Show simple item record

dc.contributor.authorClamp, Andrew R
dc.contributor.authorBlackhall, Fiona H
dc.contributor.authorHenrioud, Audrey
dc.contributor.authorJayson, Gordon C
dc.contributor.authorJavaherian, Kashi
dc.contributor.authorEsko, Jeffrey D
dc.contributor.authorGallagher, John T
dc.contributor.authorMerry, Catherine L R
dc.date.accessioned2009-07-07T12:06:22Z
dc.date.available2009-07-07T12:06:22Z
dc.date.issued2006-05-26
dc.identifier.citationThe morphogenic properties of oligomeric endostatin are dependent on cell surface heparan sulfate. 2006, 281 (21):14813-22 J. Biol. Chem.en
dc.identifier.issn0021-9258
dc.identifier.pmid16481316
dc.identifier.doi10.1074/jbc.M512400200
dc.identifier.urihttp://hdl.handle.net/10541/72752
dc.description.abstractEndostatin has attracted considerable attention because of its ability to inhibit angiogenesis. This property of monomeric endostatin contrasts with that of the trimeric endostatin moiety generated from the intact C-terminal domain of collagen XVIII that induces a promigratory phenotype in endothelial cells. This activity is inhibited by monomeric endostatin. In this study we demonstrate that the effect of oligomeric endostatin can also be inhibited by exogenous glycosaminoglycans in a size-dependent manner, with heparin oligosaccharides containing more than 20 monosaccharide residues having optimal inhibitory activity. Oligomeric endostatin was also found to induce morphological changes in Chinese hamster ovary cells, an epithelial cell line. This novel observation allowed the utilization of a panel of Chinese hamster ovary cell mutants with defined glycosaminoglycan biosynthetic defects. The action of oligomeric endostatin on these cells was shown to be dependent on cell surface glycosaminoglycans, principally heparan sulfate with N- and 6-O-sulfation of glucosamine residues rather than iduronate 2-O-sulfation being important for bioactivity. The responsiveness of a cell line (pgsE-606) with globally reduced heparan sulfate sulfation and shortened S domains, however, indicates that overall heparan sulfate domain patterning is the key determinant of the bioactivity of oligomeric endostatin. Purified heparin-monomeric endostatin constructs generated by zero-length cross-linking techniques were found to be unable to inhibit the action of oligomeric endostatin. This indicates a mechanism for the perturbation of oligomeric endostatin action by its monomeric counterpart via competition for glycosaminoglycan attachment sites at the cell surface.
dc.language.isoenen
dc.subject.meshAnimals
dc.subject.meshAorta
dc.subject.meshCHO Cells
dc.subject.meshCattle
dc.subject.meshCell Membrane
dc.subject.meshCollagen
dc.subject.meshCricetinae
dc.subject.meshEndostatins
dc.subject.meshGlucosamine
dc.subject.meshGlycosaminoglycans
dc.subject.meshHeparin
dc.subject.meshHeparitin Sulfate
dc.subject.meshIduronic Acid
dc.subject.meshProtein Structure, Tertiary
dc.titleThe morphogenic properties of oligomeric endostatin are dependent on cell surface heparan sulfate.en
dc.typeArticleen
dc.contributor.departmentDepartment of Medical Oncology, Cancer Research UK and the University of Manchester, Christie Hospital NHS Trust, Manchester M20 4BX, United Kingdom.en
dc.identifier.journalThe Journal of Biological Chemistryen
html.description.abstractEndostatin has attracted considerable attention because of its ability to inhibit angiogenesis. This property of monomeric endostatin contrasts with that of the trimeric endostatin moiety generated from the intact C-terminal domain of collagen XVIII that induces a promigratory phenotype in endothelial cells. This activity is inhibited by monomeric endostatin. In this study we demonstrate that the effect of oligomeric endostatin can also be inhibited by exogenous glycosaminoglycans in a size-dependent manner, with heparin oligosaccharides containing more than 20 monosaccharide residues having optimal inhibitory activity. Oligomeric endostatin was also found to induce morphological changes in Chinese hamster ovary cells, an epithelial cell line. This novel observation allowed the utilization of a panel of Chinese hamster ovary cell mutants with defined glycosaminoglycan biosynthetic defects. The action of oligomeric endostatin on these cells was shown to be dependent on cell surface glycosaminoglycans, principally heparan sulfate with N- and 6-O-sulfation of glucosamine residues rather than iduronate 2-O-sulfation being important for bioactivity. The responsiveness of a cell line (pgsE-606) with globally reduced heparan sulfate sulfation and shortened S domains, however, indicates that overall heparan sulfate domain patterning is the key determinant of the bioactivity of oligomeric endostatin. Purified heparin-monomeric endostatin constructs generated by zero-length cross-linking techniques were found to be unable to inhibit the action of oligomeric endostatin. This indicates a mechanism for the perturbation of oligomeric endostatin action by its monomeric counterpart via competition for glycosaminoglycan attachment sites at the cell surface.


This item appears in the following Collection(s)

Show simple item record