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一种用于斑马鱼精子冷冻保存和体外受精的高通量方法。

A high-throughput method for zebrafish sperm cryopreservation and in vitro fertilization.

作者信息

Draper Bruce W, Moens Cecilia B

机构信息

Molecular and Cellular Biology, University of California, Davis, CA, USA.

出版信息

J Vis Exp. 2009 Jul 6(29):1395. doi: 10.3791/1395.

Abstract

This is a method for zebrafish sperm cryopreservation that is an adaptation of the Harvey method (Harvey et al., 1982). We have introduced two changes to the original protocol that both streamline the procedure and increase sample uniformity. First, we normalize all sperm volumes using freezing media that does not contain the cryoprotectant. Second, cryopreserved sperm are stored in cryovials instead of capillary tubes. The rates of sperm freezing and thawing (delta degrees C/time) are probably the two most critical variables to control in this procedure. For this reason, do not substitute different tubes for those specified. Working in teams of 2 it is possible to freeze the sperm of 100 males per team in approximately 2 hrs. Sperm cryopreserved using this protocol has an average of 25% fertility (measured as the number of viable embryos generated in an in vitro fertilization divided by the total number of eggs fertilized) and this percent fertility is stable over many years.

摘要

这是一种斑马鱼精子冷冻保存方法,是对哈维方法(Harvey等人,1982年)的改进。我们对原始方案进行了两项改进,既简化了程序又提高了样本均匀性。首先,我们使用不含冷冻保护剂的冷冻培养基对所有精子体积进行标准化。其次,冷冻保存的精子储存在冻存管中而不是毛细管中。精子冷冻和解冻的速率(℃/时间变化)可能是该程序中要控制的两个最关键变量。因此,请勿用其他不同的管子替代指定的管子。两人一组工作,每组大约可以在2小时内冷冻100只雄性的精子。使用该方案冷冻保存的精子平均受精率为25%(以体外受精产生的活胚胎数量除以受精的卵总数来衡量),并且这个受精率在许多年里都很稳定。

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