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Am J Physiol Renal Physiol 288: F214-F220, 2005. First published October 26, 2004; doi:10.1152/ajprenal.00258.2004
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Expression profile of a human inducible nitric oxide synthase promoter reporter in transgenic mice during endotoxemia

Zhiyuan Yu,1 Xuefeng Xia,1 and Bruce C. Kone1,2,3

Departments of 1Internal Medicine and Integrative Biology, 2Pharmacology, and Physiology, and 3The Brown Foundation Institute of Molecular Medicine for the Prevention of Human Diseases, The University of Texas Health Sciences Center at Houston, Houston, Texas

Submitted 14 July 2004 ; accepted in final form 3 September 2004

Inducible nitric oxide synthase (iNOS) is involved in many physiological and pathophysiological processes, including septic shock and acute kidney failure. Little is known about transcriptional regulation of the human iNOS gene in vivo under basal conditions or in sepsis. Accordingly, we developed transgenic mice carrying an insertional human iNOS promoter-reporter gene construct. In these mice, the proximal 8.3 kb of the human iNOS 5'-flanking region controls expression of the reporter gene of enhanced green fluorescent protein (EGFP). Patterns of human iNOS promoter/EGFP transgene expression in tissues were examined by fluorescence microscopy and immunoblotting. Endogenous murine iNOS was basally undetectable in kidney, intestine, spleen, heart, lung, liver, stomach, or brain. In contrast, EGFP from the transgene was basally expressed in kidney, brain, and spleen, but not the other tissues of the transgenic mice. Bacterial lipopolysaccharide induced endogenous iNOS expression in kidney, intestine, spleen, lung, liver, stomach, and heart, but not brain. In contrast, human iNOS promoter/EGFP transgene expression was induced above basal levels only in intestine, spleen, brain, stomach, and lung. Within kidney, human iNOS promoter/EGFP fluorescence was detected most prominently in proximal tubules of the outer cortex and collecting ducts and colocalized with endogenous mouse iNOS. Within the collecting duct, both endogenous iNOS and the human iNOS promoter/EGFP transgene were expressed in cells lacking aquaporin-2 immunoreactivity, consistent with expression in intercalated cells. Although it remains possible that essential regulatory elements reside in remote locations of the gene, our data concerning this 8.3-kb region provide the first in vivo evidence suggesting differential transcriptional control of the human iNOS gene in these organs and marked differences in transcriptional regulatory regions between the murine and human genes.

green fluorescent protein; gene transcription; lipopolysaccharide; kidney



Address for reprint requests and other correspondence: B. C. Kone, Chairman, Dept. of Internal Medicine, The Univ. of Texas Medical School at Houston, 6431 Fannin, MSB 1.150, Houston, TX 77030 (E-mail: Bruce.C.Kone{at}uth.tmc.edu)




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