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马附睾精子的成熟

Maturation of equine epididymal spermatozoa.

作者信息

Johnson L, Amann R P, Pickett B W

出版信息

Am J Vet Res. 1980 Aug;41(8):1190-6.

PMID:7447113
Abstract

Spermatozoa from four regions of the epididymis and from ejaculated semen were evaluated for their resistance to cold shock, progressive motility, and structural stability. Spermatozoa were incubated at 38 C and their percentage of eosinophilia was compared with that of spermatozoa cooled to 0 C in 2 minutes, 10 C in 12 minutes, or 4 C in 22 minutes. Spermatozoa motility was estimated visually under phase-contrast microscopy and was recorded by cinematography. Structural stability of spermatozoa incubated in 0.05 M sodium borate buffer, 0.035 M sodium dodecyl sulfate (SDS), 0.002 M dithiothreitol (DTT), or SDS+DDT was evaluated by phase-contrast and electron microscopy. The percentage of eosinophilic spermatozoa did not differ among regions of the epididymis and was not increased by cold shock. Cooling ejaculated spermatozoa to 0 C in 2 minutes increased (P < 0.01) the occurrence of eosinophilia (32% vs 73%). Spermatozoa released from the caput or proximal corpus epididymidis into 0.154 M NaCl were not progressively motile; only 4% of the spermatozoa from the distal corpus were motile Cauda epididymal and ejaculated spermatozoa exhibited similar motility (41% vs 47%). Stability of chromatin was greater in spermatozoa from the distal corpus than those from the caput epididymis. Chromatin of spermatozoa from the distal corpus was resistant to 7.5 minutes of SDS+DTT treatment, whereas virtually all spermatozoal nuclei from the caput were decondensed by SDS alone. Tail organelles of spermatozoa acquired stability between the proximal corpus and the cauda epididymidis. All tail organelles of spermatozoa from the proximal corpus were dissolved by 7.5 minutes of SDS treatment, whereas tail organelles of distal corpus epididymal spermatozoa had dissolved after 7.5 minutes of SDS+DTT treatment. Stability of tail organelles in cauda epididymal and ejaculated spermatozoa was similar. Seemingly, equine spermatozoa are infertile until they enter the cauda epididymidis.

摘要

对来自附睾四个区域以及射出精液中的精子进行了抗冷休克能力、前进运动能力和结构稳定性评估。将精子在38℃下孵育,并将其嗜酸性百分比与在2分钟内冷却至0℃、12分钟内冷却至10℃或22分钟内冷却至4℃的精子的嗜酸性百分比进行比较。精子活力通过相差显微镜下目视估计,并通过电影摄影记录。在0.05M硼酸钠缓冲液、0.035M十二烷基硫酸钠(SDS)、0.002M二硫苏糖醇(DTT)或SDS + DTT中孵育的精子的结构稳定性通过相差显微镜和电子显微镜评估。附睾各区域的嗜酸性精子百分比无差异,冷休克也未使其增加。将射出的精子在2分钟内冷却至0℃会增加(P < 0.01)嗜酸性的发生率(32%对73%)。从附睾头或附睾体近端释放到0.154M NaCl中的精子没有前进运动能力;只有4%的附睾体远端精子有运动能力。附睾尾和射出精子的运动能力相似(41%对47%)。附睾体远端精子的染色质稳定性高于附睾头精子。附睾体远端精子的染色质对SDS + DTT处理7.5分钟有抗性,而附睾头的几乎所有精子细胞核仅用SDS就会解聚。精子的尾部细胞器在附睾体近端和附睾尾之间获得稳定性。附睾体近端精子的所有尾部细胞器在SDS处理7.5分钟后溶解,而附睾体远端精子的尾部细胞器在SDS + DTT处理7.5分钟后溶解。附睾尾和射出精子的尾部细胞器稳定性相似。显然,马的精子在进入附睾尾之前是不育的。

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