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马精子蛋白质组学分析表明冷冻保存后精子代谢发生变化,氧化还原调节受损。

Proteomic profiling of stallion spermatozoa suggests changes in sperm metabolism and compromised redox regulation after cryopreservation.

机构信息

Laboratory of Equine Reproduction and Equine Spermatology, Veterinary Teaching Hospital, University of Extremadura, Cáceres, Spain.

Facility of Innovation and Analysis in Animal Source Foodstuffs, University of Extremadura, Cáceres, Spain.

出版信息

J Proteomics. 2020 Jun 15;221:103765. doi: 10.1016/j.jprot.2020.103765. Epub 2020 Apr 2.

DOI:10.1016/j.jprot.2020.103765
PMID:32247875
Abstract

Proteomic technologies allow the detection of thousands of proteins at the same time, being a powerful technique to reveal molecular regulatory mechanisms in spermatozoa and also sperm damage linked to low fertility or specific biotechnologies. Modifications induced by the cryopreservation in the stallion sperm proteome were studied using UHPLC/MS/MS. Ejaculates from fertile stallions were collected and split in two subsamples, one was investigated as fresh (control) samples, and the other aliquot frozen and thawed using standard procedures and investigated as frozen thawed subsamples. UHPLC/MS/MS was used to study the sperm proteome under these two distinct conditions and bioinformatic enrichment analysis conducted. Gene Ontology (GO) and pathway enrichment analysis were performed revealing dramatic changes as consequence of cryopreservation. The terms oxidative phosphorylation, mitochondrial ATP synthesis coupled electron transport and electron transport chain were significantly enriched in fresh samples (P = 5.50 × 10, 4.26 × 10 and 7.26 × 10 respectively), while were not significantly enriched in frozen thawed samples (P = 1). The GO terms oxidation reduction process and oxidoreductase activity were enriched in fresh samples and the enrichment was reduced in frozen thawed samples (1.40 × 10, 1.69 × 10 versus 1.13 × 10 and 2-86 × 10 respectively). Reactome pathways (using human orthologs) significantly enriched in fresh sperm were TCA cycle and respiratory electron transport (P = 1.867 × 10), Respiratory electron transport ATP synthesis by chemiosmosis coupling (P = 2.124 × 10), Citric acid cycle (TCA cycle)(P = 8.395 × 10) Pyruvate metabolism and TCA cycle (P = 3.380 × 10), Respiratory electron transport (P = 2.764 × 10) and Beta oxidation of laurolyl-CoA to decanoyl CoA-CoA (P = 1.854 × 10) none of these pathways were enriched in thawed samples (P = 1). We have provided the first detailed study on how the cryopreservation process impacts the stallion sperm proteome. Our findings identify the metabolic proteome and redoxome as the two key groups of proteins affected by the procedure. SIGNIFICANCE: In the present manuscript we investigated how the cryopreservation of stallion spermatozoa impacts the proteome of these cells. This procedure is routinely used in horse breeding and has a major impact in the industry, facilitating the trade of genetic material. This is still a suboptimal biotechnology, with numerous unresolved problems. The limited knowledge of the molecular insults occurring during cryopreservation is behind these problems. The application and development of proteomics to the spermatozoa, allow to obtain valuable information of the specific mechanisms affected by the procedure. In this paper, we report that cryopreservation impacts numerous proteins involved in metabolism regulation (mainly mitochondrial proteins involved in the TCA cycle, and oxidative phosphorylation) and also affects proteins with oxidoreductase activity. Moreover, specific proteins involved in the sperm-oocyte interaction are also affected by the procedure. The information gathered in this study, opens interesting questions and offer new lines of research for the improvement of the technology focusing the targets here identified, and the specific steps in the procedure (cooling, toxicity of antioxidants etc.) to be modified to reduce the damage.

摘要

蛋白质组学技术允许同时检测数千种蛋白质,是揭示精子分子调节机制以及与低生育力或特定生物技术相关的精子损伤的强大技术。使用 UHPLC/MS/MS 研究了冷冻对种马精子蛋白质组的影响。从有生育能力的种马中收集精液并分为两个亚样本,一个样本作为新鲜(对照)样本进行研究,另一个样本等分冷冻和解冻,并按照标准程序进行研究作为冷冻解冻样本。使用 UHPLC/MS/MS 研究了这两种不同条件下的精子蛋白质组,并进行了生物信息学富集分析。进行了基因本体论(GO)和途径富集分析,结果显示冷冻保存导致了显著的变化。术语氧化磷酸化、线粒体 ATP 合成偶联电子传递和电子传递链在新鲜样本中显著富集(P=5.50×10、4.26×10 和 7.26×10,分别),而在冷冻解冻样本中没有显著富集(P=1)。GO 术语氧化还原过程和氧化还原酶活性在新鲜样本中富集,而在冷冻解冻样本中富集减少(1.40×10、1.69×10 与 1.13×10 和 2-86×10,分别)。新鲜精子中显著富集的反应途径(使用人类同源物)为 TCA 循环和呼吸电子传递(P=1.867×10)、通过化学渗透偶联的呼吸电子传递 ATP 合成(P=2.124×10)、柠檬酸循环(TCA 循环)(P=8.395×10)、丙酮酸代谢和 TCA 循环(P=3.380×10)、呼吸电子传递(P=2.764×10)和月桂酰辅酶 A 的β氧化为癸酰辅酶 A-CoA(P=1.854×10),这些途径在解冻样本中均未富集(P=1)。我们首次详细研究了冷冻过程如何影响种马精子的蛋白质组。我们的发现确定了代谢蛋白质组和氧化还原蛋白质组是受该过程影响的两个关键蛋白质组。意义:在本手稿中,我们研究了种马精子的冷冻保存如何影响这些细胞的蛋白质组。该程序在马的繁殖中常规使用,并对该行业产生了重大影响,促进了遗传物质的贸易。这仍然是一种不太理想的生物技术,存在许多未解决的问题。冷冻保存过程中发生的分子损伤的有限知识是这些问题的背后原因。蛋白质组学在精子中的应用和发展,可以获得该过程影响的特定机制的有价值信息。在本文中,我们报告说,冷冻保存会影响许多参与代谢调节的蛋白质(主要是参与 TCA 循环和氧化磷酸化的线粒体蛋白质),也会影响具有氧化还原酶活性的蛋白质。此外,该过程还会影响参与精子-卵子相互作用的特定蛋白质。本研究收集的信息提出了有趣的问题,并为改进该技术提供了新的研究方向,重点是确定这里的目标,以及程序中的具体步骤(冷却、抗氧化剂的毒性等)进行修改以减少损伤。

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