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在离体兔皮质肾单位中盐皮质激素作用靶点的鉴定

Identification of mineralocorticoid target sites in the isolated rabbit cortical nephron.

作者信息

Marver D, Schwartz M J

出版信息

Proc Natl Acad Sci U S A. 1980 Jun;77(6):3672-6. doi: 10.1073/pnas.77.6.3672.

Abstract

Previous evidence suggests that the activity of the mitochondrial enzyme citrate synthase [citrate oxaloacetate-lyase (pro-3S-CH(2)COO --> acetyl-CoA), EC 4.1.3.7] is increased in target tissues upon acute administration of aldosterone. Therefore, an ultramicro assay was established to determine citrate synthase levels in isolated rabbit nephron segments as a means of localizing mineralocorticoid-responsive sites within the renal cortex. The relative citrate synthase activities in normal rabbit segments (per kg of dry tissue) correlated with the metabolic activity of the segments. The order was: distal convoluted tubule > proximal convoluted tubule > cortical thick ascending limb of Henle > cortical collecting duct > pars recta. When these segments were isolated from adrenalectomized rabbits, only the citrate synthase activity in the cortical collecting duct was significantly decreased compared to normal values (3.2 mol of citrate/kg dry wt per hr compared to 7.1; P < 0.001). Furthermore, enzyme activities in segments isolated from adrenalectomized rabbits 90 min after intravenous injection of aldosterone (10 mug/kg) were unchanged from normal or adrenalectomized rabbit tubule values for all segments except the cortical collecting duct. In this segment, aldosterone significantly increased citrate synthase activity compared to adrenalectomized rabbit values (8.1 mol/kg per hr compared to 3.2; P < 0.001), in contrast to the effect of dexamethasone at 10 mug/kg (4.4 mol/kg per hr compared to 3.2; P, NS). Spirolactone SC 26304 administered 30 min prior to injection of aldosterone inhibited the increase in collecting duct citrate synthase activity seen with aldosterone alone (3.4 mol/kg per hr compared to 8.1; P < 0.001). These findings suggest that the collecting duct is the primary target for aldosterone in the renal cortex.

摘要

先前的证据表明,急性给予醛固酮后,靶组织中线粒体酶柠檬酸合酶[柠檬酸草酰乙酸裂解酶(pro-3S-CH(2)COO→乙酰辅酶A),EC 4.1.3.7]的活性会增加。因此,建立了一种超微量测定法来测定分离的兔肾单位节段中的柠檬酸合酶水平,以此作为在肾皮质内定位盐皮质激素反应位点的一种方法。正常兔节段(每千克干组织)中柠檬酸合酶的相对活性与节段的代谢活性相关。顺序为:远曲小管>近曲小管>亨氏袢皮质厚升支>皮质集合管>直部。当从肾上腺切除的兔子中分离出这些节段时,与正常值相比,仅皮质集合管中的柠檬酸合酶活性显著降低(每小时每千克干重3.2摩尔柠檬酸,而正常值为7.1;P<0.001)。此外,在静脉注射醛固酮(10微克/千克)90分钟后,从肾上腺切除的兔子中分离出的节段中,除皮质集合管外,所有节段的酶活性与正常或肾上腺切除的兔肾小管值相比均未改变。在该节段中,与肾上腺切除的兔子的值相比,醛固酮显著增加了柠檬酸合酶活性(每小时每千克8.1摩尔,而肾上腺切除的兔子为3.2;P<0.001),这与10微克/千克地塞米松的作用相反(每小时每千克4.4摩尔,而肾上腺切除的兔子为3.2;P,无显著性差异)。在注射醛固酮前30分钟给予螺内酯SC 26304可抑制单独使用醛固酮时观察到的集合管柠檬酸合酶活性增加(每小时每千克3.4摩尔,而单独使用醛固酮时为每小时每千克8.1摩尔;P<0.001)。这些发现表明,集合管是肾皮质中醛固酮的主要靶标。

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