀释液对降低人工授精成本有重要意义。本文通过成对比较实验,用5种不同配方稀释粉按照国内AI标准技术对种公猪的合格鲜精进行稀释保存,观察不同配方稀释粉对公猪鲜精保存时间长短、精子活力、精子畸形率的影响。结果表明:配方hotboar 对公猪精液的保存效果最为显著,而且其通用性及成本也显著低于现有商品化稀释粉。     

“靓精”对稀释猪精液保存质量的影响

<正>种公猪精液在采集、稀释液配制和精液稀释过程中,会因外界环境或操作疏忽而使精液或稀释液受到某些病原微生物的污染,影响稀释精液的质量和保存时间。"靓精"为一种精液净化保护剂,含5%聚维酮碘,能抑制或杀灭病原微生物,减少病原微生物对精子质量的影响,提高精子活力,延长保存时间。本试验在公猪精液中加入靓精,通过检测稀释精液在保存期间的精子活力和精子畸形率,观察靓精对稀释精液保存质量的影响。     

黄芪多糖对猪精液冷冻保存效果的影响

为了评价黄芪多糖（Astragalus polysaccharides）对外来公猪精液冷冻保存的影响情况,为猪精液冷冻稀释液配方的改良提供理论依据,试验采集美系长白、大约克与杜洛克3种公猪的精液,用添加不同浓度（0、0.01%、0.02%、0.03%、0.04%、0.05%、0.06%）黄芪多糖的冷冻稀释液稀释,0.25 mL塑料细管分装并冷冻,测定解冻后精子活力、畸形率及顶体完整率,并进行相同浓度3种公猪之间和同种公猪不同浓度之间的比较。结果表明,在相同黄芪多糖浓度下,仅杜洛克公猪冻后精子顶体完整率在不添加黄芪多糖时显著高于大约克公猪（P<0.05）,其余均无显著差异（P>0.05）;每种公猪的最佳黄芪多糖添加浓度均为0.04%,在该浓度下精液冻后质量均显著优于对照组（P<0.05）;各种公猪最佳黄芪多糖添加浓度下的精液冻后质量指标之间均无显著差异（P>0.05）。总之,稀释液中添加0.04%黄芪多糖在长白、大约克与杜洛克3种公猪的精液冷冻都可以取得较好的效果。     

不同配方稀释粉对公猪鲜精保存的效果分析

精液稀释液成本占人工授精整体成本费用很大的比例，因此研究出经济高效的稀释液对降低人工授精成本有重要意义。本文通过成对比较实验，用5种不同配方稀释粉按照国内AI标准技术对种公猪的合格鲜精进行稀释保存，观察不同配方稀释粉对公猪鲜精保存时间长短、精子活力、精子畸形率的影响。结果表明：配方hotboar^ 对公猪精液的保存效果最为显著，而且其通用性及成本也显著低于现有商品化稀释粉。     

冷冻稀释液和抗氧化剂对金华猪精液冷冻效果的影响

为了探究不同冷冻稀释液及抗氧化剂对金华猪精液冷冻效果的影响,试验通过手握法采集健康的20月龄纯种金华猪公猪精液,采用两种常用的商品冷冻稀释液(A、B)稀释精液,然后液氮冻存1 d,解冻后测定精液精子活力、顶体完整率和质膜完整率指标,筛选最适金华猪精液冷冻保存的稀释液;在最适冷冻稀释液中添加20,30,40,50μmol/L表没食子儿茶素没食子酸酯(epigallocatechin gallate, EGCG),以未添加EGCG和上述添加EGCG的冷冻稀释液稀释金华猪精液,然后液氮冷冻保存精液1 d,解冻后测定精液精子活力、顶体完整率、质膜完整率及抗氧化指标[包括活性氧(reactive oxygen species, ROS)、丙二醛(malondialdehyde, MDA)含量及超氧化物歧化酶(superoxide dismutase, SOD)和过氧化氢酶(catalase, CAT)活性],筛选EGCG的最适添加量。结果表明：两种商品冷冻稀释液的精子活力、顶体完整率、质膜完整率差异不显著(P>0.05),但考虑到价格成本,选择B冷冻稀释液作为后续试验的冷冻稀释液。随着EG...     

