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低密度脂蛋白、白藜芦醇和槲皮素作为改善公猪精液冷藏的替代添加剂。

Low-density lipoproteins, resveratrol and quercetin as alternative additives to improve boar semen cooling.

作者信息

González Darío, Rojas Mauricio, Rojano Benjamín, Restrepo Giovanni

机构信息

Faculty of Sciences, Universidad Nacional de Colombia, Medellín, Colombia.

Faculty of Medicine, Cell Immunology and Immunogenetics Group, Universidad de Antioquia, Medellín, Colombia.

出版信息

Reprod Domest Anim. 2023 Oct;58(10):1420-1427. doi: 10.1111/rda.14457. Epub 2023 Aug 16.

Abstract

Low-density lipoproteins (LDL), quercetin (Q) and resveratrol (R) have been used for sperm preservation to improve sperm quality in different species. To evaluate the effects of LDL, Q and R during the cooling of boar semen. Fifteen boar semen samples were diluted in a BTS extender supplemented with the treatments: LDL at 6%, Q at 10 μM (Q10), 30 μM (Q30) and 50 μM (Q50), or R at 10 μM (R10), 30 μM (R30) and 50 μM. A control without supplementation was included. The semen was stored by cooling at 16°C for 96 h. Every 24 h, sperm motility and kinetics were evaluated using a computer-assisted sperm analyzer (IVOS). At 24 and 96 h of cooling, functional membrane integrity and mitochondrial membrane potential (ΔΨM) of sperm were evaluated by the hypoosmotic swelling test (HOST) an flow cytometry with JC-1 probe, respectively, LDL improved progressive motility of sperm during cooling. Likewise, LDL increased average path velocity (VAP) and straight-line velocity (VSL) and/or curvilinear velocity (VCL) during the first 48 h of cooling. The use of Q between 10 and 30 μM caused a reduction in total motility, progressive motility and amplitude of the lateral head displacement during the entire cooling period, as well as a decrease in VAP, VSL and VCL at 96 h of cooling. LDL, Q10, Q30 and Q50 modulated mitochondrial activity by reducing high-ΔΨM sperm at 0 and 96 h of cooling. During the cooling of the boar semen prior to artificial insemination, the parameters of sperm quality that could influence fertility decrease; however, the inclusion of antioxidants and additives that protect the plasma membrane, such as LDL, could mitigate the damaging effects on spermatozoa. It is concluded that LDL can improve the motility and kinetics of boar semen during cooling while it could modulating the sperm's mitochondrial activity. On the contrary, Q could alter the motility and kinetics of boar sperm during the cooling period.

摘要

低密度脂蛋白(LDL)、槲皮素(Q)和白藜芦醇(R)已被用于精液保存,以提高不同物种的精子质量。为了评估LDL、Q和R在公猪精液冷却过程中的作用。将15份公猪精液样本在添加了以下处理的BTS稀释液中进行稀释:6%的LDL、10μM(Q10)、30μM(Q30)和50μM(Q50)的Q,或10μM(R10)、30μM(R30)和50μM的R。设置一个不添加任何物质的对照组。精液在16°C下冷却保存96小时。每隔24小时,使用计算机辅助精子分析仪(IVOS)评估精子活力和运动学参数。在冷却24小时和96小时时,分别通过低渗肿胀试验(HOST)和使用JC-1探针的流式细胞术评估精子的功能膜完整性和线粒体膜电位(ΔΨM)。LDL可提高冷却过程中精子的前向运动能力。同样,LDL在冷却的前48小时内提高了平均路径速度(VAP)、直线速度(VSL)和/或曲线速度(VCL)。在整个冷却期间,使用10至30μM的Q会导致总活力、前向运动能力和头部侧向位移幅度降低,以及在冷却96小时时VAP、VSL和VCL降低。LDL、Q10、Q30和Q50通过在冷却0小时和96小时时减少高ΔΨM精子来调节线粒体活性。在人工授精前公猪精液冷却过程中,可能影响生育力的精子质量参数会下降;然而,添加抗氧化剂和保护质膜的添加剂,如LDL,可以减轻对精子的损伤作用。得出的结论是,LDL可以提高公猪精液冷却过程中的活力和运动学参数,同时调节精子的线粒体活性。相反,Q可能会改变冷却期间公猪精子的活力和运动学参数。

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