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Chimeric protein for selective cell attachment onto cellulosic substrates.

作者信息

Craig Scott J, Shu Alan, Xu Yin, Foong Frances C, Nordon Robert

机构信息

Graduate School of Biomedical Engineering, University of New South Wales, Australia.

出版信息

Protein Eng Des Sel. 2007 May;20(5):235-41. doi: 10.1093/protein/gzm016. Epub 2007 Apr 12.

DOI:10.1093/protein/gzm016
PMID:17430973
Abstract

We have developed a fusion protein (CBD-LG) incorporating a cellulose-binding domain and an antibody binding domain, protein LG, to provide an adaptor molecule for cell separation with regenerated cellulose hollow fiber arrays. A single hollow fiber cell adhesion assay utilizing a CD34+ cell line, KG1a, was used to investigate whether ligand affinity interactions were strong enough for cell attachment and separation. CBD-LG efficiently captured CD34+ cells labeled with the mouse IgG2a monoclonal antibody MHCD3400. However, it was not possible to bind CD34+ cells labeled with an IgG1 antibody (HPCA-2). The low affinity of HPCA-2 for LG was overcome by secondary antibodies: KG1a cells that were dual labeled with HPCA-2 followed by rat anti-mouse IgG1 adhered inside hollow fibers coated with CBD-LG. Alternatively, immobilized rabbit polyclonal anti-mouse IgG1 captured cells labeled with HPCA-2. The development of an adaptor molecule to display recombinant domains at the surface of hollow fibers will be an effective tool to investigate cellular ligand-receptor interactions, a necessary step in the development of hollow fiber bioreactors for manufacture of human cellular products.

摘要

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