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Featured researches published by Edgar Ong.


Biochemistry | 1995

Solution structure of a cellulose-binding domain from Cellulomonas fimi by nuclear magnetic resonance spectroscopy.

Guang-Yi Xu; Edgar Ong; Neil R. Gilkes; Douglas G. Kilburn; D. R. Muhandiram; Marees Harris-Brandts; Jeremy P. Carver; Lewis E. Kay; Timothy S. Harvey

Multidimensional, multinuclear nuclear magnetic resonance spectroscopy combined with dynamical simulated annealing has been used to determine the structure of a 110 amino acid cellulose-binding domain (CBD) from Cex, a beta-1,4-glycanase from the bacterium Cellulomonas fimi (CBDcex). An experimental data set comprising 1795 interproton NOE-derived restraints, 50 phi, 34 chi 1, and 106 hydrogen bond restraints was used to calculate 20 final structures. The calculated structures have an average root-mean-square (rms) deviation about the mean structure of 0.41 A for backbone atoms and 0.67 A for all heavy atoms when fitted over the secondary structural elements. Chromatography, ultracentrifugation, and 15N NMR relaxation experiments demonstrate that CBDcex is a dimer in solution. While attempts to measure NOEs across the dimer interface were unsuccessful, a computational strategy was employed to generate dimer structures consistent with the derived data set. The results from the dimer calculations indicate that, while the monomer topologies produced in the context of the dimer can be variable, the relative positioning of secondary structural elements and side chains present in the monomer are restored upon dimer formation. CBDcex forms an extensive beta-sheet structure with a beta-barrel fold. Titration with cellohexaose, [beta-D-glucopyranosyl-(1,4)]5-D-glucose, establishes that Trp 54 and 72 participate in cellulose binding. Analysis of the structure shows that these residues are adjacent in space and exposed to solvent. Together with other proximate hydrophilic residues, these residues form a carbohydrate-binding cleft, which appears to be a feature common to all CBDs of the same family.


Trends in Biotechnology | 1989

The cellulose-binding domains of cellulases: tools for biotechnology

Edgar Ong; Jeffrey M. Greenwood; Neil R. Gilkes; Douglas G. Kilburn; Robert C. Miller; R. Anthony J. Warren

Abstract Some cellulases comprise discrete catalytic domains and cellulose-binding domains (CBDs). The CBDs retain their cellulose-binding properties when fused to heterologous proteins. They can be used as affinity tags for protein purification, and for enzyme immobilization.


Enzyme and Microbial Technology | 1991

Enzyme immobilization using a cellulose-binding domain: Properties of a β-glucosidase fusion protein

Edgar Ong; Neil R. Gilkes; Robert C. Miller; R. Antony; J. Warren; Douglas G. Kilburn

Using molecular genetic techniques, a fusion protein has been produced which contains the cellulose-binding domain (CBD) of an exoglucanase (Cex) from Cellulomonas fimi fused to a beta-glucosidase (Abg) from Agrobacterium sp. The CBD functions as an affinity tag for the simultaneous purification and immobilization of the enzyme on cellulose. Binding to cellulose was stable for prolonged periods at temperatures from 4 degrees C to at least 50 degrees C, at ionic strengths from 10 mM to greater than 1 M, and at pH values below 8. The fusion protein can be desorbed from cellulose with distilled water or at pH greater than 8. Immobilized enzyme columns of the fusion protein bound to cotton fibers exhibited stable beta-glucosidase activity for at least 10 days of continuous operation at temperatures up to 37 degrees C. At higher temperatures, the bound enzyme lost activity. The thermal stability of the fusion protein was greatly improved by immobilization. Immobilization did not alter the pH stability. Except for its ability to bind to cellulose, the properties of the fusion protein were virtually the same as those of the native enzyme.


Proceedings of the National Academy of Sciences of the United States of America | 1996

Binding of the cellulose-binding domain of exoglucanase Cex from Cellulomonas fimi to insoluble microcrystalline cellulose is entropically driven

A L Creagh; Edgar Ong; Eric Jervis; Douglas G. Kilburn; Charles A. Haynes


Nature Biotechnology | 1989

Enzyme immobilization using the cellulose-binding domain of a Cellulomonas fimi exoglucanase

Edgar Ong; Neil R. Gilkes; R. Antony J. Warren; Robert C. Miller; Douglas G. Kilburn


Biotechnology and Bioengineering | 1993

The cellulose-binding domain (CBDCex) of an exoglucanase from Cellulomonas fimi: Production in Escherichia coli and characterization of the polypeptide

Edgar Ong; Neil R. Gilkes; Robert C. Miller; R. Antony J. Warren; Douglas G. Kilburn


Gene | 1997

Cloning and sequence analysis of two laccase complementary DNAs from the ligninolytic basidiomycete Trametes versicolor

Edgar Ong; W.Brent R Pollock; Michael Smith


Protein Engineering | 1992

Cellulose-binding domains : potential for purification of complex proteins

M.Jeffrey Greenwood; Edgar Ong; R.Neil Gilkes; R. Antony J. Warren; Robert C. Miller; G.Douglas Kilburn


Journal of Bacteriology | 1994

Streptomyces lividans glycosylates the linker region of a beta-1,4-glycanase from Cellulomonas fimi.

Edgar Ong; Douglas G. Kilburn; Robert C. Miller; R. A. J. Warren


Fems Microbiology Letters | 1994

Non-S-layer glycoproteins in eubacteria

L.E. Sandercock; A.M. MacLeod; Edgar Ong; R. A. J. Warren

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Douglas G. Kilburn

University of British Columbia

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Robert C. Miller

University of British Columbia

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Neil R. Gilkes

University of British Columbia

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R. A. J. Warren

University of British Columbia

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Jeffrey M. Greenwood

University of British Columbia

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R. Antony J. Warren

University of British Columbia

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A.M. MacLeod

University of British Columbia

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Antony J. Warren

University of British Columbia

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Charles A. Haynes

University of British Columbia

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