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两种有袋动物(帚尾袋貂和尤金袋鼠)的无颗粒冷冻精子

Pellet-freezing spermatozoa of two marsupials: the tammar wallaby, Macropus eugenii, and the brushtail possum, Trichosurus vulpecula.

作者信息

Molinia F C, Rodger J C

机构信息

Department of Biological Sciences, University of Newcastle, NSW, Australia.

出版信息

Reprod Fertil Dev. 1996;8(4):681-4. doi: 10.1071/rd9960681.

Abstract

A protocol was developed for pellet-freezing spermatozoa of the tammar wallaby and the brushtail possum. Seren was collected by electro-ejaculation and wallaby spermatozoa were washed by 'swim-up' into phosphate-buffered saline (PBS), whereas possum spermatozoa were not washed. Wallaby spermatozoa were screened for toxicity in diluents containing a range of cryoprotectants (0-10%): dimethyl sulfoxide (DMSO), ethylene glycol and propanediol. Possum spermatozoa were tolerant of diluents containing 17.5% glycerol. Wallaby and possum spermatozoa were diluted 1:1 with the most promising cryoprotective diluents (final concentrations in PBS: possum, 17.5% glycerol; wallaby, 7.5% glycerol + 10% DMSO) and, after 5 min equilibration at room temperature, were pellet-frozen. Pellets were thawed (35 degrees C) and wallaby spermatozoa were washed by centrifugation (200 g for 5 min) and resuspended in PBS to minimize cryoprotectant toxicity. A high proportion of possum spermatozoa was recovered after freezing (67.5%), having good progressive motility (3.6 on a 0-5 scale). The progressive motility of frozen-thawed wallaby spermatozoa was also high (3.0), but only 10% of motile spermatozoa were recovered. The pellet-freezing method in conjunction with the post-thaw washing procedure (wallaby) may produce a viable population of cryopreserved marsupial spermatozoa suitable for use in assisted-breeding techniques such as in vitro fertilization and artificial insemination.

摘要

已制定了一项针对袋狸和帚尾袋貂无颗粒冷冻精子的方案。通过电射精收集精液,袋狸精子通过“上浮”法洗涤后置于磷酸盐缓冲盐水(PBS)中,而袋貂精子未进行洗涤。对袋狸精子在含有一系列冷冻保护剂(0 - 10%)的稀释液中进行毒性筛选,这些冷冻保护剂包括二甲基亚砜(DMSO)、乙二醇和丙二醇。袋貂精子对含有17.5%甘油的稀释液具有耐受性。将袋狸和袋貂精子与最有前景的冷冻保护稀释液按1:1稀释(PBS中的最终浓度:袋貂,17.5%甘油;袋狸,7.5%甘油 + 10% DMSO),在室温下平衡5分钟后进行无颗粒冷冻。将冻粒解冻(35摄氏度),袋狸精子通过离心(200 g,5分钟)洗涤,并重新悬浮于PBS中以尽量减少冷冻保护剂的毒性。冷冻后,袋貂精子的回收率较高(67.5%),具有良好的前进运动能力(0 - 5级评分中为3.6)。冻融后袋狸精子的前进运动能力也较高(3.0),但仅回收了10%的活动精子。结合解冻后洗涤程序(袋狸)的无颗粒冷冻方法可能会产生一批适用于体外受精和人工授精等辅助繁殖技术的可存活的冷冻保存有袋动物精子。

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