Abstract

The prevention of thrombosis is an important function of the endothelium in vivo and the maintenance of endothelial integrity is a presumed function of the heparin-binding fibroblast growth factors (HBGFs). Previous efforts from this laboratory have defined the identity, function and structure of HBGF-1, an angiogenic prototype of the HBGF family and have also elucidated similar structure-function relationships for the HBGF-1 receptor. A unique feature of the HBGF prototypes is the lack of a signal sequence for secretion and while the prior application involved studies directed toward the function of HBGF-1 receptor, this feature has led this laboratory to question whether HBGF-1 can function as an intracellular polypeptide. Indeed, recent evidence from this laboratory suggests that HBGF-1 and its structural homolog IL-1alpha can function as intracellular regulators of cell division in vitro and HBGF-1 may utilize nuclear translocation as a component of its ability to induce cell proliferation. Thus, a specific aim of this competitive renewal application is to define the minimum structure for nuclear localization in order to understand how HBGF-1 is partitioned between cytosol and the nucleus. The identification of domains within the structure of HBGF-1 and the elucidation of the structure of putative intracellular binding proteins that may participate in the partitioning of HBGF-1 between cytosol and nucleus are among these goals. These studies will employ mutagenesis of the nuclear translocation sequence and HBGF-1 ligand affinity cloning. Conventional cloning strategies are also discussed and will employ ligand affinity chromatography for the purification of cytosol- and nuclei-derived polypeptides that are able to associate with HBGF-1. Likewise, HBGF-1 is also able to associate with DNA, is phosphorylated on serine residues and is able to form stable homo and heterodimers, and while it is not known whether these interactions are indeed significant, we propose that they are interesting, reproducible and worthy of further study. Thus, another specific aim of this application is to define whether the interaction between HBGF-1 and DNA involves specific nucleotide sequences, possibly mediate through unknown cytosolic or nuclear polypeptides, or whether this association involves the ability of HBGF-1 to recognize the phosphodiester backbone. If the latter interaction is accurate, we propose to take advantage of the non-specific interaction between HBGF-1 and DNA for the delivery of IL-1alpha antisense oligomers during adjuvant-induced inflammation in the rat. If successful, this approach may enable us to study, define and regulate angiogenic phenomena during experimental solid tumor growth, atherogenesis, rheumatoid arthritis and other pathophysiologic situations in vivo.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
5R01HL032348-12
Application #
2217012
Study Section
Pathology A Study Section (PTHA)
Project Start
1987-01-01
Project End
1997-03-31
Budget Start
1995-04-01
Budget End
1996-03-31
Support Year
12
Fiscal Year
1995
Total Cost
Indirect Cost

  Institution

Name
American National Red Cross
Department
Type
DUNS #
003255213
City
Washington
State
DC
Country
United States
Zip Code
20006

  Publications

Kacer, Doreen; McIntire, Christian; Kirov, Alek et al. (2011) Regulation of non-classical FGF1 release and FGF-dependent cell transformation by CBF1-mediated notch signaling. J Cell Physiol 226:3064-75
Graziani, Irene; Doyle, Andrew; Sterling, Sarah et al. (2009) Protein folding does not prevent the nonclassical export of FGF1 and S100A13. Biochem Biophys Res Commun 381:350-4
Lee, Connie W; Raskett, Christopher M; Prudovsky, Igor et al. (2008) Molecular dependence of estrogen receptor-negative breast cancer on a notch-survivin signaling axis. Cancer Res 68:5273-81
Duarte, Maria; Kolev, Vihren; Kacer, Doreen et al. (2008) Novel cross-talk between three cardiovascular regulators: thrombin cleavage fragment of Jagged1 induces fibroblast growth factor 1 expression and release. Mol Biol Cell 19:4863-74
Di Serio, Claudia; Doria, Laura; Pellerito, Silvia et al. (2008) The release of fibroblast growth factor-1 from melanoma cells requires copper ions and is mediated by phosphatidylinositol 3-kinase/Akt intracellular signaling pathway. Cancer Lett 267:67-74
Prudovsky, Igor; Tarantini, Francesca; Landriscina, Matteo et al. (2008) Secretion without Golgi. J Cell Biochem 103:1327-43
Kathir, Karuppanan Muthusamy; Ibrahim, Khalil; Rajalingam, Dakshinamurthy et al. (2007) S100A13-lipid interactions-role in the non-classical release of the acidic fibroblast growth factor. Biochim Biophys Acta 1768:3080-9
Nikopoulos, George N; Duarte, Maria; Kubu, Chris J et al. (2007) Soluble Jagged1 attenuates lateral inhibition, allowing for the clonal expansion of neural crest stem cells. Stem Cells 25:3133-42
Di Serio, Claudia; Pellerito, Silvia; Duarte, Maria et al. (2007) Protease-activated receptor 1-selective antagonist SCH79797 inhibits cell proliferation and induces apoptosis by a protease-activated receptor 1-independent mechanism. Basic Clin Pharmacol Toxicol 101:63-9
Soldi, Raffaella; Mandinova, Anna; Venkataraman, Krishnan et al. (2007) Sphingosine kinase 1 is a critical component of the copper-dependent FGF1 export pathway. Exp Cell Res 313:3308-18

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