Temperature Effect on IgE Binding to CD23 Versus FcεRI

Chen, Bing‐Hung; Kilmon, Michelle A.; Ma, Check; Caven, Timothy H.; Chan‐Li, Yee; Shelburne, Anne E.; Tombes, Robert M.; Roush, Eric D.; Conrad, Daniel H.

doi:10.4049/jimmunol.170.4.1839

Cited by 13 publications

(12 citation statements)

References 38 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…Thus, only the upper portion of the stalk separates at 37°C, and the lower region of the stalk, near the transmembrane domain, remains tightly associated at all times. Note that these data also fit well with our recent finding that IgE and CD23 interact better at 4 than 37°C and confirm the increased instability of CD23 at physiological temperatures (44). Association of the trimers of CD23 was further investigated using FRET.…”

Section: Discussionsupporting

confidence: 88%

CD23 Trimers Are Preassociated on the Cell Surface Even in the Absence of Its Ligand, IgE

Kilmon

Shelburne

Chan‐Li

et al. 2004

The Journal of Immunology

Self Cite

View full text Add to dashboard Cite

Allergic disease is mediated by high levels of allergen-specific IgE. IgE binding to CD23, the low affinity receptor for IgE, results in a negative feedback signal leading to a decrease in IgE production. Previous studies have shown that CD23 associates as an oligomer and that cooperative binding of at least two lectin domains is required for high affinity IgE binding to CD23. We have previously shown that cooperative binding is required for regulation of IgE production. This study describes the production of several mAbs that bind the stalk region of murine CD23. One of the Abs, 19G5, inhibited the IgE/CD23 interaction at 37°C, but not at 4°C. Analysis of the binding properties of these Abs revealed that CD23 dissociates at high temperatures, such as 37°C; however, the N terminus is constitutively associated, indicating partial, rather than complete, dissociation. A novel finding was that the stalk region, previously thought to mediate trimer association, was not required for oligomerization. These data reveal important information about the structure of CD23 that may be useful in modulating IgE production.

show abstract

Section: Discussionsupporting

confidence: 88%

CD23 Trimers Are Preassociated on the Cell Surface Even in the Absence of Its Ligand, IgE

Kilmon

Shelburne

Chan‐Li

et al. 2004

The Journal of Immunology

Self Cite

View full text Add to dashboard Cite

show abstract

“…In support of this notion, stabilizing the trimeric form of soluble CD23 through a leucine zipper motif linked to the N-terminus of the receptor (lz-CD23) allows for enhanced detection of sialylated IgG binding in a solid-phase ELISA format at physiological temperature relative to the extracellular region of CD23 alone (Fig. S5), as has been reported for IgE (26). However, in contrast to IgE, binding of sialylated IgG to trimeric CD23 is not enhanced at 4°C.…”

Section: Resultsmentioning

confidence: 73%

General mechanism for modulating immunoglobulin effector function

Sondermann¹,

Pincetic

Maamary

et al. 2013

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

204

202

View full text Add to dashboard Cite

Immunoglobulins recognize and clear microbial pathogens and toxins through the coupling of variable region specificity to Fc-triggered cellular activation. These proinflammatory activities are regulated, thus avoiding the pathogenic sequelae of uncontrolled inflammation by modulating the composition of the Fc-linked glycan. Upon sialylation, the affinities for Fcγ receptors are reduced, whereas those for alternative cellular receptors, such as dendritic cellspecific intercellular adhesion molecule-3-grabbing nonintegrin (DC-SIGN)/CD23, are increased. We demonstrate that sialylation induces significant structural alterations in the Cγ2 domain and propose a model that explains the observed changes in ligand specificity and biological activity. By analogy to related complexes formed by IgE and its evolutionarily related Fc receptors, we conclude that this mechanism is general for the modulation of antibody-triggered immune responses, characterized by a shift between an "open" activating conformation and a "closed" antiinflammatory state of antibody Fc fragments. This common mechanism has been targeted by pathogens to avoid host defense and offers targets for therapeutic intervention in allergic and autoimmune disorders.conformational change | sialylated IgG Fc I gG and IgE mediate their proinflammatory properties through the crosslinking of the 1:1 complex of the Fc receptor (FcR) monomer in the Fc dimer cleft (1, 2). By contrast, both IgG and IgE can engage a second class of receptors, the evolutionarily related, C-type lectins dendritic cell-specific intercellular adhesion molecule-3-grabbing nonintegrin (DC-SIGN) (3) and CD23 (4), respectively, resulting in anti-inflammatory and immunosuppressive responses (5, 6). The structural basis for the ability of IgE to interact either with one or the other of these two disparate classes of receptors has recently been defined (7). The intrinsic flexibility of the IgE Ce3 domain results in both open and closed conformations of the IgE Fc, resulting in the binding of either FceRI or CD23, respectively. Binding of either receptor induces an allosteric change in the IgE Fc to the alternative conformation, thus precluding the interaction with the other receptor (7). Binding of IgE to the type II, C-type lectin CD23 is neither carbohydrate-nor calcium-dependent, mediated exclusively through protein-protein interactions, generating a 2:1 complex of CD23 with the Ce3-Ce4 interface (7). DC-SIGN is a structurally homologous, calcium-dependent, carbohydratebinding, type II lectin, tightly linked to CD23 on chromosome 19 (8), displaying ligand specificity for mannose-containing glycoconjugates and fucose-containing Lewis antigens. Binding of DC-SIGN to IgG requires that the complex, biantennary glycan, attached to the evolutionarily conserved glycosylation site Asn-297 and enclosed within the cavity formed by the Cγ2 domains of the A and B chains of the Fc dimer, be processed to the α2,6 sialylated form (9, 10). Importantly, no evidence has been found for DC-SIGN binding to sialylate...

