| Literature DB >> 28528777 |
Elisabeth Lobner1, Anne-Sophie Humm2, Kathrin Göritzer1, Georg Mlynek3, Martin G Puchinger3, Christoph Hasenhindl1, Florian Rüker4, Michael W Traxlmayr1, Kristina Djinović-Carugo5, Christian Obinger6.
Abstract
The crystallizable fragment (Fc) of the immunoglobulin class G (IgG) is an attractive scaffold for the design of novel therapeutics. Upon engineering the C-terminal loops in the CH3 domains, Fcabs (Fc domain with antigen-binding sites) can be designed. We present the first crystal structures of Fcabs, i.e., of the HER2-binding clone H10-03-6 having the AB and EF loop engineered and the stabilized version STAB19 derived by directed evolution. Comparison with the crystal structure of the Fc wild-type protein reveals conservation of the overall domain structures but significant differences in EF-loop conformations. Furthermore, we present the first Fcab-antigen complex structures demonstrating the interaction between the engineered Fcab loops with domain IV of HER2. The crystal structures of the STAB19-HER2 and H10-03-6-HER2 complexes together with analyses by isothermal titration calorimetry, SEC-MALS, and fluorescence correlation spectroscopy show that one homodimeric Fcab binds two HER2 molecules following a negative cooperative binding behavior.Entities:
Keywords: ErbB2; Fcab; Fcab-HER2 structure; HER2; IgG1-Fc; X-ray crystallography; binding stoichiometry; fluorescence correlation spectroscopy
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Year: 2017 PMID: 28528777 DOI: 10.1016/j.str.2017.04.014
Source DB: PubMed Journal: Structure ISSN: 0969-2126 Impact factor: 5.006