Biochemical characterization of the active heterodimer form of human heparanase (Hpa1) protein expressed in insect cells.

2.50
Hdl Handle:
http://hdl.handle.net/10541/82300
Title:
Biochemical characterization of the active heterodimer form of human heparanase (Hpa1) protein expressed in insect cells.
Authors:
McKenzie, Edward; Young, Kathryn; Hircock, Margaret; Bennett, James; Bhaman, Maina; Felix, Robert; Turner, Paul; Stamps, Alasdair; McMillan, David; Saville, Giles; Ng, Stanley; Mason, Sean; Snell, Daniel; Schofield, Darren; Gong, Haiping; Townsend, Reid; Gallagher, John T; Page, Martin; Parekh, Raj; Stubberfield, Colin
Abstract:
The mammalian endoglycosidase heparanase (Hpa1) is primarily responsible for cleaving heparan sulphate proteoglycans (HSPGs) present on the basement membrane of cells and its potential for remodelling the extracellular matrix (ECM) could be important in embryonic development and tumour metastasis. Elevated expression of this enzyme has been implicated in various pathological processes including tumour cell proliferation, metastasis, inflammation and angiogenesis. The enzyme therefore represents a potential therapeutic target. Hpa1 protein is initially synthesized as an inactive 65 kDa proenzyme that is then believed to be subsequently activated by proteolytic cleavage to generate an active heterodimer of 8 and 50 kDa polypeptides. By analysis of a series of Hpa1 deletion proteins we confirm that the 8 kDa subunit is essential for enzyme activity. We present here for the first time an insect cell expression system used for the generation of large amounts of recombinant protein of high specific activity. Individual subunits were cloned into baculoviral secretory vectors and co-expressed in insect cells. Active secreted heterodimer protein was recovered from the medium and isolated by a one-step heparin-Sepharose chromatography procedure to give protein of >90% purity. The recombinant enzyme behaved similarly to the native protein with respect to the size of HS fragments liberated on digestion, substrate cleavage specificity and its preference for acidic pH. A significant amount of activity, however, was also detectable at physiological pH values, as measured both by an in vitro assay and by in vivo degradation of cell-bound heparan sulphate.
Affiliation:
Oxford GlycoSciences (OGS), 10 The Quadrant, Abingdon Science Park, Abingdon, Oxon OX14 3YS, UK.
Citation:
Biochemical characterization of the active heterodimer form of human heparanase (Hpa1) protein expressed in insect cells. 2003, 373 (Pt 2):423-35 Biochem. J.
Journal:
The Biochemical Journal
Issue Date:
15-Jul-2003
URI:
http://hdl.handle.net/10541/82300
DOI:
10.1042/BJ20030318
PubMed ID:
12713442
Type:
Article
Language:
en
ISSN:
0264-6021
Appears in Collections:
All Paterson Institute for Cancer Research

Full metadata record

DC FieldValue Language
dc.contributor.authorMcKenzie, Edward-
dc.contributor.authorYoung, Kathryn-
dc.contributor.authorHircock, Margaret-
dc.contributor.authorBennett, James-
dc.contributor.authorBhaman, Maina-
dc.contributor.authorFelix, Robert-
dc.contributor.authorTurner, Paul-
dc.contributor.authorStamps, Alasdair-
dc.contributor.authorMcMillan, David-
dc.contributor.authorSaville, Giles-
dc.contributor.authorNg, Stanley-
dc.contributor.authorMason, Sean-
dc.contributor.authorSnell, Daniel-
dc.contributor.authorSchofield, Darren-
dc.contributor.authorGong, Haiping-
dc.contributor.authorTownsend, Reid-
dc.contributor.authorGallagher, John T-
dc.contributor.authorPage, Martin-
dc.contributor.authorParekh, Raj-
dc.contributor.authorStubberfield, Colin-
dc.date.accessioned2009-09-23T11:59:17Z-
dc.date.available2009-09-23T11:59:17Z-
dc.date.issued2003-07-15-
dc.identifier.citationBiochemical characterization of the active heterodimer form of human heparanase (Hpa1) protein expressed in insect cells. 2003, 373 (Pt 2):423-35 Biochem. J.en
dc.identifier.issn0264-6021-
dc.identifier.pmid12713442-
dc.identifier.doi10.1042/BJ20030318-
dc.identifier.urihttp://hdl.handle.net/10541/82300-
dc.description.abstractThe mammalian endoglycosidase heparanase (Hpa1) is primarily responsible for cleaving heparan sulphate proteoglycans (HSPGs) present on the basement membrane of cells and its potential for remodelling the extracellular matrix (ECM) could be important in embryonic development and tumour metastasis. Elevated expression of this enzyme has been implicated in various pathological processes including tumour cell proliferation, metastasis, inflammation and angiogenesis. The enzyme therefore represents a potential therapeutic target. Hpa1 protein is initially synthesized as an inactive 65 kDa proenzyme that is then believed to be subsequently activated by proteolytic cleavage to generate an active heterodimer of 8 and 50 kDa polypeptides. By analysis of a series of Hpa1 deletion proteins we confirm that the 8 kDa subunit is essential for enzyme activity. We present here for the first time an insect cell expression system used for the generation of large amounts of recombinant protein of high specific activity. Individual subunits were cloned into baculoviral secretory vectors and co-expressed in insect cells. Active secreted heterodimer protein was recovered from the medium and isolated by a one-step heparin-Sepharose chromatography procedure to give protein of >90% purity. The recombinant enzyme behaved similarly to the native protein with respect to the size of HS fragments liberated on digestion, substrate cleavage specificity and its preference for acidic pH. A significant amount of activity, however, was also detectable at physiological pH values, as measured both by an in vitro assay and by in vivo degradation of cell-bound heparan sulphate.en
dc.language.isoenen
dc.subjectCultured Tumour Cellsen
dc.subject.meshAmidohydrolases-
dc.subject.meshAnimals-
dc.subject.meshBaculoviridae-
dc.subject.meshBlood Platelets-
dc.subject.meshChromatography, Affinity-
dc.subject.meshDimerization-
dc.subject.meshFibrinolytic Agents-
dc.subject.meshGene Expression Regulation, Enzymologic-
dc.subject.meshGenetic Vectors-
dc.subject.meshGlucuronidase-
dc.subject.meshHeparin-
dc.subject.meshHeparitin Sulfate-
dc.subject.meshHumans-
dc.subject.meshImmunoenzyme Techniques-
dc.subject.meshMass Spectrometry-
dc.subject.meshMutagenesis, Site-Directed-
dc.subject.meshPeptide-N4-(N-acetyl-beta-glucosaminyl) Asparagine Amidase-
dc.subject.meshRecombinant Proteins-
dc.subject.meshSequence Deletion-
dc.subject.meshSpodoptera-
dc.subject.meshTumor Cells, Cultured-
dc.titleBiochemical characterization of the active heterodimer form of human heparanase (Hpa1) protein expressed in insect cells.en
dc.typeArticleen
dc.contributor.departmentOxford GlycoSciences (OGS), 10 The Quadrant, Abingdon Science Park, Abingdon, Oxon OX14 3YS, UK.en
dc.identifier.journalThe Biochemical Journalen

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