Luiking Yvette C, Hallemeesch Marcella M, Lamers Wouter H, Deutz Nicolaas E P
Dept. of Surgery, Maastricht Univ., PO Box 616, NL-6200 MD Maastricht, The Netherlands.
Am J Physiol Renal Physiol. 2005 Apr;288(4):F816-22. doi: 10.1152/ajprenal.00308.2004. Epub 2004 Nov 16.
Previously, we observed an enhanced renal protein synthesis and increased de novo arginine production in the early response to endotoxemia in wild-type Swiss mice (Hallemeesch MM, Soeters PB, and Deutz NE. Am J Physiol Renal Physiol 282: F316-F323, 2002). To establish whether these changes are regulated by nitric oxide (NO) synthesized by NO synthase isoforms NOS2 and NOS3, we studied C57BL6/J wild-type (WT), NOS2-deficient (NOS2(-/-)), and NOS3-deficient (NOS3(-/-)) mice under baseline (unstimulated) and LPS-treated conditions. The metabolism of renal protein, amino acid, and arginine was studied at the whole body level and across the kidney by infusing the stable isotopes l-[phenyl-(2)H(5)]phenylalanine, l-[phenyl-(2)H(2)]tyrosine, l-guanidino-[(15)N(2)]arginine, and l-[ureido-(13)C,(2)H(2)]citrulline. Renal blood flow was measured using radioactive PAH extraction. Under baseline conditions, renal blood flow was significantly reduced in NOS2(-/-) mice (0.29 +/- 0.01 vs. 0.48 +/- 0.07 ml.10 g body wt(-1).min(-1) in WT) (P < 0.05), and de novo arginine production was lower in NOS2(-/-) mice. After LPS challenge, renal protein turnover and arginine production increased in all three groups (P < 0.05), even though renal de novo arginine synthesis did not increase. The expected increase in renal citrulline production and disposal after LPS was not observed in NOS2(-/-) mice (P = 0.06). Collectively, these data show that NOS2 is constitutively expressed in the kidney and remarkably functional as it affects renal blood flow and de novo arginine production under baseline conditions and is important for the increase in renal citrulline turnover during endotoxemia. NOS3, in contrast, appears less important for renal metabolism. The increase in renal protein turnover during endotoxemia does not depend on NOS2 or NOS3 activity.
此前,我们观察到野生型瑞士小鼠在内毒素血症早期反应中肾蛋白合成增强且从头合成精氨酸增加(哈勒梅施·M·M、索特斯·P·B和多伊茨·N·E。《美国生理学杂志:肾脏生理学》282卷:F316 - F323,2002年)。为确定这些变化是否受一氧化氮合酶同工型NOS2和NOS3合成的一氧化氮(NO)调节,我们研究了C57BL6/J野生型(WT)、NOS2缺陷型(NOS2(-/-))和NOS3缺陷型(NOS3(-/-))小鼠在基线(未刺激)和脂多糖处理条件下的情况。通过输注稳定同位素l - [苯基 - (2)H(5)]苯丙氨酸、l - [苯基 - (2)H(2)]酪氨酸、l - 胍基 - [(15)N(2)]精氨酸和l - [脲基 - (13)C,(2)H(2)]瓜氨酸,在全身水平和整个肾脏研究肾蛋白、氨基酸和精氨酸的代谢。使用放射性对氨基马尿酸提取法测量肾血流量。在基线条件下,NOS2(-/-)小鼠的肾血流量显著降低(0.29±0.01对野生型小鼠的0.48±0.07 ml·10 g体重(-1)·min(-1))(P < 0.05),且NOS2(-/-)小鼠的从头合成精氨酸减少。脂多糖攻击后,尽管肾从头合成精氨酸未增加,但三组的肾蛋白周转和精氨酸生成均增加(P < 0.05)。在NOS2(-/-)小鼠中未观察到脂多糖攻击后肾瓜氨酸生成和处置的预期增加(P = 0.06)。总体而言,这些数据表明NOS2在肾脏中组成性表达且功能显著,因为它在基线条件下影响肾血流量和从头合成精氨酸,并且在内毒素血症期间对肾瓜氨酸周转增加很重要。相比之下,NOS3对肾脏代谢似乎不太重要。内毒素血症期间肾蛋白周转的增加不依赖于NOS2或NOS3的活性。
