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1.
绒山羊精液冷冻保存技术的研究   总被引:1,自引:0,他引:1  
为了使绒山羊精液得到长期保存,充分发挥和提高优良种公羊的利用率,本实验对绒山羊精液冷冻保存技术进行了研究,比较了4种自行研制的保存稀释液的冷冻效果。结果表明:采用Ⅰ液(葡萄糖-卵黄-柠檬酸钠)冷冻保存绒山羊精液,解冻后精子活率(0.508±0.010)极显著高于Ⅱ液(葡萄糖-卵黄-乳糖-柠檬酸钠)(0.275±0.008)、Ⅲ液(葡萄糖-卵黄-蔗糖-柠檬酸钠)(0.354±0.012)和IV液(葡萄糖-卵黄-蔗糖-乳糖-柠檬酸钠)(0.319±0.006)(P<0.01);Ⅲ液极显著高于Ⅱ液(P<0.01)和显著高于Ⅳ液(P<0.05)。解冻后Ⅰ液的精子顶体完整率(59.4%±0.5%)极显著高于Ⅱ液(47.1%±0.8%)、Ⅲ液(52.4%±0.6%)和IV液(51.3%±0.5%)(P<0.01)。精液解冻后在室温(23±2)℃下避光培养,Ⅰ液中精子活率在5h内能够保持0.30以上,Ⅱ、Ⅲ液和Ⅳ液精子活率维持在0.3不到2h。  相似文献   

2.
猪精液细管法冷冻保存技术的研究   总被引:2,自引:0,他引:2  
为研制更为简易、高效的冷冻稀释液配方及冷冻程序,充分发挥优良种公猪的生产潜力,本实验采用细管法对种公猪精液冷冻保存技术进行了研究,比较了4种基础液配方稀释液冷冻效果,基础液I:葡萄糖、蔗糖、柠檬酸钠;基础液II:葡萄糖、蔗糖;基础液III:葡萄糖、乳糖、柠檬酸钠;基础液IV:葡萄糖、乳糖。结果表明:采用一步法稀释和IV液冷冻保存猪精液,其解冻后精子活率(0.501)极显著(P<0.01)高于I液(0.359)和III液(0.359),显著(P<0.05)高于II液(0.476),II液显著(P<0.05)高于I液和III液;解冻后IV液的精子顶体完整率(26.9%)显著(P<0.05)高于I液(22.4%)、II液(24.2%)和III液(22.5%),IV液冷冻解冻后精液的精子活率,在室温(23±2)℃下4h内能够保持0.30以上。  相似文献   

3.
本试验用0.5 mL细管作为冷冻载体对金华猪精液进行冷冻保存研究,比较3种冷冻稀释液及不同冷冻方法、解冻程序对金华猪精液冷冻的效果,以解冻后的精子活力、畸形率和质膜完整率为判定指标。结果表明:Ⅱ、Ⅲ号冷冻稀释液处理组解冻后精子的活力、畸形率和质膜完整性都明显地高于Ⅰ号冷冻稀释液(P0.05);Ⅱ号冷冻稀释液和Ⅲ号冷冻稀释液处理组之间没有明显差异(P0.05)。采用程序冷冻仪冷冻法,使用Ⅲ号冷冻稀释液冷冻保存精子,并在60℃,8 s条件下水浴解冻精子后,精子活力和质膜完整率最高分别为42.3%和50.3%,畸形率最低为17.7%。因此,采用程序冷冻仪冷冻法,使用Ⅲ号冷冻稀释液,在60℃,8 s条件下水浴解冻方法较为适合0.5 mL细管金华猪精液冷冻保存及解冻。  相似文献   

