Abstract

Arginine vasopressin (AVP) hormone has a broad range of effects on mammalian tissues and is a major hormone regulating water and solute reabsorption. AVP also regulates blood pressure, acts as a mitogenic agent, and regulates a variety of biochemical and physiological functions in the brain. These actions of AVP appear to involve two well-characterized receptors, V1 and V2, that have recently been cloned and shown to belong to a superfamily of receptors characterized by the presence of seven highly conserved transmembrane regions, and to be regulated by """"""""G-proteins"""""""". Although there is no direct evidence for additional AVP receptors, several studies support this possibility. The investigators have recently identified and cloned, from rabbit kidney, what appears to be a new AVP binding protein which mediates AVP-activated cytosolic free calcium (Ca2+) mobilization (VACM-1 protein). VACM-1 shows no homology with the two known AVP receptors, or any other protein sequence presently stored in the DATABASES, and thus may represent a novel family of G-protein linked receptors. Present work is directed at characterizing VACM-1. The proposed studies will further characterize VACM-1 and are intended to help to understand the molecular mechanism of AVP action. Specifically, they may explain """"""""anomalies"""""""" in AVP actions in tissues where the presence of either V1 and V2 receptors cannot fully explain the action of AVP. Ultimately, a better understanding of AVP action at the molecular level may help in the development of specific drugs for the treatment of water imbalance and regulation of blood pressure disorders. As a consequence, the present experimental plan proposes to: 1) determine the second messenger system that couples to VACM-1 and to determine which G- protein(s) are involved in this coupling that leads to increases in the cytosolic free calcium concentration; 2) use site-directed mutagenesis and antibody probes to elucidate the structure-function characteristics of VACM-1. Specifically, the investigators will determine the glycosylation sites that may be important in the activity of VACM-1 and identify domains involved in ligand binding and in the interaction with G-proteins; and 3) examine whether VACM-1 is expressed in certain tissues where it may be involved in specific AVP-regulated biochemical and physiological responses.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK)
Type
Research Project (R01)
Project #
5R01DK047199-02
Application #
2146543
Study Section
General Medicine B Study Section (GMB)
Project Start
1994-07-01
Project End
1998-06-30
Budget Start
1995-07-01
Budget End
1996-06-30
Support Year
2
Fiscal Year
1995
Total Cost
Indirect Cost

  Institution

Name
Hope College
Department
Biology
Type
Schools of Arts and Sciences
DUNS #
City
Holland
State
MI
Country
United States
Zip Code
49422

  Publications

Burnatowska-Hledin, Maria A; Barney, Christopher C (2014) New insights into the mechanism for VACM-1/cul5 expression in vascular tissue in vivo. Int Rev Cell Mol Biol 313:79-101
Le, Isabelle P; Schultz, Sarah; Andresen, Bradley T et al. (2012) Aquaporin-2 levels in vitro and in vivo are regulated by VACM-1, a cul 5 gene. Cell Physiol Biochem 30:1148-58
Johnson, Alyssa E; Le, Isabelle P; Andresen, Bradley T et al. (2012) VACM-1/cul5 expression in vascular tissue in vivo is induced by water deprivation and its expression in vitro regulates aquaporin-1 concentrations. Cell Tissue Res 349:527-39
Bradley, Shirley E; Johnson, Alyssa E; Le, Isabelle P et al. (2010) Phosphorylation of VACM-1/Cul5 by protein kinase A regulates its neddylation and antiproliferative effect. J Biol Chem 285:4883-95
Iqbal, Jahangir; Dai, Kezhi; Seimon, Tracie et al. (2008) IRE1beta inhibits chylomicron production by selectively degrading MTP mRNA. Cell Metab 7:445-55
Buchwalter, A; Van Dort, C; Schultz, S et al. (2008) Expression of VACM-1/cul5 mutant in endothelial cells induces MAPK phosphorylation and maspin degradation and converts cells to the angiogenic phenotype. Microvasc Res 75:155-68
Sartor, Ashleigh; Kossoris, J B; Wilcox, R et al. (2006) Truncated form of VACM-1/cul-5 with an extended 3' untranslated region stimulates cell growth via a MAPK-dependent pathway. Biochem Biophys Res Commun 343:1086-93
Burnatowska-Hledin, Maria A; Kossoris, Jennifer B; Van Dort, Christa J et al. (2004) T47D breast cancer cell growth is inhibited by expression of VACM-1, a cul-5 gene. Biochem Biophys Res Commun 319:817-25
Van Dort, C; Zhao, P; Parmelee, K et al. (2003) VACM-1, a cul-5 gene, inhibits cellular growth by a mechanism that involves MAPK and p53 signaling pathways. Am J Physiol Cell Physiol 285:C1386-96
Burnatowska-Hledin; Zeneberg, A; Roulo, A et al. (2001) Expression of VACM-1 protein in cultured rat adrenal endothelial cells is linked to the cell cycle. Endothelium 8:49-63

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