Abstract

Methods currently exist for introducing cloned copies of genes into the mouse germ line to form transgenic mice. Recent studies indicate that under appropriate conditions introduced genes exhibit regulated expression characteristic of the endogenous genes. Moreover, methods are available for making defined modifications to cloned genes in vitro. Reintroduction of such modified genes into inbred mice affords novel opportunities for studying gene function and dissecting the mechanisms regulating complex gene interactions, such as those which typify physiologic homeostases, in higher animals. We propose to use such an approach to address issues pertinent to mammalian blood pressure regulation. In initial studies, we will use modified forms of renin structural gene and regulatory sequences in attempts to perturb normal physiological functions in inbred mice. Subsequently we plan to extend our studies to include other genetic components that contribute to blood pressure regulation and electrolyte balance. The initial types of modifications we will make are aimed at 1) overproducing natural murine renin at normal sites of synthesis, 2) placing renin synthesis under the control of regulatory elements that are insensitive to and independent of normal blood pressure physiologic signals, 3) producing renin polypeptides that are impaired or altered at catalytic sites and/or cellular processing and activation signals, and 4) transforming renin producing cells in situ using renin regulatory sequences fused to oncogenes. The effects of such perturbations will be monitored by directly assessing at various levels the expression of the inserted gene, the response of other known components of the regulatory network, and whole animal physiological parameters such as, for example, blood pressure and heart rate. Animals exhibiting interesting properties will then be bred to establish lines which will be available for continued study. Over the long term such in vitro mutagenesis coupled with a mammalian system that is readily manipulated genetically affords the best hope of establishing animal model systems for molecular genetic analysis of complex mechanisms governing physiological regulation in higher animals.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
1R01HL035792-01
Application #
3350089
Study Section
(SRC)
Project Start
1985-09-30
Project End
1990-09-29
Budget Start
1985-09-30
Budget End
1986-09-29
Support Year
1
Fiscal Year
1985
Total Cost
Indirect Cost

  Institution

Name
Roswell Park Cancer Institute Corp
Department
Type
DUNS #
City
Buffalo
State
NY
Country
United States
Zip Code
14263

  Publications

Jones, C A; Petrovic, N; Novak, E K et al. (1997) Biosynthesis of renin in mouse kidney tumor As4.1 cells. Eur J Biochem 243:181-90
Laframboise, M; Reudelhuber, T L; Jutras, I et al. (1997) Prorenin activation and prohormone convertases in the mouse As4.1 cell line. Kidney Int 51:104-9
Petrovic, N; Kane, C M; Sigmund, C D et al. (1997) Downregulation of renin gene expression by interleukin-1. Hypertension 30:230-5
Petrovic, N; Black, T A; Fabian, J R et al. (1996) Role of proximal promoter elements in regulation of renin gene transcription. J Biol Chem 271:22499-505
Abonia, J P; Abel, K J; Eddy, R L et al. (1993) Linkage of Agt and Actsk-1 to distal mouse chromosome 8 loci: a new conserved linkage. Mamm Genome 4:25-32
Schunkert, H; Tang, S S; Litwin, S E et al. (1993) Regulation of intrarenal and circulating renin-angiotensin systems in severe heart failure in the rat. Cardiovasc Res 27:731-5
Schunkert, H; Ingelfinger, J R; Hirsch, A T et al. (1993) Feedback regulation of angiotensin converting enzyme activity and mRNA levels by angiotensin II. Circ Res 72:312-8
Fabian, J R; Kane, C M; Abel, K J et al. (1993) Expression of the mouse Ren-1 gene in the coagulating gland: localization and regulation. Biol Reprod 48:1383-94
Schunkert, H; Ingelfinger, J R; Hirsch, A T et al. (1992) Evidence for tissue-specific activation of renal angiotensinogen mRNA expression in chronic stable experimental heart failure. J Clin Invest 90:1523-9
Andrawis, N S; Dzau, V J; Pratt, R E (1992) Autocrine stimulation of mas oncogene leads to altered growth control. Cell Biol Int Rep 16:547-56

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