4.
为筛选陕北白绒山羊精液冷冻保存稀释液中最适的甘油及卵黄浓度,试验以三羟甲基氨基甲烷(Tris)6.057 0 g,蔗糖5.134 6 g,果糖1.500 0 g,柠檬酸钠3.318 6 g,青霉素10万IU,双蒸水200 m L配制成基础液,采用双因素正交试验研究不同浓度甘油、卵黄对精液冷冻保存的影响;采用一步稀释法冷冻保存陕北白绒山羊精液,复苏后检测活率、畸形率等确定精液冷冻稀释液最佳配方。结果表明:最佳冷冻稀释液配方为基础液80.5%+甘油6%+卵黄13.5%,精液冷冻、复苏后精子活率达到(37.2±0.5)%,精子畸形率为(11.2±0.5)%,质膜完整率为(64.2±0.5)%,均优于其他组,冷冻效果达到最佳,是保存山羊精液的冷冻稀释液最佳配方。  相似文献   

5.
通过对不同配方的稀释液、添加不同剂量的维生素B12、维生素C和复合维生素B对解冻后精子存活影响的试验,结果表明,配方Ⅰ、Ⅱ、Ⅲ三种稀释液制作的冻精解冻后精子活率均大于30.00%,Ⅰ液最高,其冷冻精液解冻后活率可达43.35%±0.85%,但Ⅰ液和Ⅱ液差异不显著(P>0.05),Ⅲ液最低,差异显著(P<0.05);顶体完整率和畸形率Ⅰ液最优,差异显著(P<0.05);Ⅱ液与Ⅲ液差异不显著(P>0.05);在Ⅰ稀释液中添加维生素B12对解冻后精子的活率、精子顶体完整率影响不大,但平均值都高于对照组,并且随着维生素B12量的增加,精子畸形率有继续降低趋势;添加复合维生素B 4mL/100mL,维生素C 4mL/100mL对犬精子均有保护作用。  相似文献   

6.
从稀释液、解冻液、解冻速率方面研究了猪精液冷冻保存的效果。结果表明:在八种稀释液中,用Ⅰ号稀释液制作的冷冻精液解冻后精子活率(33&#177;1.2)%优于其它组(P〈0.05);Ⅴ号解冻液解冻后精子活率(34&#177;2.4)%极显著高于Ⅰ、Ⅲ、Ⅳ号解冻液(P〈0.01),Ⅴ号解冻液解冻后精子存活时间506.6&#177;40.4h,极显著高于Ⅰ、Ⅱ、Ⅲ号解冻液(P〈0.01);以27.5℃/s的速率解冻,解冻后精子各项指标均为最高值。  相似文献   

7.
利用甘油和二甲基亚砜(DMSO)作为冷冻保护剂,以精子存活率为评价指标,研究了冷冻保护剂对香猪精液冷冻保存效果的影响。试验分工、Ⅱ、Ⅲ、Ⅳ4个试验组和1个对照组。以解冻后的精子活力、活率为判断标准,比较了4种冷冻保护液对香猪精液冷冻保存的影响。结果表明,试验Ⅰ、Ⅱ、Ⅳ组精子活率显著高于Ⅲ组(含5%甘油)(P〈0.05);试验Ⅰ、Ⅱ、Ⅳ组之间差异不显著(P〉0.05);Ⅰ组精子活率最高,达到53.10%。  相似文献   

8.
本试验的目的是分析在新西兰兔精液冷冻保存稀释液中分别添加不同浓度的海藻糖、透明质酸、维生素E(Ve)、超氧化物歧化酶(SOD)对兔精液冷冻保存效果的影响,以冻后精子活率、质膜完整性、顶体完整率等作为质量评定指标,筛选出效果较好的新西兰兔精液的冷冻保护剂种类及浓度。结果表明,精液冷冻保存稀释液中添加3种浓度的海藻糖均未提高兔精液冷冻后的精子活率、质膜完整率和顶体完整率(P0.05);添加0.5%和1%的透明质酸提高了兔精液冷冻后的精子活率(P0.05),但各组间质膜完整率和顶体完整率无显著差异;添加2 g/L Ve提高了兔精子4℃平衡后的活率、冷冻后精子活率、质膜完整率和顶体完整率(P0.05);添加4 000 IU的SOD提高了兔精子4℃平衡后的活率、冷冻后精子活率、质膜完整率和顶体完整率(P0.05)。结果证实,在新西兰兔精液冷冻保存稀释液中添加适宜浓度的Ve和SOD可提高兔精液冷冻后的精子活率、质膜完整率和顶体完整率。  相似文献   

