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Chemical and Structural Analysis of an Antibody Folding Intermediate Trapped during Glycan Biosynthesis

by: Thomas A. Bowden, Kavitha Baruah, Charlotte H. Coles, David J. Harvey, Xiaojie Yu, Byeong-Doo Song, David I. Stuart, A. Radu Aricescu, Christopher N. Scanlan, E. Yvonne Jones, Max Crispin
J. Am. Chem. Soc. In Journal of the American Chemical Society, Vol. 134, No. 42. (1 October 2012), pp. 17554-17563, doi:10.1021/ja306068g  Key: citeulike:11570243

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Abstract

Human IgG Fc glycosylation modulates immunological effector functions such as antibody-dependent cellular cytotoxicity and phagocytosis. Engineering of Fc glycans therefore enables fine-tuning of the therapeutic properties of monoclonal antibodies. The N-linked glycans of Fc are typically complex-type, forming a network of noncovalent interactions along the protein surface of the C?2 domain. Here, we manipulate the mammalian glycan-processing pathway to trap IgG1 Fc at sequential stages of maturation, from oligomannose- to hybrid- to complex-type glycans, and show that the Fc is structurally stabilized following the transition of glycans from their hybrid- to complex-type state. X-ray crystallographic analysis of this hybrid-type intermediate reveals that N-linked glycans undergo conformational changes upon maturation, including a flip within the trimannosyl core. Our crystal structure of this intermediate reveals a molecular basis for antibody biogenesis and provides a template for the structure-guided engineering of the protein?glycan interface of therapeutic antibodies.


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