Abstract

The juxtaglomerular apparatus (JGA) is an assemblage of cells known to be the site of formation and secretion of the renal hypertensive material renin and its anatomical arrangement suggests that it functions as an intrinsic renal regulator of hemodynamics and glomerular filtration. Through these actions, the JGA has the potential to affect the levels of arterial blood pressure. This is the basis for the hypothesis that alterations in JGA function may contribute to some types of hypertensive disease. The long-term objective of this project is to understand how the JGA processes hemodynamic, tabular transport, neural, and humoral information to regulate glomerular filtration, blood flow, and renin release. With a few notable exceptions, specific information about the cells of the JGA is derived from structural studies utilizing light and electron microscopy. Progress on the cell biology and biochemistry of this important group of cells has been limited by their relative inaccessability and the small amount of material in each nephron. This proposal seeks support to develop a convenient method for the isolation of granular and macula densa cells and the subsequent growth of these cells in culture. In the first phase we will develop monoclonal antibodies directed against cell surface antigens to be used as bioaffinity reagents to isolate relatively large quantities of renin-containing and macula densa cells from collagenase dispersions of rabbit and dog kidney cortex. With the ability to isolate specific cell types from the JGA we will proceed to a second phase where we will systemically evaluate growth media and substrata conditions in order to develop culture conditions that best support retention of differentiated properties. Culture conditions for granular cells will be established by determining to conditions necessary to observe modulation of renin production by the cells in response to factors that have been previously found to influence renin release in the intact animal. Culture conditions for macula densa cells will be determined by immuno- and histochemical techniques using antigenic or enzymatic markers previously determined in situ. It is anticipated that the use of monoclonal antibodies to isolate granular and macula densa cells, and the growth of these cells in culture will provide an important model system with which to investigate stimulus-secretion coupling, cyclic nucleotide metabolism, and receptor modulation and thereby advance our understanding of the intrinsic renal regulation of hemodynamics and renin release.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
5R01HL035731-02
Application #
3349942
Study Section
(SRC)
Project Start
1985-09-30
Project End
1988-09-29
Budget Start
1986-09-30
Budget End
1987-09-29
Support Year
2
Fiscal Year
1986
Total Cost
Indirect Cost

  Institution

Name
Michigan State University
Department
Type
Schools of Medicine
DUNS #
193247145
City
East Lansing
State
MI
Country
United States
Zip Code
48824

  Publications

Burnatowska-Hledin, M A; Spielman, W S (1991) Effects of adenosine on cAMP production and cytosolic Ca2+ in cultured rabbit medullary thick limb cells. Am J Physiol 260:C143-50
Spielman, W S; Arend, L J (1991) Adenosine receptors and signaling in the kidney. Hypertension 17:117-30
Smith, W L; Sonnenburg, W K; Allen, M L et al. (1989) The biosynthesis and actions of prostaglandins in the renal collecting tubule and thick ascending limb. Adv Exp Med Biol 259:131-47
Arend, L J; Handler, J S; Rhim, J S et al. (1989) Adenosine-sensitive phosphoinositide turnover in a newly established renal cell line. Am J Physiol 256:F1067-74
Burnatowska-Hledin, M A; Spielman, W S (1989) Vasopressin V1 receptors on the principal cells of the rabbit cortical collecting tubule. Stimulation of cytosolic free calcium and inositol phosphate production via coupling to a pertussis toxin substrate. J Clin Invest 83:84-9
Allen, M L; Nakao, A; Sonnenburg, W K et al. (1988) Immunodissection of cortical and medullary thick ascending limb cells from rabbit kidney. Am J Physiol 255:F704-10
Burnatowska-Hledin, M A; Spielman, W S (1988) Immunodissection of mitochondria-rich cells from rabbit outer medullary collecting tubule. Am J Physiol 254:F907-11
Arend, L J; Burnatowska-Hledin, M A; Spielman, W S (1988) Adenosine receptor-mediated calcium mobilization in cortical collecting tubule cells. Am J Physiol 255:C581-8
Arend, L J; Bakris, G L; Burnett Jr, J C et al. (1987) Role for intrarenal adenosine in the renal hemodynamic response to contrast media. J Lab Clin Med 110:406-11
Burnatowska-Hledin, M A; Spielman, W S (1987) Vasopressin increases cytosolic free calcium in LLC-PK1 cells through a V1-receptor. Am J Physiol 253:F328-32

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