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B3(Fab)-streptavidin Tetramer Has Higher Binding Avidity than B3(scFv)-streptavidin Tetramer

Authors
Won, Jae SeonKang, Hye WonNam, Pil WonChoe, Mu Hyeon
Issue Date
20-5월-2009
Publisher
WILEY-V C H VERLAG GMBH
Keywords
Recombinant antibody; Refolding; Fab; Homo-tetramer; Antibody therapy
Citation
BULLETIN OF THE KOREAN CHEMICAL SOCIETY, v.30, no.5, pp.1101 - 1106
Indexed
SCIE
SCOPUS
KCI
Journal Title
BULLETIN OF THE KOREAN CHEMICAL SOCIETY
Volume
30
Number
5
Start Page
1101
End Page
1106
URI
https://scholar.korea.ac.kr/handle/2021.sw.korea/120037
ISSN
0253-2964
Abstract
Multivalent and multi-specific antibodies can provide valuable tools for bio-medical research, diagnosis and therapy. In antigen-anti body interactions, the avidity of anti bodies depends on the affinity and the number of binding sites. As artificial multivalent antibody agents, single chain Fv-streptavidin fusion tetramer proteins (scFv-SA)(4) have been previously tested.(1,2) Although, the Fab domain is known to be more stable than scFv in animal models, (3,4) it has never been used to make a multivalent agent with a streptavidin fusion. In this study, we prepared tetra-valent (Fab-cSA)(4) by fusing Fab with core streptavidin (cSA). This molecule was made using inclusion body production, refolding and chromatography purification. Affinities of the Fab-cSA tetramer and a scFv-cSA tetramer to a cell surface antigen were compared by ELISA using biotin-HRP. The Fab-cSA tetramer showed higher binding avidity than the scFv-cSA tetramer. The higher binding avidity of the Fab-cSA tetramer demonstrates its potential as a therapeutic agent for target-specific antibody therapy.
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