show abstract

“…Clearly this is not, as previously thought, due to overlapping binding sites, but to an allosteric linkage between the two distant sites. The idea that the open and closed conformations might interact differently with FcεRI and CD23 was in fact anticipated by Conrad et al (24) after their surprising discovery that CD23 bound more strongly to IgE at 4°C than 37°C, whereas the opposite was true for FcεRI. They hypothesized that a change in the relative proportion of these open and closed conformational states might account for this temperature effect, and it will certainly be revealing to explore further the temperature dependence of the kinetics and thermodynamics of these receptor interactions as well as the conformational dynamics of the IgE molecule, particularly with respect to the Cε3 domains.…”

Section: Discussionmentioning

confidence: 94%

“…The fact that sCD23 can compete with FcεRI binding, albeit at high concentrations (23), was thought to be due to overlap of the two receptor binding sites. This competition was observed at considerably lower concentrations of a trimeric sCD23 molecule, presumably owing to the avidity effect (10,11), and subsequently an intriguing effect of temperature upon the relative affinities of IgE for FcεRI and CD23 was discovered (24). We now report the crystal structure of the complex between the head domain of CD23 [termed derCD23 because it corresponds to the sCD23 fragment generated by the house dust mite allergenic protease Der p 1 (25)] and Fcε3-4.…”

mentioning

confidence: 99%

Crystal structure of IgE bound to its B-cell receptor CD23 reveals a mechanism of reciprocal allosteric inhibition with high affinity receptor FcεRI

Dhaliwal

Yuan

Pang

et al. 2012

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

136

View full text Add to dashboard Cite

The role of IgE in allergic disease mechanisms is performed principally through its interactions with two receptors, FcεRI on mast cells and basophils, and CD23 (FcεRII) on B cells. The former mediates allergic hypersensitivity, the latter regulates IgE levels, and both receptors, also expressed on antigen-presenting cells, contribute to allergen uptake and presentation to the immune system. We have solved the crystal structure of the soluble lectin-like "head" domain of CD23 (derCD23) bound to a subfragment of IgE-Fc consisting of the dimer of Cε3 and Cε4 domains (Fcε3-4). One CD23 head binds to each heavy chain at the interface between the two domains, explaining the known 2:1 stoichiometry and suggesting mechanisms for crosslinking membrane-bound trimeric CD23 by IgE, or membrane IgE by soluble trimeric forms of CD23, both of which may contribute to the regulation of IgE synthesis by B cells. The two symmetrically located binding sites are distant from the single FcεRI binding site, which lies at the opposite ends of the Cε3 domains. Structural comparisons with both free IgE-Fc and its FcεRI complex reveal not only that the conformational changes in IgE-Fc required for CD23 binding are incompatible with FcεRI binding, but also that the converse is true. The two binding sites are allosterically linked. We demonstrate experimentally the reciprocal inhibition of CD23 and FcεRI binding in solution and suggest that the mutual exclusion of receptor binding allows IgE to function independently through its two receptors.antibody-receptor interactions | X-ray crystallography

show abstract

Temperature Effect on IgE Binding to CD23 Versus FcεRI

Cited by 13 publications

References 38 publications

CD23 Trimers Are Preassociated on the Cell Surface Even in the Absence of Its Ligand, IgE

CD23 Trimers Are Preassociated on the Cell Surface Even in the Absence of Its Ligand, IgE

General mechanism for modulating immunoglobulin effector function

Crystal structure of IgE bound to its B-cell receptor CD23 reveals a mechanism of reciprocal allosteric inhibition with high affinity receptor FcεRI

Contact Info

Product

Resources

About