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不同活跃精子运动水平公猪睾丸组织的蛋白质谱分析。

Protein profiling of testicular tissue from boars with different levels of hyperactive sperm motility.

机构信息

Norsvin, Storhamargata 44, 2317, Hamar, Norway.

Department of Animal and Aquacultural Sciences, Faculty of Biosciences, Centre for Integrative Genetics (CIGENE), Norwegian University of Life Sciences, 1432, Ås, Norway.

出版信息

Acta Vet Scand. 2022 Sep 5;64(1):21. doi: 10.1186/s13028-022-00642-1.

Abstract

Hyperactive sperm motility is important for successful fertilization. In the present study, a proteome profiling approach was performed to identify the differences between Landrace boars with different levels of hyperactive sperm motility in liquid extended semen. Two contrasts were studied: (i) high versus low levels of sperm hyperactivity at semen collection day and (ii) high versus low change in levels of sperm hyperactivity after 96 h semen storage. Testicular samples were analyzed on a Q Exactive mass spectrometer and more than 6000 proteins were identified in the 13 samples. The most significant differentially expressed proteins were mediator complex subunit 28 (MED28), cell division cycle 37 like 1 (CDC37L1), ubiquitin specific peptidase 10 (USP10), zinc finger FYVE-type containing 26 (ZFYVE26), protein kinase C delta (PRKCD), actinin alpha 4 (ACTN4), N(alpha)-acetyltransferase 30 (NAA30), C1q domain-containing (LOC110258309) and uncharacterized LOC100512926. Of the differentially expressed proteins, 11 have previously been identified as differentially expressed at the corresponding mRNA transcript level using the same samples and contrasts. These include sphingosine kinase 1 isoform 2 (SPHK1), serine and arginine rich splicing factor 1 (SRSF1), and tubulin gamma-1 (TUBG1) which are involved in the acrosome reaction and sperm motility. A mass spectrometry approach was applied to investigate the protein profiles of boars with different levels of hyperactive sperm motility. This study identified several proteins previously shown to be involved in sperm motility and quality, but also proteins with no known function for sperm motility. Candidates that are differentially expressed on both mRNA and protein levels are especially relevant as biological markers of semen quality.

摘要

精子的超活跃运动能力对于成功受精至关重要。在本研究中,采用蛋白质组学分析方法来鉴定在液态延长精液中精子超活跃运动能力不同的长白猪之间的差异。研究了两个对比:(i)在精液采集日精子超活跃度的高低,以及(ii)在 96 小时精液储存后精子超活跃度水平的高低变化。对睾丸样本进行了 Q Exactive 质谱仪分析,在 13 个样本中鉴定出了超过 6000 种蛋白质。差异最显著的表达蛋白有:中介复合体亚基 28(MED28)、细胞分裂周期蛋白 37 样 1(CDC37L1)、泛素特异性肽酶 10(USP10)、锌指 FYVE 型结构域包含蛋白 26(ZFYVE26)、蛋白激酶 C 德尔塔(PRKCD)、肌动蛋白α 4(ACTN4)、N(α)-乙酰转移酶 30(NAA30)、C1q 结构域包含蛋白(LOC110258309)和未知的 LOC100512926。在差异表达蛋白中,有 11 种蛋白之前在使用相同样本和对比的情况下,在相应的 mRNA 转录水平上被鉴定为差异表达。其中包括鞘氨醇激酶 1 同工型 2(SPHK1)、丝氨酸/精氨酸丰富剪接因子 1(SRSF1)和微管蛋白γ-1(TUBG1),它们参与顶体反应和精子运动。本研究采用质谱分析法来研究具有不同超活跃精子运动能力的公猪的蛋白质谱。该研究鉴定了一些以前被认为与精子运动和质量有关的蛋白质,但也鉴定了一些对精子运动没有已知功能的蛋白质。在 mRNA 和蛋白质水平上都有差异表达的候选蛋白作为精液质量的生物标志物尤其相关。

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本文引用的文献

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