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人肾素肾脏增强子是维持肾素基线表达所必需的,但对于组织特异性、细胞特异性和调控表达而言并非必需。

The human renin kidney enhancer is required to maintain base-line renin expression but is dispensable for tissue-specific, cell-specific, and regulated expression.

作者信息

Zhou Xiyou, Davis Deborah R, Sigmund Curt D

机构信息

Molecular and Cellular Biology Graduate Program, Department of Internal Medicine, Roy J. and Lucille A. Carver College of Medicine, University of Iowa, Iowa City, Iowa 52242, USA.

出版信息

J Biol Chem. 2006 Nov 17;281(46):35296-304. doi: 10.1074/jbc.M608055200. Epub 2006 Sep 21.

DOI:10.1074/jbc.M608055200
PMID:16990260
Abstract

Renin is the rate-limiting enzyme in the renin-angiotensin system and thus dictates the level of the pressor hormone angiotensin-II. The classical site of renin expression and secretion is the renal juxtaglomerular cell, where its expression is tightly regulated by physiological cues. An evolutionarily conserved transcriptional enhancer located 11 kb upstream of the human RENIN gene has been reported to markedly enhance transcription in renin expressing cells in vitro. However, its importance in vivo remains unclear. We tested whether this enhancer is required for appropriate tissue- and cell-specific expression, or for physiological regulation of the human RENIN gene. To accomplish this, we used a retrofitting technique employing homologous recombination in bacteria to delete the enhancer from a 160-kb P1-artificial chromosome containing human RENIN, two upstream genes and one downstream gene, and then generated two lines of transgenic mice. We previously showed that human renin expression in transgenic mice containing the wild type construct is tightly regulated as is expression of the linked genes. Deletion of the enhancer had no effect on tissue-specific expression of human RENIN, but using the downstream gene as an internal control, found that human RENIN mRNA levels were 3-10-fold decreased compared with constructs containing the enhancer. Despite this decrease in expression, renin protein remained localized to renal juxtaglomerular cells and was appropriately regulated by cues that either increase or decrease expression of renin. Our results suggest that sequences other than the enhancer may be necessary for tissue-specific, cell-specific, and regulated expression of human RENIN.

摘要

肾素是肾素-血管紧张素系统中的限速酶,因此决定了升压激素血管紧张素II的水平。肾素表达和分泌的经典部位是肾近球细胞,其表达受生理信号严格调控。据报道,位于人类肾素基因上游11 kb处的一个进化保守的转录增强子在体外能显著增强肾素表达细胞中的转录。然而,其在体内的重要性仍不清楚。我们测试了该增强子对于人类肾素基因的适当组织和细胞特异性表达或生理调节是否必要。为实现这一点,我们使用了一种改造技术,利用细菌中的同源重组从一个包含人类肾素、两个上游基因和一个下游基因的160 kb P1人工染色体中删除该增强子,然后生成了两系转基因小鼠。我们之前表明,含有野生型构建体的转基因小鼠中的人类肾素表达与相关基因的表达一样受到严格调控。增强子的缺失对人类肾素的组织特异性表达没有影响,但以下游基因作为内部对照,发现与含有增强子的构建体相比,人类肾素mRNA水平降低了3至10倍。尽管表达有所下降,但肾素蛋白仍定位于肾近球细胞,并受到增加或减少肾素表达的信号的适当调控。我们的结果表明,除增强子外的其他序列可能是人类肾素组织特异性、细胞特异性和调控表达所必需的。

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