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携带血管紧张素1A受体基因“区域”靶向缺失的嵌合小鼠。关于局部血管紧张素在球旁细胞肾素合成体内反馈调节中作用的反对证据。

Chimeric mice carrying 'regional' targeted deletion of the angiotensin type 1A receptor gene. Evidence against the role for local angiotensin in the in vivo feedback regulation of renin synthesis in juxtaglomerular cells.

作者信息

Matsusaka T, Nishimura H, Utsunomiya H, Kakuchi J, Niimura F, Inagami T, Fogo A, Ichikawa I

机构信息

Department of Pediatrics, Vanderbilt University School of Medicine, Nashville, Tennessee 37232, USA.

出版信息

J Clin Invest. 1996 Oct 15;98(8):1867-77. doi: 10.1172/JCI118988.

Abstract

We have developed chimeric mice carrying 'regional' null mutation of the angiotensin type 1A (AT1A) receptor, the AT1 receptor subtype exclusively present in mouse juxtaglomerular (JG) cells. The chimeric mouse (Agtr1a -/- <--> +/+) is made up of wild-type (Agtr1a +/+) cells or cells homozygous for Agtr1a deletion (Agtr1a -/-). In the latter, the AT1A coding exon was replaced with a reporter gene, lacZ. In Agtr1a -/- <--> +/+ mice, these two clones of cells are found to be clustered and display patchy distributions in the kidney and heart. Tracking of lacZ activities in hetero- (Agtr1a +/-) and homozygous (Agtr1a -/-) deletion mutant offspring from Agtr1a -/- <--> +/+ mice revealed that the promoter activity of Agtr1a is localized in JG cells, afferent arteriolar walls, glomerular mesangial region and endothelial cells, and apical and basolateral proximal tubule membranes. The JG apparatuses of Agtr1a -/- mice are markedly enlarged with intense expression of renin mRNA and protein. In Agtr1a -/- <--> +/+ mice, these changes were proportional to the degree of chimerism. Within a given Agtr1a -/- <--> +/+ mouse, however, the degree of JG hypertrophy/hyperplasia and the expression of renin mRNA and protein were identical between Agtr1a +/+ and Agtr1a -/- cells. Thus, in the in vivo condition tested, the local interaction between angiotensin and the AT1 receptor on the JG cells has little functional contribution to the feedback regulation of JG renin synthesis.

摘要

我们培育出了携带血管紧张素1A(AT1A)受体“区域”无效突变的嵌合小鼠,AT1受体亚型仅存在于小鼠肾小球旁(JG)细胞中。嵌合小鼠(Agtr1a -/- <--> +/+)由野生型(Agtr1a +/+)细胞或Agtr1a缺失纯合子(Agtr1a -/-)细胞组成。在后者中,AT1A编码外显子被报告基因lacZ取代。在Agtr1a -/- <--> +/+小鼠中,发现这两种细胞克隆聚集在一起,并在肾脏和心脏中呈斑驳分布。追踪Agtr1a -/- <--> +/+小鼠的杂合子(Agtr1a +/-)和纯合子(Agtr1a -/-)缺失突变后代中的lacZ活性,发现Agtr1a的启动子活性定位于JG细胞、入球小动脉壁、肾小球系膜区和内皮细胞,以及近端小管的顶端和基底外侧膜。Agtr1a -/-小鼠的JG装置明显增大,肾素mRNA和蛋白表达强烈。在Agtr1a -/- <--> +/+小鼠中,这些变化与嵌合程度成正比。然而,在给定的Agtr1a -/- <--> +/+小鼠体内,Agtr1a +/+和Agtr1a -/-细胞之间的JG肥大/增生程度以及肾素mRNA和蛋白的表达是相同的。因此,在测试的体内条件下,血管紧张素与JG细胞上的AT1受体之间的局部相互作用对JG肾素合成的反馈调节几乎没有功能贡献。

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