Expression of GnTIII in a recombinant anti‐CD20 CHO production cell line: Expression of antibodies with altered glycoforms leads to an increase in ADCC through higher affinity for FCγRIII

Davies, Julian; Jiang, Liying; Pan, Li-Zhen; LaBarre, Michael J.; Anderson, Darrell R.; Reff, Mitchell E.

doi:10.1002/bit.1119

Cited by 303 publications

(178 citation statements)

References 15 publications

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“…Similarly, glycosylation pathway engineering has been developed to improve the biological function and reduce the heterogenecity of therapeutic antibodies (23,24). Of these methods, the most practical way to acquire homogeneous glycoproteins is based on the strategy of glycoprotein remodeling, a strategy first reported in 1997…”

mentioning

confidence: 99%

A common glycan structure on immunoglobulin G for enhancement of effector functions

Lin

Tsai²,

et al. 2015

Proc. Natl. Acad. Sci. U.S.A.

186

178

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Antibodies have been developed as therapeutic agents for the treatment of cancer, infection, and inflammation. In addition to binding activity toward the target, antibodies also exhibit effector-mediated activities through the interaction of the Fc glycan and the Fc receptors on immune cells. To identify the optimal glycan structures for individual antibodies with desired activity, we have developed an effective method to modify the Fc-glycan structures to a homogeneous glycoform. In this study, it was found that the biantennary N-glycan structure with two terminal alpha-2,6-linked sialic acids is a common and optimized structure for the enhancement of antibody-dependent cell-mediated cytotoxicity, complement-dependent cytotoxicity, and antiinflammatory activities.endoglycosidase | Fc glycosylation | glycoengineered antibodies | homogeneous antibodies | sugar oxazoline

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mentioning

confidence: 99%

A common glycan structure on immunoglobulin G for enhancement of effector functions

Lin

Tsai²,

et al. 2015

Proc. Natl. Acad. Sci. U.S.A.

186

178

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“…Cell engineering of glycosylation patterns (Davies et al 2001;Natsume et al 2006;Shields et al 2002;Shinkawa et al 2003;Umañ a et al 1999;Warner 1999;Weikert et al 1999) and in vitro glycosylation (Butler 2005;Raju et al 2001) has provided new possibilities for biopharmaceutical design and optimization thus lowering immunogenicity effects, increasing stability and enhancing functional activity. Weikert et al (1999) engineered CHO cells that secreted either tissue necrosis factor receptor-IgG1 fusion protein (TNFR-IgG) or tissue plasminogen activator (TNK-tPA) to over-express a2,3-sialyltransferase and the resultant glycoproteins had a considerable longer pharmacokinetic mean residence time in rabbit models.…”

Section: Glycosylation Engineeringmentioning

confidence: 99%

“…Bisected oligosaccharides have been implicated in enhanced antibody dependant cellular cytotoxicity (ADCC) activity. When CHO cells were engineered to over express b1,4 N-acetyl glucosaminoyltransferase (GnTIII), the bisected oligosaccharide glycoforms, ADCC activity was increased 20-100 fold (Davies et al 2001;Umañ a et al 1999). A silencing approach has also been used in CHO cells to increase the antibody effector function of ADCC by introducing siRNA targeting a1,6 fucosyltransferase (FUT8) mRNA (Mori et al 2004).…”

Section: Glycosylation Engineeringmentioning

confidence: 99%

Using cell engineering and omic tools for the improvement of cell culture processes

et al. 2007

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Significant strides have been made in mammalian cell based biopharmaceutical process and cell line development over the past years. With several established mammalian host cell lines and expression systems, optimization of selection systems to reduce development times and improvement of glycosylation patterns are only some of the advances being made to improve cell culture processes. In this article, the advances pertaining to cell line development and cell engineering strategies are discussed. An overview of the cell engineering strategies to enhance cellular characteristics by genetic manipulation are illustrated, focusing on the use of genomics and proteomics tools and their application in such endeavors. Included in this review are some of the early studies using the 'omic' technique to understand cellular mechanisms of product synthesis and secretion, apoptosis, cell proliferation and the influence of the physicochemical environment. The article highlights the significance of integrating genomics and proteomics data with the vast amounts of bioprocess data for improved analysis of the biological pathways involved. Further improvements of the techniques and methodologies used are needed but ultimately, the new cell engineering strategies should provide great insight into the regulatory networks within the cell in a bioprocess environment and how to manipulate them to increase overall productivity.

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“…The contents of the dead and lysed cells are released to the cell culture supernatant, leading to contamination of the product. Most of the presently popular mammalian producer cell lines have been optimized with respect to technological requirements by adaptation and maintenance for extended periods of time under the appropriate culture conditions, while adaptation of the cellular physiology by genetic engineering is still in its infancy (Grabenhorst et al 1995;Monaco et al 1996;Irani et al 1999Irani et al , 2002Uman˜a et al 1999;Davies et al 2001;Fogolin et al 2004; for a review see Grabenhorst et al 1999). However, due to comparatively high costs and low productivities of cultured mammalian cells, there is a constant pressure to further improve the producer cell lines as well as the protein production processes.…”

Section: Introductionmentioning

confidence: 99%

Application of a Reversible Immortalization System for the Generation of Proliferation-Controlled Cell Lines

et al. 2004

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To employ physiological mechanisms to control cell growth primary cells were reversibly immortalized using the SV40 TAg. The cells showed a fibroblast-like morphology. When the expression of the TAg was turned off, the cells arrested in the G0/G1 cell cycle phase. The cell culture could be kept for over 1 week in the proliferation-controlled state while the growth arrest remained fully reversible. The regulation was highly efficacious in that the arrested cell population did not spontaneously resume growth, suggesting that in the absence of the immortalizing gene expression endogenous growth-control mechanisms can keep these cells in a viable state for a prolonged time. Recombinant protein expression increased in growth-controlled cells when compared to conventionally cultured cells. Analysis of a secreted pharmaceutical protein revealed high product integrity without any signs of degradation. Therefore, it is feasible to apply genetic regulation of cell immortalization to obtain proliferation-controlled cell lines and this technique may be of interest to generate novel biotechnological producer cells.Abbreviations: DMEM -Dulbecco's modified Eagle's medium; Dox -doxycycline; eGFP -enhanced green fluorescent protein; EPO -recombinant human erythropoietin; FCS -fetal calf serum; IRES -internal ribosomal binding site; LTR -long terminal repeat; MEF -murine embryonic fibroblast cell; neoNeomycin phosphotransferase; TAg -SV40 virus large T-antigen; w.t. -wild type

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Expression of GnTIII in a recombinant anti‐CD20 CHO production cell line: Expression of antibodies with altered glycoforms leads to an increase in ADCC through higher affinity for FCγRIII

Cited by 303 publications

References 15 publications

A common glycan structure on immunoglobulin G for enhancement of effector functions

A common glycan structure on immunoglobulin G for enhancement of effector functions

Using cell engineering and omic tools for the improvement of cell culture processes

Application of a Reversible Immortalization System for the Generation of Proliferation-Controlled Cell Lines

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