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发动蛋白2是集合管中一种新型的一氧化氮合酶1β相互作用蛋白和负调节因子。

Dynamin-2 is a novel NOS1β interacting protein and negative regulator in the collecting duct.

作者信息

Hyndman Kelly A, Arguello Alexandra M, Morsing Sofia K H, Pollock Jennifer S

机构信息

Section of Cardio-Renal Physiology and Medicine, Division of Nephrology, Department of Medicine, University of Alabama at Birmingham, Birmingham, Alabama.

Section of Cardio-Renal Physiology and Medicine, Division of Nephrology, Department of Medicine, University of Alabama at Birmingham, Birmingham, Alabama

出版信息

Am J Physiol Regul Integr Comp Physiol. 2016 Apr 1;310(7):R570-7. doi: 10.1152/ajpregu.00008.2015. Epub 2016 Jan 20.

Abstract

Nitric oxide synthase 1 (NOS1)-derived nitric oxide (NO) production in collecting ducts is critical for maintaining fluid-electrolyte balance. Rat collecting ducts express both the full-length NOS1α and its truncated variant NOS1β, while NOS1β predominates in mouse collecting ducts. We reported that dynamin-2 (DNM2), a protein involved in excising vesicles from the plasma membrane, and NOS1α form a protein-protein interaction that promotes NO production in rat collecting ducts. NOS1β was found to be highly expressed in human renal cortical/medullary samples; hence, we tested the hypothesis that DNM2 is a positive regulator of NOS1β-derived NO production. COS7 and mouse inner medullary collecting duct-3 (mIMCD3) cells were transfected with NOS1β and/or DNM2. Coimmunoprecipitation experiments show that NOS1β and DNM2 formed a protein-protein interaction. DNM2 overexpression decreased nitrite production (index of NO) in both COS7 and mIMCD-3 cells by 50-75%. mIMCD-3 cells treated with a panel of dynamin inhibitors or DNM2 siRNA displayed increased nitrite production. To elucidate the physiological significance of IMCD DNM2/NOS1β regulation in vivo, flox control and CDNOS1 knockout mice were placed on a high-salt diet, and freshly isolated IMCDs were treated acutely with a dynamin inhibitor. Dynamin inhibition increased nitrite production by IMCDs from flox mice. This response was blunted (but not abolished) in collecting duct-specific NOS1 knockout mice, suggesting that DNM2 also negatively regulates NOS3 in the mouse IMCD. We conclude that DNM2 is a novel negative regulator of NO production in mouse collecting ducts. We propose that DNM2 acts as a "break" to prevent excess or potentially toxic NO levels under high-salt conditions.

摘要

集合管中一氧化氮合酶1(NOS1)衍生的一氧化氮(NO)生成对于维持体液电解质平衡至关重要。大鼠集合管同时表达全长的NOS1α及其截短变体NOS1β,而NOS1β在小鼠集合管中占主导地位。我们报道,参与从质膜切除囊泡的动力蛋白2(DNM2)与NOS1α形成蛋白质 - 蛋白质相互作用,促进大鼠集合管中的NO生成。发现NOS1β在人肾皮质/髓质样本中高表达;因此,我们测试了DNM2是NOS1β衍生的NO生成的正调节因子这一假设。将NOS1β和/或DNM2转染到COS7和小鼠肾内髓集合管 - 3(mIMCD3)细胞中。免疫共沉淀实验表明NOS1β和DNM2形成了蛋白质 - 蛋白质相互作用。DNM2的过表达使COS7和mIMCD - 3细胞中的亚硝酸盐生成(NO指标)降低了50 - 75%。用一组动力蛋白抑制剂或DNM2 siRNA处理的mIMCD - 3细胞显示亚硝酸盐生成增加。为了阐明体内IMCD中DNM2/NOS1β调节的生理意义,将flox对照小鼠和集合管特异性NOS1基因敲除小鼠置于高盐饮食中,并将新鲜分离的IMCD用动力蛋白抑制剂进行急性处理。动力蛋白抑制增加了flox小鼠IMCD的亚硝酸盐生成。在集合管特异性NOS1基因敲除小鼠中,这种反应减弱(但未消除),表明DNM2在小鼠IMCD中也对NOS3起负调节作用。我们得出结论,DNM2是小鼠集合管中NO生成的新型负调节因子。我们提出,DNM2起到“刹车”作用,以防止在高盐条件下NO水平过高或产生潜在毒性。

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