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肾脏促红细胞生成素信使核糖核酸的生理调节及组织定位

Physiologic regulation and tissue localization of renal erythropoietin messenger RNA.

作者信息

Schuster S J, Wilson J H, Erslev A J, Caro J

出版信息

Blood. 1987 Jul;70(1):316-8.

PMID:3593969
Abstract

Although erythropoietin (Epo) is produced primarily by the kidneys in response to hypoxia, the precise cell type(s) and mechanisms by which these cells regulate production are poorly understood. In the experiments we report, the kinetics of renal Epo production in response to acute hypoxia and the intrarenal localization of cellular Epo synthesis were studied at the level of Epo mRNA. Erythropoietin mRNA expression was determined by Northern blot analysis of rat kidney RNAs using a probe derived from the mouse Epo gene. Renal Epo mRNA content increased as early as 1 hour after initiation of hypoxia and continued to accumulate during 4 hours of stimulation. Discontinuation of the hypoxic stimulus resulted in rapid decay of mRNA levels. Kidney and plasma Epo levels measured by radioimmunoassay paralleled, with respective lag times, the changes in renal Epo mRNA content, suggesting that Epo production in response to acute hypoxia represents de novo synthesis and is regulated by changes in Epo mRNA. Northern blot analysis of RNAs extracted from separated glomerular and tubular tissue fractions revealed Epo mRNA in the tubular fraction, whereas glomerular tissue did not contain Epo mRNA. Thus, the site of cellular Epo synthesis is located in the renal tubule or its interstitium and not in the glomerular tuft.

摘要

尽管促红细胞生成素(Epo)主要由肾脏在低氧状态下产生,但这些细胞调节其产生的精确细胞类型和机制仍知之甚少。在我们报告的实验中,在促红细胞生成素mRNA水平上研究了急性低氧反应中肾脏促红细胞生成素产生的动力学以及细胞促红细胞生成素合成在肾脏内的定位。使用源自小鼠促红细胞生成素基因的探针,通过对大鼠肾脏RNA进行Northern印迹分析来测定促红细胞生成素mRNA的表达。低氧开始后1小时,肾脏促红细胞生成素mRNA含量就开始增加,并在刺激的4小时内持续积累。停止低氧刺激导致mRNA水平迅速下降。通过放射免疫测定法测量的肾脏和血浆促红细胞生成素水平,分别有相应的延迟时间,与肾脏促红细胞生成素mRNA含量的变化平行,这表明急性低氧反应中的促红细胞生成素产生代表从头合成,并受促红细胞生成素mRNA变化的调节。对从分离的肾小球和肾小管组织部分提取的RNA进行Northern印迹分析,结果显示肾小管部分存在促红细胞生成素mRNA,而肾小球组织中不含促红细胞生成素mRNA。因此,细胞促红细胞生成素合成的部位位于肾小管或其间质中而非肾小球丛。

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