BMY牛冷冻精液质量控制及影响因素研究

[目的]为了加大BMY牛的推广应用力度和提高人工授精受胎率,开展了BMY牛冷冻精液质量控制研究,优选出冷冻稀释液及得出冷冻精液质量控制技术程序。[方法]采用不同的初始冷冻温度、不同种类的稀释液、不同的冷冻方法对BMY牛精液冷冻及解冻效果进行试验。[结果]不同的初始冷冻温度、不同种类的稀释液、不同的冷冻方法,BMY牛精液冷冻解冻效果各异。初始冷冻温度为-121--140℃时,TRIS液为基础稀释液添加糖类和氨基酸一步法稀释BMY牛精液冷冻6-10 min BMY牛冷冻精液解冻效果较好,用程控冷冻仪冷冻BMY牛精液,同样获得良好的解冻效果,解冻活力达到0.372±0.026。BMY牛冷冻精液平均解冻活力可达0.357±0.029以上,精子解冻复苏率达50%以上。精子畸形率平均为16.8%±4.26%,BMY牛采精成功率为75.3%。[结论]全放牧条件下BMY牛电刺激采精法获得很好效果,精液质量好,更有利于种质资源的保存和利用。     

提高奶牛细管冻精精子活力的试验研究

为了提高奶牛细管冻精精子的活力,试验探索了稀释液种类、最佳熏蒸距离、最佳冷冻温度、最佳熏蒸时间、不同解冻温度及时间对精子活力的影响。结果表明:精子在由柠檬酸钠和果糖组成的稀释液中存活时间长,在三羟甲基氨基甲烷稀释液中冷冻后精子活力高于其他稀释液;牛细管冻精最佳熏蒸距离为2.5 cm,时间影响不显著(5～10 min均可);用50℃温水解冻15 s的精子活力比其他解冻温度和时间时的精子活力要好。     

Study on Technology of Black Silkies Chicken Semen Freezing by DMA Pellet

The aim was to explore the effects of different kinds of dilution and thawing devices on the N,N-dimethylformamide (DMA) pellet frozen semen of Black Silkies. Firstly,the motility and fertility of the frozen semen thawed by different dilutions were compared;Then,the motility of the frozen semen was compared when the pellets were thawed using different tube and different number.Finally,the motility and fertility of the sperm thawed by three kinds of thawing devices (thermostat water bath,hotfunnel and hotplate ) were tested. The results showed that:①There was similar order of the sperm motility and fertility in the different dilution groups (LR > F > B > L),and there was significant difference among those groups (P < 0.05).②The motility was the best when the frozen semen was thawed with large thin-wall glass tube at 60℃.③The best temperature range of the 3 devices was different. The highest motility for thermostat water bath was 50 to 60℃ (0.51 to 0.59),and thermostat hotfunnel was 40 to 45℃ (0.42 to 0.46),while thermostat hotplate was 50 to 55℃ (0.61 to 0.63).There was no significant difference of the motility in the optimum temperature range for each device (P > 0.05).④The fertility of the different devices in their best thawing temperature was 26.91% (55℃,thermostat hotplate),23.08% (60℃, thermostat water bath), 20.93% (40℃, thermostat funnel),respectively,and there was no significant differences among those groups (P > 0.05).Therefore,the efficiency thawing condition for the Black Silkies frozen semen was the LR diluent,DMA cryoprotectant,pellet freezing,thawed in the thermostat hotplate at 54.9℃.     

