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一氧化氮在调节牛黄体内皮细胞中超氧化物歧化酶和前列腺素F(2α)生成中的作用。

Role of nitric oxide in the regulation of superoxide dismutase and prostaglandin F(2alpha) production in bovine luteal endothelial cells.

作者信息

Lee Seunghyung, Acosta Tomas J, Nakagawa Yuji, Okuda Kiyoshi

机构信息

Laboratory of Reproductive Endocrinology, Graduate School of Natural Science and Technology, Okayama University, Okayama, Japan.

出版信息

J Reprod Dev. 2010 Aug;56(4):454-9. doi: 10.1262/jrd.10-013k. Epub 2010 Jun 1.

DOI:10.1262/jrd.10-013k
PMID:20519832
Abstract

Prostaglandin F(2alpha) (PGF) induces a rapid reduction in progesterone production (functional luteolysis) followed by tissue degeneration and cell death (structural luteolysis). Reactive oxygen species (ROS) including nitric oxide (NO) play crucial roles in the luteolytic action of PGF. The local concentration of intraluteal ROS is controlled by superoxide dismutase (SOD), the main enzyme involved in the control of intraluteal ROS. To clarify the roles of NO in the regulation of SOD in luteolysis, we examined the effects of NO on SOD expression and activity in cultured bovine luteal endothelial cells (LECs) during short-term (2 h, mimicking functional luteolysis) and long-term (24 h, mimicking structural luteolysis) incubation. We also investigated whether NO modulates PGF production by LECs. LECs were isolated from mid-luteal phase CLs, and exposed to NONOate (a NO donor) for 2 or 24 h. SOD mRNA expression was stimulated by NONOate (10-100 microM) at 2 h (P<0.05). Moreover, 10 microM NONOate stimulated SOD protein expression and SOD activity at 2 h (P<0.05), whereas NONOate inhibited SOD mRNA and protein expressions at 24 h (P<0.05). NONOate stimulated PGF biosynthesis at both incubation times. The overall findings suggest that NO differently regulates SOD in cultured LECs, depending on the exposure time. Acute elevation of SOD may represent a response of LECs to protect themselves against oxidative stress induced by PGF during functional luteolysis, whereas a later reduction of SOD levels by NO may facilitate an excess of intraluteal ROS during structural luteolysis.

摘要

前列腺素F(2α)(PGF)可迅速降低孕酮生成(功能性黄体溶解),随后导致组织退化和细胞死亡(结构性黄体溶解)。包括一氧化氮(NO)在内的活性氧(ROS)在PGF的黄体溶解作用中起关键作用。黄体中ROS的局部浓度由超氧化物歧化酶(SOD)控制,SOD是参与控制黄体中ROS的主要酶。为了阐明NO在黄体溶解过程中对SOD调节的作用,我们研究了在短期(2小时,模拟功能性黄体溶解)和长期(24小时,模拟结构性黄体溶解)孵育期间,NO对培养的牛黄体内皮细胞(LECs)中SOD表达和活性的影响。我们还研究NO是否调节LECs产生PGF。从黄体中期的黄体中分离出LECs,并将其暴露于NONOate(一种NO供体)2或24小时。在2小时时,NONOate(10 - 100微摩尔)刺激SOD mRNA表达(P<0.05)。此外,10微摩尔NONOate在2小时时刺激SOD蛋白表达和SOD活性(P<0.05),而在24小时时,NONOate抑制SOD mRNA和蛋白表达(P<0.05)。在两个孵育时间点,NONOate均刺激PGF生物合成。总体研究结果表明,根据暴露时间不同,NO对培养的LECs中SOD的调节作用也不同。SOD的急性升高可能代表LECs在功能性黄体溶解期间为保护自身免受PGF诱导的氧化应激而做出的反应,而后期NO导致SOD水平降低可能会在结构性黄体溶解期间促进黄体中ROS过量。

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