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Oxygen metabolism of mammalian spermatozoa. Generation of hydrogen peroxide by rabbit epididymal spermatozoa

机译:哺乳动物精子的氧代谢。兔附睾精子产生过氧化氢

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摘要

Rabbit spermatozoa from the cauda epididymis produced 0.7–0.8nmol of H2O2/min per 108 cells at cell concentrations below 107 cells/ml with linear dependence on cell concentration. Above 2 × 107 cells/ml, the rate again became linear with cell concentration but decreased to 0.1–0.2nmol/min per 108 cells. Spermatozoa treated with amphotericin B, which makes the plasma membrane highly permeable to low-molecular-weight compounds, showed a similar dependence of H2O2 production rate on cell concentration; below 107 cells/ml the rate was 0.3–0.4nmol/min per 108 cells; above 2 × 107 cells/ml, the rate was 0.1–0.2nmol/min per 108 cells. Hypo-osmotically treated rabbit epididymal spermatozoa, a preparation useful for studying mitochondrial function in sperm [Keyhani & Storey (1973) Biochim. Biophys. Acta 305, 557–565] produced 0.1–0.2nmol/min per 108 cells in the absence of added substrates. The dependence of rate on cell concentration was linear from 107 to 2.2 × 108 cells/ml. This endogenous rate was unaffected by rotenone, but stimulated 4-fold by antimycin A. Addition of the mitochondrial substrates lactate plus malate increased the rate of H2O2 production to 0.3nmol/min per 108 cells. The decreased rate of H2O2 production observed with intact sperm at high cell concentrations is attributed to reaction of H2O2 with the cells, possibly with the plasma membrane, which is lost after hypo-osmotic treatment. Rabbit spermatozoa have glutathione peroxidase and glutathione reductase activities, but these seem to play little role in removal of H2O2 generated. The rate at low cell concentration is taken to be the unperturbed rate. The sources of H2O2 production in rabbit spermatozoa have been tentatively resolved into a low-molecular-weight component, lost after amphotericin treatment, a mitochondrial component and a rotenone-insensitive component that has not been identified.
机译:来自附睾马尾的兔精子每108个细胞在低于107个细胞/毫升的细胞浓度下产生0.7-0.8nmol的H2O2 / min,线性依赖于细胞浓度。高于2×107细胞/ ml时,速率再次与细胞浓度成线性关系,但降至每108个细胞0.1-0.2nmol / min。用两性霉素B处理的精子使质膜对低分子量化合物具有高渗透性,并显示出H2O2产生速率对细胞浓度的相似依赖性;低于107个细胞/毫升时,每108个细胞的速率为0.3-0.4nmol / min;高于2×107细胞/ ml时,速率为每108个细胞0.1-0.2nmol / min。经低渗处理的兔附睾精子,一种可用于研究精子中线粒体功能的制剂[Keyhani&Storey(1973)Biochim。生物物理学。在没有添加底物的情况下,Acta 305,557–565]每108个细胞产生0.1–0.2nmol / min。速率对细胞浓度的依赖性从107到​​2.2×108细胞/ ml呈线性关系。该内源性速率不受鱼藤酮的影响,但被抗霉素A刺激4倍。线粒体底物乳酸和苹果酸的添加使H2O2生成速率增加到每108个细胞0.3nmol / min。完整精子在高细胞浓度下观察到的H2O2产生速率降低归因于H2O2与细胞(可能与质膜)的反应,在低渗处理后这种反应会丢失。兔精子具有谷胱甘肽过氧化物酶和谷胱甘肽还原酶活性,但这些似乎在去除生成的H2O2中几乎没有作用。低细胞浓度下的速率被认为是不受干扰的速率。兔子精子中H2O2的产生来源已被初步解析为低分子量成分,两性霉素处理后会丢失,线粒体成分和鱼藤酮不敏感成分尚未确定。

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