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大鼠肾脏中肾素和脑型一氧化氮合酶(b-NOS)mRNA水平的协同变化。

Coordinate changes of renin and brain-type nitric-oxide-synthase (b-NOS) mRNA levels in rat kidneys.

作者信息

Schricker K, Pötzl B, Hamann M, Kurtz A

机构信息

Institut für Physiology I, Universität Regensburg, Postfach 101042, D-93040 Regensburg, Germany.

出版信息

Pflugers Arch. 1996 Jul;432(3):394-400. doi: 10.1007/s004240050150.

Abstract

In our study we have examined the mRNA levels of nitric-oxide-(NO-)synthases in rat kidneys during states of stimulated and reduced renin gene expression, to find out whether renal mRNA levels of NO-synthases are correlated with the activity of the renin system. Stimulation of the renin system was achieved by unilateral renal artery clipping (2-kidney/1-clip rats), treatment with the angiotensin II (ANG II) antagonist losartan (40 mg/kg), application of furosemide (12 mg x kg-1 x day-1) and a low-sodium diet (0.02% w/w Na+), which increased renin mRNA levels to 464%, 495%, 309% and 219% of those of control animals, respectively. Inhibition of the renin system was achieved in the nonclipped (contralateral) kidneys of 2-kidney/1-clip rats and in the kidneys of rats which were fed a high-sodium diet (4% w/w Na+); in both cases renin mRNA levels decreased to about 50% of the control values. First screening of the gene expression of brain-type NO-synthase (b-NOS), endothelial NOS (e-NOS) and inducible NOS (i-NOS) during all these alterations of the renin system was done using the reverse transcriptase-polymerase chain reaction (RT-PCR) technique. Results from such noncompetitive PCR experiments indicated that only b-NOS mRNA levels change concordantly with the levels of renin. These changes in b-NOS mRNA levels were checked by the more reliable method of RNase protection assay. Results of the RNase protection assay proved that the renal levels of b-NOS mRNA were significantly increased by about 50% after a low-sodium diet and hypoperfusion of the kidney. Given a stimulatory role of endothelium-derived relaxing factor (EDRF)/NO on the renin system our findings may provide the first evidence that increases of renal levels of b-NOS mRNA and, as a consequence, of renal EDRF/NO formation could be important mediators of the well-known effect of salt intake and hypoperfusion on the renin system.

摘要

在我们的研究中,我们检测了大鼠肾脏中一氧化氮合酶(NO合酶)在肾素基因表达受刺激和降低状态下的mRNA水平,以确定肾脏中NO合酶的mRNA水平是否与肾素系统的活性相关。通过单侧肾动脉夹闭(2肾/1夹大鼠)、用血管紧张素II(ANG II)拮抗剂氯沙坦(40 mg/kg)治疗、应用呋塞米(12 mg·kg⁻¹·天⁻¹)和低钠饮食(0.02% w/w Na⁺)来刺激肾素系统,这些处理分别使肾素mRNA水平增加至对照动物的464%、495%、309%和219%。在2肾/1夹大鼠的未夹闭(对侧)肾脏以及喂食高钠饮食(4% w/w Na⁺)的大鼠肾脏中抑制肾素系统;在这两种情况下,肾素mRNA水平均降至对照值的约50%。在肾素系统的所有这些变化过程中,使用逆转录聚合酶链反应(RT-PCR)技术首次筛查脑型NO合酶(b-NOS)、内皮型NOS(e-NOS)和诱导型NOS(i-NOS)的基因表达。这种非竞争性PCR实验的结果表明,只有b-NOS mRNA水平与肾素水平一致变化。通过更可靠的核糖核酸酶保护分析方法检查了b-NOS mRNA水平的这些变化。核糖核酸酶保护分析结果证明,低钠饮食和肾脏灌注不足后,肾脏中b-NOS mRNA水平显著增加约50%。鉴于内皮源性舒张因子(EDRF)/NO对肾素系统具有刺激作用,我们的发现可能首次证明肾脏中b-NOS mRNA水平的增加以及由此导致的肾脏EDRF/NO生成的增加可能是盐摄入和灌注不足对肾素系统的众所周知的影响的重要介导因素。

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