提高牛细管冻精精子活力的试验研究

本文从细管冻精的3个关键技术环节研究了稀释液的种类对精子活力与存活的影响,确定了细管冻精精子在液氮冷冻度过冰晶期对其损伤最小的最佳熏蒸高度（最佳冷冻温度）和最佳熏蒸时间,并且对成品冷冻的细管冻精不同解冻温度及时间进行研究。由柠檬酸钠和果糖组成的稀释液精子存活时间长,Tris稀释液冷冻后精子活力高于其他配方;牛细管冻精最佳熏蒸距离为2cm,时间影响不显著,7~9min均可;用50℃温水15s解冻精子的活力最高。     

黑丝羽乌骨鸡精液DMA颗粒冷冻技术研究

为研究不同稀释液与解冻装置对黑丝乌骨鸡N,N-二甲基甲酰胺（N,N-dimethylformamide,DMA）颗粒冻精解冻后精子质量的影响,试验首先采用不同稀释液对精液进行稀释并比较其解冻后精子活力与人工输精的受精率;其次,选取不同解冻管及冻精颗粒数进行恒温水浴解冻,比较其活力;最后,依据解冻后的精子活力,筛选恒温水浴、恒温漏斗、恒温板3种解冻装置各自的最佳解冻温度,并利用各自最佳解冻温度解冻后的精液进行人工输精,检测受精率。结果显示：①不同稀释液组的精子活力与受精率高低趋势一致,为LR > F > B > L组,且各组之间差异显著（P < 0.05）。②在60℃恒温水浴中,用薄壁大玻璃管解冻的精子活力最好。③不同解冻装置有各自最佳解冻活力的温度范围,恒温水浴为50~60℃（0.51~0.59）、恒温漏斗为40~45℃（0.42~0.46）、恒温板为50~55℃（0.61~0.63）,每种装置最佳温度段内的精子活力差异不显著（P > 0.05）。④3种解冻装置最佳解冻状态相比：在精子活力上,60℃恒温水浴与55℃恒温板分别显著高于40℃恒温漏斗（P < 0.05）,但60℃恒温水浴与55℃恒温板之间差异不显著（P > 0.05）;在受精率上,55℃恒温板最高（26.91%）,60℃恒温水浴次之（23.08%）、40℃恒温漏斗最低（20.93%）,三者之间差异不显著（P > 0.05）。因此,黑丝羽乌骨鸡精液应采用LR稀释液、DMA冷冻保护剂及颗粒冷冻技术,在54.9℃恒温板解冻可获得较高的受精率。     

Effect of green buffer storage on the fertility of fresh camel semen after artificial insemination

Artificial insemination (AI) is one of the most widely used reproductive technologies, and there is considerably interest in commercializing this technology in camels. Storage of semen extender frozen (at -20 °C) is of considerable interest to scientists working with camels, as transportation of diluents at refrigeration temperature is not always possible given the hot, arid and remote conditions that dromedary camels exist in. Therefore, this study was conducted to compare the fertility of fresh camel semen, after dilution in fresh or frozen-thawed green buffer (GB), after AI into single and multiple ovulating female camels. No differences were observed in any sperm characteristics (motility, membrane integrity, acrosome integrity or morphology) when semen was diluted in fresh or frozen-thawed GB (p>0.05). Sperm motility was increased by dilution (fresh: 70.7 ± 4.9% and frozen: 68.8 ± 3.1%) compared with the motility of sperm in neat semen (35 ± 2.85%; p<0.05), and sperm motility changed from oscillatory to forward progressive after dilution. Pregnancy rates were higher (p<0.05) for single ovulating camels inseminated with semen diluted in fresh (72.7%) compared with frozen-thawed GB (27.3%), and fertilization rates were also higher (p<0.05) for multiple ovulating camels inseminated with semen diluted in fresh (83.3%) compared with frozen-thawed GB (11.1%). These results clearly demonstrate the detrimental effect of freezing and thawing semen diluent on the fertility of fresh camel semen. However, further studies are required to elucidate the mechanism responsible for this reduction in fertility. Moreover, these results demonstrate that the fertility of fresh camel semen diluted in fresh GB is high enough to be considered commercially viable.     

