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纯化纤维素【荐】.pdf
Biotechnol. Appl. Biochem. (2000) 31, 197–203 (Printed in Great Britain) 197
Expression, purification and applications of staphylococcal
Protein A fused to cellulose-binding domain
Etai Shpigel*, Arie Goldlust, Adi Eshel, Idit Kaplan Ber*, Gilat Efroni, Yossi Singer,
Ilan Levy*, Mara Dekel* and Oded Shoseyov*1
*The Kennedy Leigh Centre for Horticulture Research and The Otto Warburg Center for Agricultural Biotechnology,
The Faculty of Agricultural, Food and Environmental Quality Sciences, The Hebrew University of Jerusalem, P.O. Box 12,
Rehovot 76100, Israel, and CBD-Technologies Ltd., Park Tamar, P.O. Box 199, Rehovot 76100, Israel
Because staphylococcal Protein A (ProtA) binds Efficient immobilization of ProtA is required for most of
specifically to IgG, it has been used for many immuno- these applications, and various methods of immobilization
logical manipulations, most notably antibody puri- have been developed in recent years. Most of them require
fication and diagnostics. Immobilization is required for chemical modifications of the matrix. These modifications,
most of these applications. Here we describe a genetic- leading to covalent bonding of the ligand to the matrix, result
engineering approach to immobilizing ProtA on cellu- in many cases in loss of activity of the ligand as well as the
lose, by fusing it to cellulose-binding domain (CBD) inclusion of toxic organic compounds that must be removed
derived from the cellulose-binding Protein A of Clos- before use. A genetic engineering approach has been used to
tridium cellulovorans. The bifunctional fusion protein overcome some of these problems by fusing different affinity
was expressed in Escherichia coli, recovered o
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