Chemical modifications of heparin that diminish its anticoagulant but preserve its heparanase-inhibitory, angiostatic, anti-tumor and anti-metastatic properties

Structural features of heparin potentially important for heparanase-inhibitory activity were examined by measuring the ability of heparin derivatives to affect the degradation of [3H]acetylated heparan sulphate by tumor cell heparanases. IC50 values were determined using an assay which distinguished...

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Bibliographic Details
Published in:Glycobiology (Oxford) 1996-04, Vol.6 (3), p.355-366
Main Authors: Lapierre, France, Holme, Kevin, Lam, Lun, Tressler, Robert J., Storm, Neil, Wee, Jennifer, Stack, Robert J., Castellot, John, Tyrrell, David J.
Format: Article
Language:English
Subjects:
angiogenesis
Animals
Anticoagulants - chemistry
Anticoagulants - pharmacology
Antineoplastic Agents - chemistry
Antineoplastic Agents - pharmacology
cancer
chemically-modified heparins
Chick Embryo
Chondroitin Sulfates - pharmacology
endoglycosidase
Enzyme Inhibitors - chemistry
Enzyme Inhibitors - pharmacology
Female
Glucuronidase
Glycoside Hydrolases - antagonists & inhibitors
hepara sulphate
Heparin - analogs & derivatives
Heparin - chemistry
Heparin - pharmacology
Heparitin Sulfate - metabolism
Humans
Lung Neoplasms - secondary
Male
Melanoma, Experimental - drug therapy
Melanoma, Experimental - secondary
Mice
Mice, Inbred C57BL
Mice, Nude
Molecular Structure
Neoplasm Metastasis - prevention & control
Neoplasms, Experimental - drug therapy
Neovascularization, Physiologic - drug effects
Pancreatic Neoplasms - drug therapy
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Summary:Structural features of heparin potentially important for heparanase-inhibitory activity were examined by measuring the ability of heparin derivatives to affect the degradation of [3H]acetylated heparan sulphate by tumor cell heparanases. IC50 values were determined using an assay which distinguished degraded from undegraded substrate by precipitation of the latter with cetylpyridinium chloride (CPC). Removal of heparin's 2-O-sulphate and 3-O-sul-phate groups enhanced heparanase-inhibitory activity (50%). Removal of its carboxyl groups slightly lowered the activity (18%), while combining the treatments abolished the activity. At least one negative charge on the iduronic acid/idose moiety, therefore, is necessary for heparanase-inhibitory activity. Replacing heparin's N-sulphate groups with N-acetyl groups reduced its activity (37%). Comparing this heparin derivative with 2,3-O-de-sulphated heparin, the placement of sulphate groups appears important for activity since the two structures have similar nominal linear charge density. In addition, unsubstituted uronic acids are nonessential for inhibition since their modification (periodate-oxidation/borohydride-reduction) enhanced rather than reduced heparanase-inhibitory activity. The most effective heparanase inhibitors (2,3-O-desulphated heparin, and [periodate-oxidized, borohydride-reduced] heparin) were tested in the chick chorioallantoic membrane (CAM) bioassay for anti-angiogenic activity and found to be at least as efficacious as heparin. 2,3-O-desulphated heparin also significantly decreased the tumor growth of a subcutaneous human pancreatic (Ca-Pan-2) adenocarcinoma in nude mice and prolonged the survival times of C57BL/6N mice in a B16-F10 melanoma experimental lung metastasis assay.
ISSN:0959-6658
1460-2423
DOI:10.1093/glycob/6.3.355