AMPK激活剂在绵羊精液冷冻保存中的作用研究

旨在研究AMPK激活剂二甲双胍（metformin，Met）和阿卡地新（acadesine，AICAR）对绵羊精液冷冻保存效果的影响。本研究首先在冷冻基础稀释液中分别添加不同浓度（0、100、200、300、400、500 μmol·L^-1）的Met和AICAR，冷冻解冻后根据精子活力、运动性能和结构完整性指标筛选出最佳的添加浓度（400 μmol·L^-1 Met、200 μmol·L^-1 AICAR）；然后分别使用不同的冷冻稀释液（对照组：稀释液；Met组：含400 μmol·L^-1 Met的稀释液；AICAR组：含200 μmol·L^-1 AICAR的稀释液）冷冻精液，解冻后检测精子中AMPK蛋白表达、顶体酶活性、代谢指标、线粒体功能以及抗氧化酶活性。结果表明，稀释液中添加400 μmol·L^-1 Met和200 μmol·L^-1AICAR均可显著提高解冻后精子活力、运动性能及精子结构完整性（P<0.05），其中400 μmol·L^-1 Met组精子总活力达43.20%，顶体完整率为91%，质膜完整率为46%。与对照组相比，Met组和AICAR组解冻后精子中AMPK磷酸化水平显著升高（P<0.05）；顶体酶活性显著提高（P<0.05）；丙酮酸水平显著下降（P<0.05），乳酸脱氢酶活性、乳酸以及ATP含量均显著升高（P<0.05）；与对照组相比，Met和AICAR组稀释液更有利于维持线粒体膜电位（P<0.05），提高ATP酶（P<0.05）以及抗氧化酶的活性（P<0.05）。添加适当浓度的AMPK激活剂可以提高绵羊精液冷冻保存的效果。     

Study on the Role of AMPK Activator in Cryopreservation of Sheep Semen

This study aimed to investigate the effects of AMPK activators metformin (Met) and acadesine (AICAR) on sheep semen cryopreservation. Firstly, Met and AICAR with different concentrations (0, 100, 200, 300, 400, 500 μmol·L^-1) were added into the frozen diluent. After freezing and thawing, the optimal concentration (400 μmol·L^-1 Met, 200 μmol·L^-1 AICAR) were selected based on sperm motility, motion performance and membrane integrity; Secondly, the collected semen was froze using different frozen diluents (control group:diluent; Met group:diluent + 400 μmol·L^-1 Met; AICAR group:diluent + 200 μmol·L^-1 AICAR). After thawing, the sperm AMPK protein expression, acrosomal enzyme activity, metabolic index, mitochondrial function and antioxidant enzyme activity were examined. The results showed that the addition of 400 μmol·L^-1 Met and 200 μmol·L^-1 AICAR could significantly improve sperm motility, motion performance and membrane integrity(P<0.05) after thawing. In 400 μmol·L^-1 Met group, the total sperm motility, acrosome integrity rate and plasma membrane integrity rate were 43.20%, 91% and 46%, respectively. Compared with the control group, the level of AMPK phosphorylation in the sperm of the Met and AICAR groups was significantly increased after thawing (P<0.05), the acrosome enzyme activity of sperm was significantly increased(P<0.05); the pyruvate level was significantly decreased (P<0.05), the lactate dehydrogenase activity, lactic acid content, and ATP content were significantly increased(P<0.05). Compared with the control group, the dilution of Met group and AICAR group was more conducive to maintain mitochondrial membrane potential (P<0.05), increase ATPase and antioxidant enzyme activity (P<0.05). The addition of appropriate concentrations of Met and AICAR could improve semen quality of cryopreservation in sheep.     

