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实验研究了不同成熟培养时间的牛卵母细胞玻璃化冷冻及胞质内单精子注射(ICSI)后的受精效果。结果表明:成熟后的新鲜牛卵母细胞按照ICSI注射方法穿刺而不注射精子组与未经穿刺的对照组相比,孤雌激活后的卵裂率、囊胚发育率及囊胚细胞数无显著差异(P>0.05);成熟培养16h(MⅠ)和23h(MⅡ)卵母细胞冷冻解冻后形态正常率均显著低于新鲜对照组(76.66%、87.33%vs100.0%)(P<0.05),冷冻解冻后二者分别成熟培养至24h,ICSI后胚胎的囊胚发育率(5.29%、14.41%)显著低于新鲜对照组(24.40%)(P<0.05);成熟培养23h与成熟培养16h的卵母细胞冷冻解冻后形态正常率及ICSI后囊胚发育率(14.41%vs5.29%)均有显著性差异(P<0.05)。实验证明,ICSI操作不会影响卵母细胞发育潜力;玻璃化冷冻影响卵母细胞解冻后形态正常率以及ICSI后胚胎的发育能力;成熟培养23h比16h的卵母细胞冷冻保存后经ICSI的胚胎发育潜力高。 相似文献
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精子不同处理和胰岛素不同浓度对猪卵母细胞胞质内单精子显微受精的影响 总被引:1,自引:0,他引:1
探讨了分别使用新鲜、冷冻和超声波断尾精子以及在胚胎培养液中分别添加不同浓度胰岛素对猪卵母细胞胞质内单精子显微受精(ICSI)胚胎早期发育的影响.结果:(1)使用冷冻解冻精子与新鲜精子相比对猪卵母细胞ICSI后的卵裂率和囊胚率均无显著影响(P>0.05);2)精子断尾与否对猪卵母细胞ICSI后的分裂率和囊胚率没有显著影响(P>0.05);3)在胚胎培养液中添加5 mg/L胰岛素与对照组相比可显著提高猪ICSI胚胎的囊胚发育率(18.22% vs 3.60%,P<0.05). 相似文献
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本试验探讨了不同辅助激活方法(Calciumionophore A23187激活、Calciumionophore A23187+6-DMAP联合激活和电激活)、不同精子预处理方法(液氮冻融处理和0.1%Triton X-100处理)和在添加半胱氨酸的胚胎培养液中培养不同时间(0 h、4 h、12 h和168 h)对猪卵母细胞内单精子注射(ICSI)胚胎体外发育的影响。结果显示:与无辅助激活相比,A23187+6-DMAP联合激活和电激活均能显著提高ICSI卵母细胞的激活率、卵裂率和囊胚率(P0.05),A23187+6-DMAP联合激活能显著提高ICSI卵母细胞的受精率(P0.05)。液氮冻融精子组ICSI卵母细胞的雄原核形成率显著高于活精子组(P0.05)。在添加半胱氨酸的胚胎培养液中培养4 h的ICSI卵母细胞受精率、雄原核形成率和囊胚率显著高于0 h组(P0.05)。以上结果表明,猪卵母细胞在ICSI后需要辅助激活来启动胚胎顺利发育,A23187+6-DMAP激活效果较好。液氮冻融精子可以促进ICSI后雄原核的形成。半胱氨酸处理4 h对猪ICSI卵母细胞受精和发育均有促进作用。 相似文献
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《中国畜牧杂志》2017,(10)
为应用牛性控精液进行体外受精(IVF)获得大量廉价的性控胚胎,本实验利用微流控精子分离器(MFSS)分离有活力的精子,将体外成熟的卵母细胞放置在MFSS的C室进行体IVF,与常用的微滴-IVF法进行对比,检测2种受精方法的受精率和囊胚发育率。结果表明:MFSS-IVF的单精子入卵率和囊胚率(分别为64.38%、40.12%)均显著高于微滴-IVF法(29.02%、24.55%)(P0.05),受精率和卵裂率差异不显著(P0.05)。由以上得出,MFSS-IVF方法可获得较高的单精子入卵率和囊胚发育率,利用MFSS使用奶牛性控精液进行体外受精生产胚胎是可行的。 相似文献
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为探讨荷斯坦牛和西门塔尔牛冻精的精液品质及体外受精后胚胎发育能力的差异,利用目测法、低渗膨胀法和考马斯亮蓝染色法评估了荷斯坦牛和西门塔尔牛冻精的活力、质膜完整率和顶体完整率,并比较了二者冻精体外受精后胚胎的卵裂率和囊胚率。结果表明,荷斯坦牛和西门塔尔牛冻精的活力(30.4%和27.2%)、质膜完整率(41.96%和36.22%)和顶体完整率(77.02%和73.02%)均无显著差异(P>0.05),但荷斯坦牛冻精体外受精后的卵裂率(57.5%和48.6%)和囊胚率(30.3%和23.2%)显著高于西门塔尔牛冻精(P<0.05)。提示,不同品种公牛精液体外受精后的发育能力有显著差异(P>0.05)。 相似文献
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《畜牧与兽医》2019,(12):19-24
应用体外受精(in vitro fertilization, IVF)等生物技术可以缩短种猪培育时间,地方猪精液的冷冻保存可以解决保存和运输问题。通过对不同个体冷冻前后的精子质量、获能方式、卵子质量及多精受精率对IVF的影响进行了研究。结果显示:当精子活率从83.26%降至74.20%时,IVF的卵裂率、桑椹胚率显著下降(P0.05)。不同的获能方式对IVF胚胎的卵裂率无显著影响(P0.05)。3层(及以上)卵丘细胞的卵子IVF的卵裂率、桑椹率显著高于3层以下组(P0.05)。冷冻精子的IVF中,2-细胞、4-细胞和囊胚的发育能力显著低于新鲜精子(P0.05),受精后6~12 h的多精受精率也显著高于新鲜精子组(P0.05)。猪体外受精胚胎的发育能力受精子和卵母细胞的影响。无论使用新鲜精液还是冷冻精液的IVF胚胎,在桑椹胚期后的发育能力都会受到阻碍,多精受精可能是原因之一,但具体原因还需要更多的研究。 相似文献
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Toyonaga M Morita M Hori T Tsutsui T 《The Journal of veterinary medical science / the Japanese Society of Veterinary Science》2011,73(6):827-829
Glycoproteins (GPs) are known to be involved in the phenomenon of sperm maturation and capacitation. In the present study, we investigated the attachment of GPs on sperm cell membrane during the process of feline sperm maturation from testicular sperm to ejaculated sperm by using 8 FITC-labeled lectins. The results showed that 3 types of GPs were presented on testicular sperm and 7 on caput epididymal sperm. Corpus and cauda epididymal sperm and ejaculated sperm had GPs detected by 8 FITC-labeled lectins used in the present study. This study demonstrates the part of the characteristic of GPs that are present on the feline sperm cell membrane during the process of sperm maturation. 相似文献
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精子载体转基因法是一种简便、高效、低廉的生产转基因动物的方法。而精子供体猪的合适选择是此方法成功的关键步骤之一。试验结果表明,长白猪和杂种猪精子的质量比大约克猪精子质量要好些。 相似文献
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The Beltsville sperm sexing technology is currently the only effective means of altering the sex ratio of offspring in livestock. The method is based on the flow-cytometric separation of X- and Y-chromosome-bearing sperm based on X/Y DNA content difference. It is an effective means of producing progeny of predetermined sex in cattle, swine, sheep, and laboratory animals. The method involves treating sperm with a DNA-binding fluorochrome, Hoechst 33342, and flow-cytometrically sorting them into separate X and Y populations that can subsequently be used for surgical intratubal or intrauterine insemination, deep-uterine insemination, regular