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Optimized Cryopreservation of Mouse Sperm Based on Fertilization Rate

机译:基于受精率的小鼠精子冻存优化

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Although procedures for in vitro fertilization with cryopreserved sperm have been published there is a lack of data indicating that the cryoprotectant and cryopreservation procedures used for those procedures were optimal. To redress this, fertilization rate of eggs exposed to sperm in vitro was used as the outcome in the optimization of raffinose concentration in the cryoprotectant (raffinose in water), volume of cryoprotectant, and freezing conditions for C57BL/6J mouse sperm. Sperm were frozen in a cylindrical Dewar with an internal diameter and height of 14.0 cm and 36.0 cm respectively. The optimal concentration of raffinose was 23-24% (510-540 mOsm/kg). The optimal volume of cryoprotectant used to prepare the sperm suspension from a single mouse was 180-400 μl, and sperm proved most fertile when frozen 13-25 mm above liquid nitrogen. Raffinose in the fertilization medium did not inhibit fertilization. Fertilized eggs transferred to oviducts of recipient mice developed into viable offspring.
机译:尽管已经公开了用冷冻保存的精子进行体外受精的方法,但是缺乏数据表明用于这些程序的冷冻保护剂和冷冻保存方法是最佳的。为了解决这个问题,将体外暴露于精子的卵的受精率用作优化冷冻保护剂中棉子糖浓度(水中的棉子糖),冷冻保护剂体积和C57BL / 6J小鼠精子冷冻条件的结果。将精子冷冻在圆柱形杜瓦瓶中,杜瓦瓶的内径和高度分别为14.0 cm和36.0 cm。棉子糖的最佳浓度为23-24%(510-540 mOsm / kg)。用于从单只小鼠制备精子悬液的冷冻保护剂的最佳体积为180-400μl,并且当在液氮上方冷冻13-25 mm时,精子被证明是最可育的。受精培养基中的棉子糖不抑制受精。转移到受体小鼠输卵管的受精卵发育成后代。

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