3种稀释液对乐至黑山羊精液品质的影响

旨在评价不同种类稀释液对乐至黑山羊精液品质的影响。配制柠檬酸-Tris（1号）、磷酸盐（2号）和OviXcell（3号）3种稀释液,采集8只乐至黑山羊新鲜精液,采用上述稀释液进行冷冻保存;测定并比较添加不同稀释液冷冻保存的山羊精液在采集后、平衡后以及解冻后的精子活力、精子畸形率、精子顶体完整率。结果表明：在3种稀释液中,添加OviXcell稀释液（3号）的精液其解冻后精子活力和顶体完整率均最高,精子畸形率最低。提示OviXcell稀释液更适用于乐至黑山羊精液的体外冷冻保存。     

冷冻稀释液中添加大豆卵磷脂对梅花鹿冻融精子质量的影响

【目的】 探究在冷冻稀释液中添加大豆卵磷脂代替10%卵黄对梅花鹿精液冷冻保存效果的影响,为梅花鹿人工授精体系的完善提供参考。【方法】 采用电刺激法采集梅花鹿精液,以精液冷冻稀释液中分别添加1%、2%、3%、4%和5%大豆卵磷脂代替10%卵黄作为试验组,添加20%卵黄作为对照组,分别进行各组精液冷冻保存。5 d后,进行精液解冻,检测解冻后各组精子的活力、质膜完整率、顶体完整率、线粒体活性、存活时间,筛选合适浓度的大豆卵磷脂。选取4~5岁健康雌性梅花鹿,肌肉注射300 IU孕马血清促性腺激素（PMSG）和0.4 mg氯前列醇钠进行同期发情处理,发情后第20 h用20%卵黄组与筛选出的大豆卵磷脂组冻精进行人工输精,输精后30 d使用B超检测仪检测妊娠情况,统计妊娠率。【结果】 与对照组相比,1%大豆卵磷脂组冻融后的精子活力、向前活动力、快速前进活力、活率、质膜完整率、顶体完整率及线粒体活性均显著提高（P<0.05）;随着稀释液中大豆卵磷脂浓度的增加,其冻融后精子活力、向前活动力、快速前进活力、活率、质膜完整率、顶体完整率以及线粒体活性呈下降趋势,精子存活时间也随浓度的增加而减少。1%大豆卵磷脂组冻融精子人工授精梅花鹿的妊娠率为61.11%,高于对照组、2%和3%大豆卵磷脂组,但差异均不显著（P>0.05）。【结论】 在梅花鹿精子冷冻稀释液中添加1%大豆卵磷脂替代10%卵黄,能有效提高梅花鹿冻融精子的质量,为进一步筛选新型梅花鹿精液冷冻稀释液提供理论基础。     

Changes in proacrosin levels during preservation of ram semen

The percentual change in the content of pro-acrosin taking place in ram semen preserved for a short and long time was examined in the period from April to October. Two diluents for keeping semen at the temperature of 16 degrees C and one diluent for keeping semen at 3 to 4 degrees C were used in short-time preservation. The content of pro-acrosin was measured 2, 8 and 12 hours after dilution. The lactoso-yolk diluent and the diluent after Milovanov (1980) were used for cryopreservation. The content of pro-acrosin was examined before and after semen freezing. In short-time preservation, no statistically significant decrease of pro-acrosin content was demonstrated in the H Milch diluent (Peter, 1975) at the storage temperature of 16 degrees C and in the diluent after Milovanov (1980) at the temperature of 3 to 4 degrees C. In the diluent prepared after Milovanov (1980) a significant decrease of pro-acrosin content during preservation was recorded at the storage temperature of 16 degrees C. When the short-time preservation diluents were compared, significant differences in pro-acrosin content were found between them. In the long-time preservation diluents a significant difference in pro-acrosin content was found before and after semen freezing; the difference between the short- and long-time preservation diluents was also significant. A positive correlation was found between sperm activity and pro-acrosin content.