9.
本试验采用不同的稀释液对兔精液进行冷冻保存,并比较了在稀释液中添加不同防冻剂以及平衡时间对兔精液冷冻保存效果的影响.结果表明:稀释液Ⅱ稀释的精液,解冻后,精子活率明显高于稀释液Ⅰ稀释的(P<0.01),其复苏率显著高于后者(P<0.05).以稀释液Ⅱ为基础液,添加不同浓度(27.3%,15%,12%,9%)的DMSO对兔精液冷冻保存,结果解冻后精子活率以15%及12%两组较好,其中添加15%的优于12%的,但差异不显著(P>0.05).选择不同种类的防冻剂(7%甘油与15%DMSO)比较时,发现7%甘油组解冻后精子活率明显低于15%DMSO组,二者差异极显著(P<0.01),其复苏率显著低于后者(P<0.05).以15%DMSO作为防冻剂,采用不同的平衡时间在5 ℃平衡,结果发现平衡30 min和60 min的解冻后精子活率较好,但差异不显著(P>0.05),而90 min和120 min的冷冻效果较差.  相似文献   

10.
旨在探讨辅酶Q10对绒山羊精液冷冻保存效果的影响。利用添加不同浓度辅酶Q10(4、40、400?滋g/mL)的精液冷冻稀释液对绒山羊精液样本进行冷冻保存,待冷冻精液解冻后,采用流式细胞仪和计算机辅助精液分析系统(CASAS)分别检测不同精液样本的精子活率、质膜完整率、顶体完整率、DNA完整率、线粒体膜电位和细胞内ROS水平。结果表明,当冷冻稀释液中添加浓度为40μg/mL辅酶Q10时,经历冷冻—解冻过程的绒山羊精液样本的精子活率、质膜完整率、顶体完整率均显著高于对照组(P<0.05);在冷冻稀释液中添加浓度为40μg/mL或400μg/mL的辅酶Q10均能显著提高线粒体膜电位并降低细胞内ROS水平(P<0.05)。综上所述,在冷冻稀释液中添加40μg/mL的辅酶Q10能够显著提高绒山羊精子抗氧化能力和冷冻保存效果。  相似文献   

11.
本试验旨在研究围产期奶牛饲喂过瘤胃胆碱(RPC)对泌乳性能、血液生化指标及繁殖性能的影响。试验采用单因素试验设计,选用60头年龄、胎次、预产期、上一胎次产奶量相近的健康围产期奶牛,随机分为3组,每组20头。Ⅰ组饲喂基础日粮,Ⅱ组和Ⅲ组在基础日粮上分别添加25 g/d和50 g/d RPC,饲喂期从产前3周至产后3周,共42 d。结果表明:Ⅱ组产奶量在产后1~8周显著高于Ⅰ组和Ⅲ组(P0.05);在产后第2周,Ⅲ组的乳脂率、乳蛋白率显著高于Ⅰ组(P0.05);在整个试验期,Ⅱ组的谷丙转氨酶含量显著低于Ⅰ组(P0.05),Ⅲ组的天门冬氨酸转氨酶显著含量低于Ⅰ组(P0.05);产后第1周和第2周,Ⅱ组的β-羟丁酸、非酯化脂肪酸含量显著低于Ⅰ组(P0.05);Ⅱ组的甘油三酯含量显著高于Ⅰ组和Ⅲ组(P0.05),Ⅲ组的总胆固醇含量显著高于Ⅰ组(P0.05);日粮中添加RPC可以显著提高情期受胎率(P0.05),显著缩减奶牛空怀天数(P0.05),也对产后初次配种时间的缩短和配种次数的降低有影响。日粮中添加RPC可提高围产期奶牛生产性能,对血液生化指标和繁殖性能产生有利影响,本试验条件下RPC最佳添加剂量为每头牛25 g/d。  相似文献   