artificial insemination in some cases, in vitro fertilization to produce sexed embryos for transfer, and intracytoplasmic sperm injection of ova. Skewed sex ratios of 85 to 95% of one sex or the other have been repeatably achieved in most species. The method has been used worldwide to produce several hundred morphologically normal animal offspring of the predicted sex. It has also been validated in the laboratory using DNA reanalysis of the sorted sperm populations and by fluorescence in situ hybridization and PCR of individual sperm. We developed a new orienting nozzle that we have fitted to both conventional and high-speed cell sorters that have been modified for sperm sorting. Recently we completed the adaptation of the new orienting nozzle to a Cytomation MoFlo high-speed cell sorter modified for sperm. This adaptation of the nozzle has increased the overall production rate of sorted X and Y sperm from about .35 million/h to 5 or 6 million sperm/h (each population). Calves have been born from cows artificially inseminated using conventional technique and sexed sperm. In addition, numerous litters of pigs have been born after transfer of embryos produced from X or Y sorted sperm. 相似文献
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Identification of sperm morphometric subpopulations in cooled‐stored canine sperm and its relation with sperm DNA integrity 
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下载免费PDF全文 The aims of this study were to (i) identify different morphometric subpopulations in cooled‐stored canine sperm and their patterns of distribution during cool‐storage for up to 240 hr and (ii) determine whether or not morphometric sperm subpopulations (sP) are related to sperm DNA integrity. For that purpose, morphometric parameters were analysed by computer‐assisted sperm analysis (CASA) and sperm DNA fragmentation (sDFi) using the sperm Halomax test. Four morphometric sperm heads subpopulations were identified: sP1 (large and rounded), sP2 (large and elongated), sP3 (small and rounded) and sP4 (small and elongated). sP1 was the most predominant subpopulation for up to 72 hr and thereafter sP3 increased progressively. sDFi increased after 48 hr of cool‐storage. Although sP3 showed a positive correlation with sDFi, and both increased over time, it could not be ensured that only the sperm with fragmented DNA are accumulated in sP3. In conclusion, sP3 and DNA fragmentation increased progressively during cool‐storage, becoming possible indicators of sperm damage. However, it cannot be concluded that sP3 only contains sperm with fragmented DNA. 相似文献
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A decrease of sperm freezability occurred at the K. breeding station, and this situation lasted longer than a year. Out of the 2550 ejaculates taken from 42 breeding bulls within 12 months, 685, i.e. 26.7%, were unfit for use immediately after sperm collection, mostly owing to a low activity of spermatozoa and pathological forms of their motility, and another 469 ejaculates, i. e. 18.3%, were unfit for use after sperm freezing; on the whole, 1154 (i. e. 45.2%) ejaculates had to be excluded. It was revealed by the vital-lethal primuline test that the spermatozoa died quickly after collection. The findings obtained during an electron-microscopic examination of the spermatozoa at the beginning of the process included visible changes in the ultrastructure of the flagellum, particularly its middle piece (deformed shape, incomplete set of axial filaments, vacuolization of the flagellum, abnormal arrangement of the mitochondrial spiral), numerous abnormities of the external cytoplasmic membrane and invagination, vacuolization, and abnormal density of nucleoplasm. The primary changes on the flagella and in the nucleus give evidence that the testicular tissues were altered. The etiological factors behind these processes are believed to include a reduction in the resistance of bulls due to long-lasting consumption of feeds contaminated with the fungus Aspergillus fumigatus, insufficient movement and bad zoo-hygienic practices, all this combined with the secondary action of the infectious germs of Mycoplasma bovigenitalium, which were revealed by cultivation tests in 50% of the ejaculates of the bulls; a positive antibody titre was demonstrated in all bulls. 相似文献