利用抽空绵羊卵巢卵泡的人类精子冷冻新技术。
New Technique for Human Sperm Cryopreservation Using Emptied Sheep's Ovarian Follicles.
机构信息
Radiology Techniques Department, College of Medical Technology, the Islamic University, Najaf, Iraq.
Department of Medical Physiology, Faculty of Medicine, Jabir Ibn Hayyan Medical University, Najaf, Iraq.
出版信息
Arch Razi Inst. 2023 Apr 30;78(2):721-727. doi: 10.22092/ARI.2022.359719.2460. eCollection 2023 Apr.
This study aimed to investigate the efficacy of emptied ovarian follicles of sheep as a container for cryopreservation of human spermatozoa to preserve the presence of low concentrations of spermatozoa at the post-thawing stage. This research was performed on 30 semen samples from oligozoospermic patients and 10 samples from normozoospermic males. They were diagnosed according to the standard criteria of the World Health Organization 2010. Semen samples were classified into four groups of G1-G4 according to sperm concentration: 3-5 million/mL, 6-10 million/mL, 11-15 million/mL, and 16-20 million/mL, respectively. Each sample was divided into two equal parts. One part was cryopreserved without cryoprotectant, while the other was diluted 1:1 with 10% glycerol-based cryosolution. The ovarian follicles of sheep were obtained from a local slaughterhouse and prepared by slicing the ovaries and evacuating the follicular fluid and oocyte. The emptied follicles were injected with the prepared semen samples. After cryopreservation and thawing, the semen mixture aspired outside the follicles, and sperm parameters were measured, namely concentration, progressive motility, total motility, and normal morphology. Sperm concentration and progressive and total sperm motility were significantly (<0.01) decreased in all groups at the post-thawing stage, compared to the pre-freezing stage. The sperm concentration was significantly higher (<0.01) in samples cryopreserved without cryoprotectant, compared to that in those cryopreserved with glycerol. However, progressive and total motility were significantly (<0.01) higher in samples cryopreserved with glycerol, compared to that in the samples cryopreserved without cryoprotectant in all groups. Moreover, no significant difference was found between the pre-freezing and post-thawing stages in terms of normal morphology. Emptied ovarian follicles are an appropriate carrier for cryopreservation of human sperms, especially for patients with oligozoospermia. The best sperm survival rate in this technique was observed when using glycerol-based cryosolution.
本研究旨在探讨绵羊排空卵泡作为人类精子冷冻保存容器的功效,以保持解冻后阶段低浓度精子的存在。该研究在 30 名少精子症患者和 10 名正常精子症男性的 30 份精液样本上进行。他们的诊断依据是 2010 年世界卫生组织的标准标准。精液样本根据精子浓度分为 G1-G4 四组:分别为 3-5 百万/ml、6-10 百万/ml、11-15 百万/ml 和 16-20 百万/ml。每个样本均分为两等份。一部分不经冷冻保护剂冷冻保存,另一部分用 10%甘油基冷冻液稀释 1:1。从当地屠宰场获得绵羊的卵泡,通过切片卵巢和排空卵泡液和卵母细胞来准备。排空的卵泡用准备好的精液样本注射。冷冻保存和解冻后,将吸出卵泡外的精液混合物,并测量精子参数,即浓度、前向运动、总运动和正常形态。与冷冻前阶段相比,所有组的解冻后阶段精子浓度、前向运动和总运动均显著(<0.01)降低。与甘油冷冻相比,无冷冻保护剂冷冻的样本中精子浓度显著(<0.01)更高。然而,在所有组中,与无冷冻保护剂冷冻的样本相比,甘油冷冻的样本中前向运动和总运动显著(<0.01)更高。此外,在正常形态方面,冷冻前和冷冻后阶段之间没有发现显著差异。排空的卵泡是人类精子冷冻保存的合适载体,特别是对少精子症患者。在该技术中,使用甘油基冷冻液观察到最佳的精子存活率。
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