Catalase and Uric Acid Prevent Morphological Damage to the Sperm Flagella of Colossoma macropomum During 96 Hours at Low Storage Temperatures.

IF 16.4 1区化学 Q1 CHEMISTRY, MULTIDISCIPLINARY Accounts of Chemical Research Pub Date : 2024-10-01 Epub Date: 2024-03-22 DOI:10.1089/bio.2022.0213

Yugo M Pastrana, Jaydione L Marcon, Amanda P de Amaral, Francisco Bruno P Santos, Emerson S Lima, Leonard D R Acho, Rodrigo Otávio S de Souza, Carolina C Grando, Danilo P Streit Junior, Leandro Godoy

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Abstract

Oxidative stress is one of the main causes of loss of sperm function during chilled storage. The aim of the current study was to evaluate the effects of a fructose-based extender, which was supplemented with catalase or uric acid, on the motility, viability, morphological integrity, and lipid peroxidation (LPO) of Colossoma macropomum spermatozoa. Sperm was diluted in extenders containing catalase (0; 0.1; 0.8; and 1.5 kU/L) or uric acid (0; 0.25; 0.5; and 1.0 mmol/L) and then stored at 4.3 ± 0.6°C for 96 hours. The chilling storage time had more significant and pronounced effects on practically all the measured sperm quality parameters than the different concentrations of both antioxidants added to the extenders. This was true for sperm motility, motility duration, sperm viability, and the percentage of normal spermatozoa. In fact, for all these parameters, values were higher in the extenders supplemented with catalase or uric acid, than those not supplemented with these antioxidants, especially after 96 hours. The LPO process showed an antioxidant-dependent response. In catalase-supplemented extenders thiobarbituric acid reactive substance (TBARS) levels increased gradually and significantly with time, but remained stable during the 96 hours of chilled storage in all samples in which uric acid was added. Despite this, TBARS levels were lower in the extenders supplemented with both catalase and uric acid than in those not having these antioxidants. Inverse correlations were found between sperm motility and the damage in sperm flagella. Our findings suggest that the supplementation of an extender with catalase or uric acid is beneficial and protects fish sperm membranes from damage caused by oxidative stress during low-temperature storage. The extenders containing 0.1 kU/L of catalase and 0.25 mmol/L of uric acid provided effective antioxidant protection for the spermatozoa of this important Amazonian fish.

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过氧化氢酶和尿酸可防止大疣梭子蟹精子鞭毛在低温储存 96 小时期间的形态损伤

氧化应激是冷藏期间精子功能丧失的主要原因之一。本研究的目的是评估以果糖为基础、添加过氧化氢酶或尿酸的扩展剂对巨眼瘤精子的活力、存活率、形态完整性和脂质过氧化（LPO）的影响。将精子稀释在含过氧化氢酶（0；0.1；0.8；和 1.5 kU/L）或尿酸（0；0.25；0.5；和 1.0 mmol/L）的扩展剂中，然后在 4.3 ± 0.6°C 下储存 96 小时。与添加到扩展剂中的两种抗氧化剂的不同浓度相比，冷藏时间对几乎所有测量的精子质量参数都有更显著、更明显的影响。在精子活力、活力持续时间、精子存活率和正常精子百分比方面都是如此。事实上，在所有这些参数中，添加过氧化氢酶或尿酸的扩展剂的数值都高于未添加这些抗氧化剂的扩展剂，尤其是在 96 小时之后。LPO 过程显示出抗氧化剂依赖性反应。在添加了过氧化氢酶的延展剂中，硫代巴比妥酸活性物质（TBARS）的含量随着时间的推移逐渐显著增加，但在添加了尿酸的所有样品中，TBARS 的含量在冷藏的 96 小时内保持稳定。尽管如此，添加了过氧化氢酶和尿酸的延长剂中的 TBARS 水平要低于未添加这些抗氧化剂的延长剂。精子活力与精子鞭毛的损伤之间存在反相关关系。我们的研究结果表明，在扩展剂中添加过氧化氢酶或尿酸是有益的，可以保护鱼类精子膜在低温储存过程中免受氧化应激的损害。含有 0.1 kU/L 过氧化氢酶和 0.25 mmol/L 尿酸的扩展剂能为这种重要的亚马逊鱼类精子提供有效的抗氧化保护。

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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来源期刊

Accounts of Chemical Research 化学-化学综合

CiteScore

31.40

自引率

1.10%

发文量

312

审稿时长

2 months

期刊介绍： Accounts of Chemical Research presents short, concise and critical articles offering easy-to-read overviews of basic research and applications in all areas of chemistry and biochemistry. These short reviews focus on research from the author’s own laboratory and are designed to teach the reader about a research project. In addition, Accounts of Chemical Research publishes commentaries that give an informed opinion on a current research problem. Special Issues online are devoted to a single topic of unusual activity and significance. Accounts of Chemical Research replaces the traditional article abstract with an article "Conspectus." These entries synopsize the research affording the reader a closer look at the content and significance of an article. Through this provision of a more detailed description of the article contents, the Conspectus enhances the article's discoverability by search engines and the exposure for the research.

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