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缺乏连续的精子特异性糖酵解酶的小鼠的精子功能、蛋白质磷酸化和代谢存在差异。

Sperm function, protein phosphorylation, and metabolism differ in mice lacking successive sperm-specific glycolytic enzymes.

机构信息

Department of Cell Biology and Physiology, University of North Carolina School of Medicine, Chapel Hill, North Carolina, USA.

Department of Immunology, Florida International University College of Medicine, Miami, Florida, USA.

出版信息

Biol Reprod. 2017 Oct 1;97(4):586-597. doi: 10.1093/biolre/iox103.

Abstract

Glyceraldehyde 3-phosphate dehydrogenase-S (GAPDHS) and phosphoglycerate kinase 2 (PGK2), two isozymes restricted to the male germline, catalyze successive steps in the glycolytic pathway in mammalian sperm. Although gene targeting of each isozyme demonstrated that glycolysis is required for normal sperm motility and male fertility, the phenotype of mice lacking GAPDHS is more severe than that of mice lacking PGK2. This study examined sperm function, signaling pathways, and metabolism to investigate factors that contribute to the phenotypic differences between these knockout models. Sperm from the two knockouts exhibited comparable deficits in zona binding, in vitro fertilization with or without zona drilling, and capacitation-dependent tyrosine phosphorylation. In contrast, signaling and metabolic differences were apparent prior to capacitation. Phosphorylation of sperm protein phosphatase 1, which has been associated with the acquisition of motile capacity during epididymal maturation, was deficient only in GAPDHS-null sperm. Carnitine, choline, phosphocholine, and taurine were elevated in sperm from both knockouts immediately after collection from the epididymis. However, only carnitine levels in PGK2-null sperm were significantly different from wild-type sperm, while all four metabolites were significantly higher in GAPDHS-null sperm. We confirmed that glycolysis is required for robust hyperactivation, but found that the motility of PGK2-null sperm improved to levels comparable to wild-type sperm with pyruvate as the sole metabolic substrate. This nonglycolysable substrate did not improve progressive motility in GAPDHS-null sperm. These results identify multiple signaling and metabolic defects that are likely contributors to male infertility and the absence of progressive sperm motility seen in mice lacking GAPDHS.

摘要

甘油醛-3-磷酸脱氢酶-S(GAPDHS)和磷酸甘油酸激酶 2(PGK2)是两种局限于精原细胞的同工酶,它们在哺乳动物精子的糖酵解途径中催化连续步骤。虽然两种同工酶的基因靶向都表明糖酵解是正常精子运动和雄性生育力所必需的,但缺乏 GAPDHS 的小鼠的表型比缺乏 PGK2 的小鼠更为严重。本研究检查了精子功能、信号通路和代谢,以研究导致这些敲除模型表型差异的因素。来自两种敲除的精子在透明带结合、体外受精(有或没有透明带钻孔)以及与顶体反应相关的酪氨酸磷酸化方面表现出相似的缺陷。相比之下,在顶体反应之前,信号和代谢差异明显。与获得附睾成熟过程中的运动能力相关的精子蛋白磷酸酶 1 的磷酸化仅在 GAPDHS 缺失的精子中缺乏。在从附睾中收集后立即,两种敲除的精子中的肉碱、胆碱、磷酸胆碱和牛磺酸都升高。然而,只有 PGK2 缺失的精子中的肉碱水平与野生型精子明显不同,而 GAPDHS 缺失的精子中的所有四种代谢物都明显升高。我们证实糖酵解是强烈的超激活所必需的,但发现 PGK2 缺失的精子的运动能力改善到与野生型精子相当的水平,而丙酮酸是唯一的代谢底物。这种非糖酵解底物并不能改善 GAPDHS 缺失的精子的进行性运动。这些结果确定了多种信号和代谢缺陷,这些缺陷可能是导致男性不育和缺乏 GAPDHS 缺失的精子进行性运动的原因。

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