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动力蛋白通过与 NOS1 的蛋白-蛋白相互作用激活大鼠肾髓质集合管中的 NO 产生。

Dynamin activates NO production in rat renal inner medullary collecting ducts via protein-protein interaction with NOS1.

机构信息

Vascular Biology Center, CB-3213, Medical College of Georgia, Georgia Health Sciences University, Augusta, GA 30912, USA.

出版信息

Am J Physiol Renal Physiol. 2011 Jul;301(1):F118-24. doi: 10.1152/ajprenal.00534.2010. Epub 2011 Apr 13.

Abstract

We hypothesized that nitric oxide synthase (NOS) isoforms may be regulated by dynamin (DNM) in the inner medullary collecting duct (IMCD). The aims of this study were to determine which DNM isoforms (DNM1, DNM2, DNM3) are expressed in renal IMCDs, whether DNM interacts with NOS, whether a high-salt diet alters the interaction of DNM and NOS, and whether DNM activates NO production. DNM2 and DNM3 are highly expressed in the rat IMCD, while DNM1 is localized outside of the IMCD. We found that DNM1 interacts with NOS1α, NOS1β, and NOS3 in the inner medulla of male Sprague-Dawley rats on a 0.4% salt diet. DNM2 interacts with NOS1α, while DNM3 interacts with both NOS1α and NOS1β. DNM2 and DNM3 do not interact with NOS3 in the rat inner medulla. We did not observe any change in the DNM/NOS interactions with rats on a 4% salt diet after 7 days. Furthermore, NOS1α interacts with DNM2 in mIMCD3 and COS7 cells transfected with NOS1α and DNM2-GFP constructs and the NOS1 reductase domain is necessary for the interaction. Finally, COS7 cells expressing NOS1α or NOS1α/DNM2-GFP had significantly higher nitrite production compared with DNM2-GFP only. Nitrite production was blocked by the DNM inhibitor dynasore or the dominant negative DNM2K44A. Ionomycin stimulation further increased nitrite production in the NOS1α/DNM2-GFP cells compared with NOS1α only. In conclusion, DNM and NOS1 interact in the rat renal IMCD and this interaction leads to increased NO production, which may influence NO production in the renal medulla.

摘要

我们假设一氧化氮合酶 (NOS) 同工型可能受动蛋白 (DNM) 在髓质集合管 (IMCD) 内的调节。本研究的目的是确定哪种 DNM 同工型 (DNM1、DNM2、DNM3) 在肾脏 IMCD 中表达,DNM 是否与 NOS 相互作用,高盐饮食是否改变 DNM 和 NOS 的相互作用,以及 DNM 是否激活 NO 产生。DNM2 和 DNM3 在大鼠 IMCD 中高度表达,而 DNM1 位于 IMCD 之外。我们发现 DNM1 在雄性 Sprague-Dawley 大鼠 0.4%盐饮食的内髓质中与 NOS1α、NOS1β 和 NOS3 相互作用。DNM2 与 NOS1α 相互作用,而 DNM3 与 NOS1α 和 NOS1β 相互作用。DNM2 和 DNM3 与大鼠内髓质中的 NOS3 没有相互作用。我们没有观察到在大鼠 4%盐饮食 7 天后 DNM/NOS 相互作用的任何变化。此外,NOS1α 与 mIMCD3 和转染了 NOS1α 和 DNM2-GFP 构建体的 COS7 细胞中的 DNM2 相互作用,并且 NOS1 还原酶结构域是相互作用所必需的。最后,与仅表达 DNM2-GFP 的 COS7 细胞相比,表达 NOS1α 或 NOS1α/DNM2-GFP 的 COS7 细胞的亚硝酸盐产量显著更高。亚硝酸盐的产生被 DNM 抑制剂 dynasore 或显性负性 DNM2K44A 阻断。与仅 NOS1α 相比,离子霉素刺激进一步增加了 NOS1α/DNM2-GFP 细胞中亚硝酸盐的产生。总之,DNM 和 NOS1 在大鼠肾脏 IMCD 中相互作用,这种相互作用导致 NO 产生增加,这可能影响肾脏髓质中的 NO 产生。

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