The 3.2-Å crystal structure of the human IgG1 Fc fragment–FcγRIII complex

Sondermann, Peter; Huber, Robert; Oosthuizen, Vaughan; Jacob, Uwe

doi:10.1038/35018508

Cited by 671 publications

(663 citation statements)

References 46 publications

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“…In the purified monomeric deamidated sample, reduced binding was still measured on the low‐affinity Fcγ receptors, which could only be attributed to D‐N. The main deamidation site of this IgG is present in the CDR at the LC (up to 40% modified), which is positioned relatively far away from the Fc interaction site (lower hinge, upper CH2 domain 37, 38). Deamidation at this position is not likely to change the folding of the protein in such a way that it would have a large impact on Fc receptor binding.…”

Section: Discussionmentioning

confidence: 96%

Rapid screening of IgG quality attributes – effects on Fc receptor binding

Geuijen¹,

Oppers-Tiemissen

Egging

et al. 2017

FEBS Open Bio

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The interactions of therapeutic antibodies with fragment crystallizable γ (Fcγ) receptors and neonatal Fc receptors (FcRn) are measured in vitro as indicators of antibody functional performance. Antibodies are anchored to immune cells through the Fc tail, and these interactions are important for the efficacy and safety of therapeutic antibodies. High‐throughput binding studies on each of the human Fcγ receptor classes (FcγRI, FcγRIIa, FcγRIIb, FcγRIIIa, and FcγRIIIb) as well as FcRn have been developed and performed with human IgG after stress‐induced modifications to identify potential impact in vivo. Interestingly, we found that asparagine deamidation (D‐N) reduced the binding of IgG to the low‐affinity Fcγ receptors (FcγRIIa, FcγRIIb, FcγRIIIa, and FcγRIIIb), while FcγRI and FcRn binding was not impacted. Deglycosylation completely inhibited binding to all Fcγ receptors, but showed no impact on binding to FcRn. On the other hand, afucosylation only impacted binding to FcγRIIIa and FcγRIIIb. Methionine oxidation at levels below 7%, multiple freeze/thaw cycles and short‐term thermal/shake stress did not influence binding to any of the Fc receptors. The presence of high molecular weight species, or aggregates, disturbed measurements in these binding assays; up to 5% of aggregates in IgG samples changed the binding and kinetics to each of the Fc receptors. Overall, the screening assays described in this manuscript prove that rapid and multiplexed binding assays may be a valuable tool for lead optimization, process development, in‐process controls, and biosimilarity assessment of IgGs during development and manufacturing of therapeutic IgGs.

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Section: Discussionmentioning

confidence: 96%

Rapid screening of IgG quality attributes – effects on Fc receptor binding

Geuijen¹,

Oppers-Tiemissen

Egging

et al. 2017

FEBS Open Bio

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“…The first crystal structure of FcγRIII-IgG1-Fc complex was reported in 2000 9 . The FcγRIII used in the study was a soluble FcγRIIIb (sFcγRIIIb) produced in E. coli and the Fc was isolated from pooled human IgG1.…”

Section: Molecular Mechanisms To Account For the Enhanced Affinity Ofmentioning

confidence: 99%

“…As the sFcγRIII preparation used in the study was unglycosylated, it was impossible to evaluate the impact of its N -linked glycan on the FcγRIII-Fc interaction. Nonetheless, the authors did highlight that Asn162 is a potential glycosylation site of FcγRIII that is close to a binding site and a larger carbohydrate moiety attached to this site may influence the affinity to IgG 9 . Indeed, a subsequent study revealed that, compared to the unglycosylated form of FcγRIII (by mutating Asn162 to Gln162), the glycosylated FcγRIII (Asn162) showed reduced affinity for native (fucosylated) IgG antibodies, while antibodies with or without the core fucose showed a similar affinity for unglycosylated FcγRIII 20 .…”

Section: Molecular Mechanisms To Account For the Enhanced Affinity Ofmentioning

confidence: 99%

“…demonstrated that the glycosylation at Asn162 of FcγRIII is not essential for the expression of the receptor; however, this glycosylation site is conserved among all FcγRIIIs (or the equivalent) in all mammals studied 19 . Furthermore, in all FcγRs, the regions that interact with the antibody are highly conserved, yet all other receptors lack this glycosylation site 9 . It is tempting to speculate that ADCC may be modulated by IgG core fucosylation because of the presence of the glycan at Asn162 of FcγRIII.…”

Section: Molecular Mechanisms To Account For the Enhanced Affinity Ofmentioning

confidence: 99%

“…, 9 This Fc-FcγRIII interaction is significantly affected by the glycan present at the conserved N -glycosylation site Asn297 (N297) in each of the CH2 domains 10 . Mutations in the CH2 domain that destroyed the conserved N -glycosylation motif and hence gave rise to aglycosylated Fc resulted in complete loss of binding to most FcγRs except FcγRI 11 .…”

Section: Introductionmentioning

confidence: 99%

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The “less-is-more” in therapeutic antibodies: Afucosylated anti-cancer antibodies with enhanced antibody-dependent cellular cytotoxicity

Pereira

Chan

Lin

et al. 2018

mAbs

253

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Therapeutic monoclonal antibodies are the fastest growing class of biological therapeutics for the treatment of various cancers and inflammatory disorders. In cancer immunotherapy, some IgG1 antibodies rely on the Fc-mediated immune effector function, antibody-dependent cellular cytotoxicity (ADCC), as the major mode of action to deplete tumor cells. It is well-known that this effector function is modulated by the N-linked glycosylation in the Fc region of the antibody. In particular, absence of core fucose on the Fc N-glycan has been shown to increase IgG1 Fc binding affinity to the FcγRIIIa present on immune effector cells such as natural killer cells and lead to enhanced ADCC activity. As such, various strategies have focused on producing afucosylated antibodies to improve therapeutic efficacy. This review discusses the relevance of antibody core fucosylation to ADCC, different strategies to produce afucosylated antibodies, and an update of afucosylated antibody drugs currently undergoing clinical trials as well as those that have been approved.

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Overview of Protein Structural and Functional Folds

2004

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This overview provides an illustrated, comprehensive survey of some commonly observed protein-fold families and structural motifs, chosen for their functional significance. It opens with descriptions and definitions of the various elements of protein structure and associated terminology. Following is an introduction into web-based structural bioinformatics that includes surveys of interactive web servers for protein fold or domain annotation, protein-structure databases, protein-structure-classification databases, structural alignments of proteins, and molecular graphics programs available for personal computers. The rest of the overview describes selected families of protein folds in terms of their secondary, tertiary, and quaternary structural arrangements, including ribbon-diagram examples, tables of representative structures with references, and brief explanations pointing out their respective biological and functional significance.

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The 3.2-Å crystal structure of the human IgG1 Fc fragment–FcγRIII complex

Cited by 671 publications

References 46 publications

Rapid screening of IgG quality attributes – effects on Fc receptor binding

Rapid screening of IgG quality attributes – effects on Fc receptor binding

The “less-is-more” in therapeutic antibodies: Afucosylated anti-cancer antibodies with enhanced antibody-dependent cellular cytotoxicity

Overview of Protein Structural and Functional Folds

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