12.
The aim of the present study was to investigate the influence of various centrifugation methods on sperm loss and quality of frozen-thawed semen. From at a total of 8 Warmblood stallions of the National Stud Farm in Avenches, 3 ejaculates each were collected and seminal plasma was removed using 3 different centrifugation regimes. In method I (reference method) centrifugation occurred by a speed of 600 x g during 10 minutes. In method II 1000 x g was used during 2 minutes while in method III centrifugation was performed by 2000 x g during 2 minutes. After centrifugation 90%, of the supernatant was removed and sperm loss calculated. After resuspension of the pellet with freezing medium, functional membrane integrity was evaluated by HOS-test and motility determined. In frozen-thawed semen motility, viability as well as functional membrane integrity (HOS-test) and acrosome status using chlortetracyclinassay (CTA) were assessed. Our results demonstrate that mean sperm loss (I, 1.9%; II, 8.7%; III, 3.7%) was significantly (P < 0.05) different between the three centrifugation regimes. Regarding semen quality of frozen-thawed semen, HOS in method III (52.1%) was significantly lower than in methods I (55.5%) and II (55.3%). Evaluation of the acrosome status by CTA showed that more than 70% of sperm cells were capacitated and 25% capacitated and acrosome reacted. From our results we conclude that sperm loss and functional membrane integrity (HOS-test) in frozen-thawed semen were significantly influenced by the centrifugation regime. Therefore, stallion semen should be centrifuged at 600 x g during 10 minutes before freezing in order to obtain low sperm loss and a good quality of frozen-thawed semen.  相似文献   

13.
试验旨在研究白藜芦醇对山羊冷冻精子质膜、DNA完整性和温度耐受性的影响。采用假阴道法采集8只云上黑山羊精液,用含不同浓度(0、0.1、1、10和20 μmol//L)白藜芦醇的Optidyl稀释液稀释后进行细管分装,对照组不添加白藜芦醇。在5 ℃平衡4 h后,将细管于液氮蒸气中预冻10 min,最后在液氮中保存30 d。37 ℃水浴解冻后,采用低渗耐受性试验检测质膜完整性和温度耐受性,精子染色质扩散法检测DNA碎片率等指标。结果显示,10 μmol/L白藜芦醇冷冻组精子弯尾率显著高于其他各处理组(P<0.05),而其他各冷冻组之间无显著性差异(P>0.05);10 μmol/L白藜芦醇冷冻组精子DNA碎片率极显著高于鲜精组(P<0.01),极显著低于未添加白藜芦醇冷冻组(P<0.01)。温度耐受性试验结果表明,不同浓度白藜芦醇冷冻组精子37 ℃水浴1 h后的精子弯尾率以10 μmol/L冷冻组最高,与其他各冷冻组间差异极显著(P<0.01);精子弯尾率随着孵育时间的延长而呈逐步下降的趋势,当孵育4 h时,10 μmol/L白藜芦醇冷冻组精子弯尾率与对照组无显著差异(P>0.05)。透射电镜结果表明,10 μmol/L白藜芦醇组精子质膜完整率显著高于不添加白藜芦醇对照组(P<0.05)。上述结果表明,在冷冻稀释液中添加白藜芦醇可显著改善山羊冻精质膜状态、DNA完整率和温度耐受性,其最佳作用浓度为10 μmol/L,但白藜芦醇是否能改善山羊冻精的人工授精效果还有待进一步研究。  相似文献   

14.
1992只1日龄AA肉鸡随机分为4个处理组,饲喂四种不同的日粮。42日龄测定各组肉鸡组织及血清抗氧化指标的水平。结果表明:(1)除心脏和血清外,各试验组MDA含量均与IV组差异显著(P<0.05)。(2)肝脏中SOD变化较明显,各试验组均高于IV组,且差异显著(P<0.05)。心脏各组之间差异不显著。(3)心脏GSH-Px含量以III、II组较高,且均与IV组差异显著。血清以II组最高,且与其他各组之间差异显著(P<0.05)。(4)心脏T-AOC含量变化较大,各试验组均高于IV组,且差异显著(P<0.05)。血清以II组最高,且与其他试验组差异显著(P<0.05)。  相似文献   

