首页> 外文期刊>Journal of the World Aquaculture Society >The use of dairy protocols for sperm cryopreservation of blue catfish Ictalurus furcatus
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The use of dairy protocols for sperm cryopreservation of blue catfish Ictalurus furcatus

机译:奶牛操作规程用于冷冻保存蓝I鱼Ictalurus furcatus的精子

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The commercial-scale production of fish by use of artificial (induced) spawning would require reliable, large-volume sources of sperm. Cryopreservation can be used to preserve and store sperm within commercial and research germplasm repositories, but is limited in its application to aquaculture. Straw volume and cooling chamber size restrict the quantity of sperm that can be frozen, and straws must be filled by hand. In contrast, the dairy industry has refined methods for freezing of bull sperm, including automation of straw filling and the use of large cooling chambers. These methods could be used for commercial-scale cryopreservation of fish sperm, although application would require testing. To supply sperm in large volumes, bags originally developed for swine semen could be cooled using dairy protocols and used as a container for fish sperm. The current study documented the use of commercial-scale dairy cryopreservation techniques for the production of hybrids of channel catfish Ictalurus punctatus (female) by blue catfish Ictalurus furcatus. Four cryoprotectants (methanol, dimethyl sulfoxide, dimethyl acetamide, and glycerol) were initially evaluated for use with blue catfish sperm. During May 2000 and March to April 2001, suspensions of blue catfish sperm were cryopreserved with 10% methanol in 0.5-mL French straws and in commercial swine semen bags (Cochette* bags, IMV International, Minneapolis, Minnesota, USA). Cryopreservation took place at a dairy breeding cooperative, using technology employed for bull semen. Sperm motility before freezing was 26 +/- 18% during Year 1 (2000) and 62 +/- 30% during 2001. Sperm were thawed at 40 C and used to fertilize the eggs of channel catfish (yielding hybrids). Motility after thawing for sperm frozen in 0.5-mL straws was 11 +/- 10% during 2000 and 50 +/- 24% during 2001. Motility after thawing was 41 +/- 17% for sperm frozen in swine semen bags in 5-mL aliquots and 43 +/- 10% for sperm frozen in 10-mL aliquots. Neurulation of eggs fertilized with thawed sperm from straws was 83 +/- 13% during 2000 and 54 +/- 27% during 2001. Neurulation was 57 +/- 24% using sperm frozen in swine semen bags in 5-mL aliquots and 55 +/- 10% using sperm frozen in 10-mL aliquots. There was no correlation between sperm motility before freezing (in 0.5-mL straws) and after thawing during 2000 (r = 0.52) or during 2001 (r = 0.49). In addition, there was no correlation between initial motility and neurulation of channel catfish eggs fertilized using thawed sperm during 2000 (r = 0.14) or during 2001 (r = 0.29). Sperm of blue catfish can thus be cryopreserved at a commercial scale using dairy protocols and can be made available for the production of hybrid catfish when viable eggs are available.
机译:通过使用人工(诱导)产卵实现商业规模的鱼类生产将需要可靠的大量精子来源。冷冻保存可用于在商业和研究种质库中保存和储存精子,但在水产养殖中的应用受到限制。秸秆的体积和冷却室的大小限制了可冷冻的精子数量,必须用手填充秸秆。相比之下,乳制品行业已经完善了冷冻公牛精子的方法,包括自动填充稻草和使用大型冷却室。这些方法可用于鱼精的商业规模冷冻保存,尽管应用需要进行测试。为了大量供应精子,最初为猪精液开发的袋子可以使用乳制品协议进行冷却,并用作鱼精的容器。当前的研究记录了使用商业规模的乳品冷冻保存技术来生产蓝I鱼伊卡特鲁斯·富卡图斯(Ictalurus furcatus)的channel鱼伊卡特鲁斯·马齿hybrid(雌性)的杂种。最初评估了四种冷冻保护剂(甲醇,二甲基亚砜,二甲基乙酰胺和甘油)与蓝cat鱼精子一起使用。在2000年5月和2001年3月至2001年4月期间,将蓝色cat鱼精子的悬浮液用10%甲醇冷冻保存在0.5 mL法国稻草中和商业猪精液袋(Cochette *袋,IMV International,明尼苏达州,明尼苏达州,美国)中。冷冻保存是在奶牛育种合作社中进行的,采用的是牛精液技术。第一年(2000年)冷冻前的精子活力为26 +/- 18%,2001年为62 +/- 30%。将精子在40°C融化并用于施肥cat鱼卵(产生杂交种)。冷冻的精子在0.5 mL吸管中解冻后的运动力在2000年为11 +/- 10%,在2001年为50 +/- 24%。在5头猪精液袋中冷冻的精子解冻后的运动力为41 +/- 17%。毫升等分试样,冷冻在10毫升等分试样中的精子为43 +/- 10%。用吸管从融化的精子中受精的卵在2000年的发芽率为83 +/- 13%,在2001年的发芽率为54 +/- 27%。使用在猪精液袋中冷冻的精子以5 mL的等分试样的发芽率是57 +/- 24%。 +/- 10%的精子以10 mL等分冷冻。在2000年(r = 0.52)或2001年(r = 0.49)期间,冷冻前(在0.5 mL吸管中)和解冻后的精子活力之间没有相关性。此外,在2000年(r = 0.14)或2001年(r = 0.29)期间,使用解冻的精子受精的channel鱼卵的初始运动能力与其养育之间没有相关性。因此,可以使用乳品操作规程以商业规模冷冻保存蓝cat鱼的精子,并且在有活卵的情况下,可以使蓝cat鱼的精子用于杂交the鱼的生产。

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