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用台盼兰—姬姆萨染色检测家畜精子顶导反应的研究 总被引:1,自引:0,他引:1
本文探讨了用台盼兰—姬姆萨染色检测家畜精子顶体反应的可行性。用肝素或钙离子载体诱发精子顶体反应。根据染色结果将精子分为四类:a)核后帽部不着色或淡青色,顶体不着色或部分紫红色(有顶体反应活精子);b)核后帽部暗青色.顶体部不着色或部分暗红色(有顶体反应死精子);c)核后帽部不着色或淡青色,顶体部紫红色(无顶体反应活精子);d)核后帽部暗青色,顶体部暗紫红色(无顶体反应死精子)。有顶体反应活精子百分率与仓鼠卵穿透率呈强正相关。从而证明台盼兰—姬姆萨染色是检测家畜精子顶体反应的有效手段,并能预测获能处理后精子的受精能力。 相似文献
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应用电子显微镜和X射线微分析技术,对貉受精过程和受精卵膜元素研究的结果表明,貉卵子的卵丘细胞具有吞噬和过滤功能;卵丘细胞间的精子顶体尚未发生囊泡化,而附着于透明带的精子发生了顶体反应,并以80°角穿入透明带,在其穿入的前方打开一个通道,最后穿过。穿过透明带的精子以赤道段或顶体后区同卵膜融合,并激发皮质颗粒释放,接着穿入卵内,最终发育成雌、雄原核。原核期受精卵质膜上具有高含量的钙,并呈集团分布,它在皮质颗粒胞吐释放中起着重要作用。 相似文献
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史氏鲟精子超微结构 总被引:4,自引:1,他引:3
利用扫描和透射电镜观察了史氏鲟精子形态和超微结构。精子具有顶体、头部、中段和单鞭毛等部分。顶体长0.99±0.06μm,宽0.87±0.09μm。细胞核从后往前逐渐变细,前端宽度为0.88±0.04μm,后端宽度为1.26±0.06μm,细胞核长7.29±0.32μm。核内含有3条核管(E),核管上行至顶体下行至植入窝而止。中段紧接头后部,长为0.51±0.12μm,宽0.91±0.05μm。中段含有线粒体、中心粒复合体和鞭毛的起始部分。线粒体分2~3层排列,线粒体中可见髓样嵴结构。在细胞核与中段接合部细胞核向内凹陷形成植入窝,纤维体位于植入窝内,其后是中心粒复合体。中段后缘延长为袖套,袖套腔中含有线粒体、脂质空泡。鞭毛从袖套中伸出,由轴丝组成,为典型的"9+2"微管结构。 相似文献
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为探究不同冷冻解冻方法对猪精子损伤的影响,采用2种常用的冷冻解冻方法处理猪精子,分别对其顶体膜蛋白进行分离,进行SDS-PAGE电泳和总灰度值的检测和分析。结果表明,采用一次稀释法进行猪精液的冷冻保存较二次稀释法解冻后精子活率高,精子顶体膜蛋白组分中除125 ku和90 ku处蛋白表达水平低于二次稀释法外,120 ku、48 ku、36 ku均高于二次稀释法。可见,猪精子在受到更深层次(二次稀释法对精子冷冻解冻损伤大)的冷冻损伤时,伴随着顶体膜蛋白125 ku和90 ku表达水平的升高以及120、48及36 ku表达水平的降低。 相似文献
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对棕熊精子体外获能前后和异种穿卵的超微结构观察表明,棕熊精子全长77μm,由头、颈和尾3部分组成.头部长7.3μm,宽2.5μm,主要由核、顶体及顶体后区组成;颈部由中心粒和9条纵行分节的节往组成;尾部全长68.2μm,其中中段长13.2μm,线粒体为65~68旋,主段中央为“9 2”的微管结构,其外方被9条致密纤维和纤维鞘包裹.精子获能前群集成簇,运动缓慢;获能后精子呈超激活运动.获能的精子质膜膨胀,顶体外膜囊泡化,引起顶体反应,质膜并未参加囊泡化.顶体反应完成后,仅有顶体内膜包在精子核膜的外面.棕熊精子与仓鼠的卵相互作用,多以赤道段和顶体后区附着于卵膜. 相似文献
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Eduardo R. S. Roldan 《Reproduction in domestic animals》2019,54(Z4):14-21
Sperm competition is a powerful selective force that has influenced many reproductive traits in males and females although additional evolutionary explanations may help to understand the diversity of mammalian reproduction. Sperm morphology varies considerably in mammals with extreme examples in several rodent lineages in which a wide range of sizes and complex head morphologies have been identified. Mammalian spermatozoa also differ in function, with swimming velocity and trajectory showing much divergence. Underlying processes mediating function have received little attention so far, but differences in timing and proportion of sperm undergoing capacitation or acrosomal exocytosis may be related to variation in signalling processes. Furthermore, energy required for sperm functions (such as motion, signalling and overall maintenance of cell integrity) can be produced and consumed, following different