15.
During the cryopreservation process, the level of polyunsaturated fatty acids, especially docosahexaenoic acid (DHA), in the sperm plasma membrane decreases significantly because of lipid peroxidation, which may contribute to sperm loss quality (i.e. fertility) of frozen–thawed semen. The aim of this study was to investigate the effect of supplementation of DHA (fish oil) in freezing extender II on frozen–thawed semen quality. Semen from 20 boars of proven motility and morphology, were used in this study. Boar semen was split into four groups, in which the lactose–egg yolk (LEY) extender used to resuspend the centrifuged sperm pellet was supplemented with various levels of fish oil to reach DHA level of 1X (group I, control, no added fish oil), 6X (group II), 12X (group III) and 18X (group IV). Semen solutions were frozen by using a controlled rate freezer. After cryopreservation, frozen semen was thawed and evaluated for progressive motility, viability by using SYBR‐14/Ethidiumhomodimer‐1 (EthD‐1) staining and acrosome integrity by using FITC‐PNA/EthD‐1 staining. There was a significantly higher (p < 0.001) percentage of progressive motility, viability and acrosome integrity in DHA (fish oil) supplemented groups than control group. Generally, there seemed to be a dose‐dependent effect of DHA, with the highest percentage of progressive motility, viability and acrosome integrity in group‐III. In conclusion, supplementation of the LEY extender with DHA by adding fish oil was effective for freezing boar semen as it resulted in higher post‐thaw plasma membrane integrity and progressive motility.  相似文献   

16.
本试验旨在探讨海藻糖对猪精子冷冻效果以及精子内活性氧(ROS)的含量影响。试验分对照组和4个海藻糖处理组(0.025,0.05,0.1和0.2 mol/L)。精子冷却后,添加0.1 mol/L海藻糖处理组精子活力显著(P<0.05)高于对照组,而精子内和稀释液中各组间ROS发生量都没有显著的差异。精子冷冻解冻后,添加0.05 mol/L海藻糖处理组的精子活力显著(P<0.05)高于对照组;添加0.05 mol/L和0.1 mol/L海藻糖处理组的精子生存率显著(P<0.05)高于对照组;添加0.1 mol/L海藻糖处理组顶体完整的精子百分比显著(P<0.05)高于对照组;4个海藻糖处理组膨胀精子百分比都显著(P<0.05)高于对照组;添加0.025 mol/L海藻糖处理组ROS水平显著(P<0.05)低于对照组。结果表明:海藻糖对精子冷冻保存是有益的,且能抑制精子内ROS的发生,但它的作用机制有待于进一步的研究。  相似文献   

17.
摘要:本试验旨在研究不同方法处理的玉米青贮饲喂肉牛效果对比,选择体重340kg左右的西门塔尔杂交牛30头,随机分为3组,保证精饲料不变,粗饲料分别饲喂3种不同方法处理的玉米青贮,其中试验Ⅰ组为全株玉米青贮、试验Ⅱ组添加剂全株玉米青贮、试验Ⅲ组玉米秸秆黄贮,试验期70d。结果表明:1)试验Ⅱ组的平均日增重极显著高于试验Ⅰ组、试验Ⅲ组(P<0.01),分别比Ⅰ组、Ⅲ组高出17.57%、65.71%;Ⅲ组干物质采食量显著高于Ⅰ组、Ⅱ组(P<0.05);Ⅰ组和Ⅱ组料重比极显著低于Ⅲ组(P<0.01)。试验Ⅱ组养殖效益最高为14.14元?天-1?头-1,比试验Ⅰ组高5.05元,比试验Ⅲ组高15.74元。综上,添加剂全株玉米青贮饲喂肉牛效果和养殖效益最佳,全株玉米青贮、玉米秸秆黄贮次之。  相似文献   

