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本文引用的文献

1
Apoptosis and DNA damage in human spermatozoa.人精子细胞的凋亡和 DNA 损伤。
Asian J Androl. 2011 Jan;13(1):36-42. doi: 10.1038/aja.2010.68. Epub 2010 Aug 30.
2
Implication of apoptosis in sperm cryoinjury.凋亡在精子冷冻损伤中的意义。
Reprod Biomed Online. 2010 Oct;21(4):456-62. doi: 10.1016/j.rbmo.2010.05.011. Epub 2010 Jun 1.
3
Analysis of the relationships between oxidative stress, DNA damage and sperm vitality in a patient population: development of diagnostic criteria.分析患者群体中氧化应激、DNA 损伤与精子活力之间的关系:诊断标准的制定。
Hum Reprod. 2010 Oct;25(10):2415-26. doi: 10.1093/humrep/deq214. Epub 2010 Aug 17.
4
Deficiency in mouse Y chromosome long arm gene complement is associated with sperm DNA damage.鼠 Y 染色体长臂基因缺失与精子 DNA 损伤有关。
Genome Biol. 2010;11(6):R66. doi: 10.1186/gb-2010-11-6-r66. Epub 2010 Jun 23.
5
Clinical significance of sperm DNA damage in assisted reproduction outcome.辅助生殖结局中精子 DNA 损伤的临床意义。
Hum Reprod. 2010 Jul;25(7):1594-608. doi: 10.1093/humrep/deq103. Epub 2010 May 6.
6
Sperm DNA: organization, protection and vulnerability: from basic science to clinical applications--a position report.精子 DNA:组织、保护和脆弱性:从基础科学到临床应用——一份立场报告。
Hum Reprod. 2010 Apr;25(4):824-38. doi: 10.1093/humrep/dep465. Epub 2010 Feb 6.
7
Preservation of sperm within the mouse cauda epididymidis in salt or sugars at room temperature.
Zygote. 2010 Aug;18(3):245-56. doi: 10.1017/S096719940999027X. Epub 2010 Jan 29.
8
Sperm DNA fragmentation: mechanisms of origin, impact on reproductive outcome, and analysis.精子 DNA 碎片化:起源机制、对生殖结局的影响及分析。
Fertil Steril. 2010 Mar 1;93(4):1027-36. doi: 10.1016/j.fertnstert.2009.10.046. Epub 2010 Jan 18.
9
Memoirs of an insult: sperm as a possible source of transgenerational epimutations and genetic instability.侮辱的回忆:精子可能是跨代表观突变和遗传不稳定性的来源。
Mol Hum Reprod. 2010 Jan;16(1):48-56. doi: 10.1093/molehr/gap098. Epub 2009 Nov 6.
10
On the possible origins of DNA damage in human spermatozoa.人类精子中 DNA 损伤的可能起源。
Mol Hum Reprod. 2010 Jan;16(1):3-13. doi: 10.1093/molehr/gap059. Epub 2009 Jul 31.

在无电解质的介质中短期储存人类精子而不冷冻,比冷冻保存更能维持精子染色质的完整性。

Short-term storage of human spermatozoa in electrolyte-free medium without freezing maintains sperm chromatin integrity better than cryopreservation.

机构信息

Institute for Biogenesis Research, John A. Burns School of Medicine, University of Hawaii, Honolulu, Hawaii, USA.

出版信息

Biol Reprod. 2011 Sep;85(3):536-47. doi: 10.1095/biolreprod.111.091322. Epub 2011 May 18.

DOI:10.1095/biolreprod.111.091322
PMID:21593474
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3159537/
Abstract

Previous attempts to maintain human spermatozoa without freezing were based on short-term storage in component-rich medium and led to fast decline in motility and increased incidence of chromosome breaks. Here we report a new method in which sperm are maintained without freezing in an electrolyte-free medium (EFM) composed of glucose and bovine serum albumin. Human sperm were stored in EFM or human tubal fluid medium (HTFM) or were cryopreserved, and their motility, viability, and DNA integrity were examined at different intervals. Cryopreservation led to significant decline in sperm motility and viability and induced DNA fragmentation. Sperm stored in EFM maintained motility and viability for up to 4 and 7 wk, respectively, much longer than sperm stored in HTFM (<2 and <4 wk, respectively). DNA integrity, assessed with comet assay, was also maintained significantly better in EFM than in HTFM. One-week storage in EFM yielded motility and viability similar to that of cryopreserved sperm, but DNA integrity was significantly higher, resembling that of fresh sperm. After several weeks of storage in EFM, sperm were able to activate oocytes, undergo chromatin remodeling, and form normal zygotic chromosomes after intracytoplasmic sperm injection. This study demonstrated that human spermatozoa can be stored in EFM without freezing for several weeks while maintaining motility, viability, and chromatin integrity and that 1-wk storage in EFM offers better protection of sperm DNA integrity than cryopreservation. Sperm storage in EFM may become a viable option for the physicians working in assisted reproduction technology clinics, which would avoid cryodamage.

摘要

先前的不冷冻保存人类精子的尝试是基于在富含成分的培养基中进行短期储存,这导致精子活力迅速下降,染色体断裂的发生率增加。在这里,我们报告了一种新方法,即在由葡萄糖和牛血清白蛋白组成的无电解质培养基(EFM)中不冷冻保存精子。将人类精子储存在 EFM 或人输卵管液培养基(HTFM)中或进行冷冻保存,并在不同时间间隔检查其活力、活力和 DNA 完整性。冷冻保存导致精子活力和活力显著下降,并诱导 DNA 片段化。储存在 EFM 中的精子分别可维持长达 4 周和 7 周的活力和活力,比储存在 HTFM 中的精子分别长(分别<2 周和<4 周)。彗星试验评估的 DNA 完整性在 EFM 中也得到了更好的维持。EFM 中 1 周的储存可产生与冷冻保存精子相似的活力和活力,但 DNA 完整性明显更高,类似于新鲜精子。在 EFM 中储存数周后,精子能够激活卵母细胞,在胞浆内精子注射后经历染色质重塑并形成正常的合子染色体。这项研究表明,人类精子可以在不冷冻的情况下储存在 EFM 中数周,同时保持活力、活力和染色质完整性,并且在 EFM 中储存 1 周比冷冻保存更能保护精子 DNA 的完整性。EFM 中的精子储存可能成为辅助生殖技术诊所中工作的医生的可行选择,这将避免冷冻损伤。