Cryopreservation of Human Spermatozoa: A New Frontier in Reproductive Medicine

N. Saymé
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引用次数: 2

Abstract

Cryopreservation is a worldwide technique that makes it possible to preserve different living cells and tissues, including male and female gametes and embryos, in a structurally intact state using low temperature over time. Since the starting point of the cryopreservation era in 1776, until today, this was one of the most important steps in assisted reproductive techniques. Conventional slow freezing of spermatozoa is commonly used for cryopreservation of both ejaculated and surgically retrieved spermatozoa. The technique of the slow freezing is principally based on dehydration of cells which is performed through slow cooling combined with low concentrations of a cryoprotectant agent for achieving a balance. Besides of slow freezing, for more than a decade, many reports suggest the sperm vitrification technique as an alternative to slow freezing. Contrary to the slow freezing method, with vitrification, the effects of the cryoprotectants in spermatozoa are eliminated since this method is cryoprotectant-free. All of these interesting and promising protocols of vitrification, however, have not been implemented in the lab routine yet, and slow freezing remains the standard cryopreservation method in most laboratories worldwide.
人类精子的低温保存:生殖医学的新前沿
低温保存是一项世界性的技术,它可以在低温下保存不同的活细胞和组织,包括雄性和雌性配子和胚胎,使其在结构上保持完整。自1776年低温保存时代开始,直到今天,这是辅助生殖技术中最重要的一步。传统的精子慢速冷冻通常用于冷冻保存射精和手术取出的精子。缓慢冷冻技术主要是基于细胞的脱水,通过缓慢冷却结合低浓度的冷冻保护剂来达到平衡。除了慢速冷冻之外,十多年来,许多报告都建议将精子玻璃化技术作为慢速冷冻的替代方法。与玻璃化的慢速冷冻方法相反,由于这种方法不含冷冻保护剂,因此消除了精子中冷冻保护剂的影响。然而,所有这些有趣和有前途的玻璃化保存方案尚未在实验室常规中实施,缓慢冷冻仍然是世界上大多数实验室的标准冷冻保存方法。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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