18.
The present investigation was carried out to study the effect of various levels of dissolved oxygen (DO) on reactive oxygen species (ROS) and cryocapacitation‐like changes in bull sperm. Egg yolk–Tris–glycerol (EYTG) extender was split into four subextenders; viz., Extender I (control; no flushing with liquid nitrogen (LN2)), Extender II, Extender III and Extender IV were flushed with LN2 for 40, 16 and 8 min, respectively. The DO levels were standardized to 11.7, 2, 4 and 8 ppm, respectively, in control (Extender I), Extender II, Extender III and Extender IV. Ejaculates with mass motility of ≥ 3+ were divided into group I (diluted with Extender I), group II (diluted with Extender II), group III (diluted with Extender III) and group IV (diluted with Extender IV) up to 80 × 106 sperm/ml. Extended semen samples were packed in French mini straws (0.25 ml), equilibrated and cryopreserved. Semen samples were evaluated at prefreeze and post‐thaw stage for various parameters (DO, progressive motility (PM), viability (VIB), acrosomal integrity (AI), hypo‐osmotic swelling (HOS) test, ROS, cholesterol (C) and phospholipid (P). The percentage of PM, VIB, AI, HOS test, cholesterol (C) and phospholipid (P) levels, and capacitated sperm were significantly (p < 0.05) higher in groups III and IV as compared to groups I and II. However, the acrosome‐reacted sperm (%; pattern AR) were significantly (p < 0.05) decreased in group III as compared to all other groups. Besides the proportion of sperm displaying tyrosine‐phosphorylated pattern, EA (fluorescence at both equatorial and anterior acrosomal regions, i.e. high capacitation level) was significantly (p < 0.05) reduced in group III compared to all other groups. In conclusion, varying DO levels in the extender significantly affect sperm quality, ROS production and capacitation‐like changes in bulls.  相似文献   

19.
本实验旨在探讨添加低剂量大豆卵磷脂稀释液对绵羊精液低温保存效果。实验一采用6个浓度(0%、0.25%、0.5%、0.75%、1.0%、1.25%)大豆卵磷脂替代TRIS专利稀释液中卵黄低温保存绵羊精液,在第0、1、4、7、10、12、18天检测精子活率、顶体完整率;实验二选用实验一中最优添加组(0.5%组)和TRIS专利稀释液制成粉剂低温保存绵羊精液,在保存第0、1、4、7、10、12天对精子活率和顶体完整率进行测定,并在保存第10天对绵羊进行人工授精。结果表明:实验一中,0%组从第1天精子活率低于其他组(P<0.05),0.25%组精子活率观测值从第10天开始低于0.25%以上浓度组(P<0.05),0.5%、0.75%、1.0%、1.25%组保存第10天精子活率均大于50%,0.5%组保存第18天精子活率高于1.0%、1.25%组(P<0.05);各组顶体完整率缓慢下降,各时间点均无显著性差异;实验二中,0.5%组与TRIS组在各时间点的精子活率、顶体完整率与受胎率均无显著性差异,保存第10天精子活率均高于50%;0.5%组受胎率为65.49%,略低于TRIS组67.65%(P>0.05)。本实验条件下,绵羊精液低温保存稀释液中添加0.5%大豆卵磷脂替代卵黄效果最佳。  相似文献   

20.
选用1日龄樱桃谷肉鸭1600羽,随机分成4组,分别饲喂4种不同处理的日粮,以研究酶制剂在肉鸭日粮中应用效果。对照组饲喂基础日粮不添加酶制剂;试验1组为饲喂基础日粮并添加酶制剂250 g/t;试验2组和3组分别饲喂能量降低250.8 MJ/kg和334.4/kg基础日粮,并添加酶制剂250 g/t。结果表明:在基础日粮和降低能量的日粮中添加酶制剂,均能提高肉鸭日增重,改善饲料转化率和能量消化率。其中,基础日粮中添加酶制剂,能显著提高肉鸭日增重和饲料利用率(P<0.05),能量消化率最高,按毛利润计算,试验组肉鸭收益率分别比对照组提高了7.02%、4.45%和5.26%。  相似文献   

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