patterns among species and this could be the result of several selective forces. A more thorough understanding of the diversity in structure and function of sperm cells, and underlying selective forces, may help us develop better methods to assess them taking into account particulars and generalities of sperm form and performance. Such tests could then become more reliable in estimations of the impact of cryopreservation or effect of changes in the environment and their relevance for fertility. 相似文献
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Weiwei Zhang Han Zhang Shumei Mu Juhui Yan Meiqin Guo Wenyan Li Xianjiang Kang 《Aquaculture Research》2020,51(3):890-905
SLO1 potassium channels are pivotal to many aspects of spermatogenic cell. Experiments were conducted to assess physiology and function of SLO1 potassium channels in different developmental stages of spermatogenic cell in Eriocheir sinensis. First, the expression of SLO1 protein was examined via Western blot, RT‐PCR, immunohistochemistry and immunofluorescence assays. The results showed that the expression of the SLO1 protein was not uniform in the spermatogenic cells of E. sinensis. Second, whole‐cell patch clamp technique was used to record the potassium current of spermatogenic cells and to analyse the electrophysiological characteristics of the potassium channels with the aid of inhibitors. It is proved that the potassium current in E. sinensis germ cells is associated with intracellular Ca2+, and the calcium‐activated potassium channel mediated by SLO1 protein is mainly large‐conductance Ca2+‐activated K+ channels (BKCa). Based on these researches, the cDNA of SLO1 from testis was cloned and sequenced. The SLO1 protein contained domains bound to calcium ions, and the spatial structure formed by its tetramers constituted potassium channels. Phylogenetic analysis revealed that SLO1 was much closer to Scylla paramamosain than other examined species. Finally, iberiotoxin (IbTX) and CdCl2 were used to inhibit the acrosome reaction (AR) induced by A23187 and to explore the role of SLO1 potassium channels in the AR of E. sinensis. The experimental results showed that SLO1 potassium channels were expressed in E. sinensis spermatogenic cells and played an important role in the AR of crab sperm (SP). 相似文献
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本试验皆在研究添加不同浓度大豆卵磷脂(SL)冷冻保存东佛里生奶绵羊精液的效果。我们在Tris基础稀释液中,添加18%蛋黄为对照组,添加0.5%、1%、1.5%、2%、2.5%SL设为试验组,检测冷冻精液解冻后的精子活率和顶体完整率。结果显示,添加0.5%、2.5% SL冷冻稀释液稀释的精液,解冻后精子活率和顶体完整率与其他组之间存在显著差异(P<0.05);添加18%蛋黄和1%~2% SL冷冻稀释液稀释的精液,冷冻解冻后精子活率和顶体完整率之间无显著差异(P>0.05);添加18%蛋黄和1.0%~1.5% SL冷冻稀释液稀释后的精液,进行人工授精后母羊的妊娠率与对照组无显著差异(P>0.05)。因此,大豆卵磷脂可以作为冷冻保护剂用于东佛里生奶绵羊精液的冷冻保存,其最佳添加浓度为1~2%(g/L)。 相似文献
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