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使用吖啶橙试验和TUNEL分析来评估冻干牛精子DNA的完整性。

The use of the acridine orange test and the TUNEL assay to assess the integrity of freeze-dried bovine spermatozoa DNA.

作者信息

Martins C F, Dode M N, Báo S N, Rumpf R

机构信息

Embrapa Recursos Genéticos e Biotecnologia, Brasília, DF, Brasil.

出版信息

Genet Mol Res. 2007 Mar 15;6(1):94-104.

Abstract

The ability to detect nuclear damage is an important tool for the development of sperm preservation methods. We used the acridine orange test (AOT) and the terminal deoxynucleotidyl transferase-mediated dUDP nick-end labeling (TUNEL) assay to assess the DNA status of sperm cells preserved with different lyophilization media. The AOT did not detect any differences between different lyophilization media. However, differences in DNA integrity were observed among treatments with the TUNEL assay, suggesting that TUNEL is a more sensitive method to evaluate sperm DNA. The use of TCM 199 and 10% FCS as a lyophilization medium resulted in 14% of the cells with DNA fragmentation in TUNEL test. The AOT indicated only 4% of the cells with chromatin damage, with this same treatment, with no significant differences when compared to the other treatments. The degree of DNA fragmentation was negatively related to fertilizing potential, as sperm DNA damage was inversely correlated with pro-nucleus formation. The TUNEL assay was found to be an efficient method to detect DNA damage in sperm, and it could be used as a tool to predict male fertility.

摘要

检测核损伤的能力是精子保存方法开发的一项重要工具。我们使用吖啶橙试验(AOT)和末端脱氧核苷酸转移酶介导的dUTP缺口末端标记(TUNEL)分析法来评估用不同冻干介质保存的精子细胞的DNA状态。AOT未检测到不同冻干介质之间存在任何差异。然而,通过TUNEL分析法在各处理组中观察到了DNA完整性的差异,这表明TUNEL是评估精子DNA的更灵敏方法。使用TCM 199和10%胎牛血清作为冻干介质,在TUNEL试验中导致14%的细胞出现DNA片段化。采用相同处理时,AOT显示只有4%的细胞存在染色质损伤,与其他处理相比无显著差异。DNA片段化程度与受精潜能呈负相关,因为精子DNA损伤与原核形成呈负相关。发现TUNEL分析法是检测精子DNA损伤的有效方法,可作为预测男性生育能力的工具。

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