AI Article Synopsis

  • Human FcγRI is a high-affinity receptor for IgG, featuring three extracellular domains, including a unique third domain (D3) that differs from low-affinity receptors.
  • This study explored how D3 impacts the binding ability between rhFcγRI and human IgG, finding that the first two domains (D1D2) alone can bind similarly to human IgG subclasses.
  • Surface plasmon resonance analysis revealed that while D1D2 binds strongly to IgG, it dissociates faster than the full rhFcγRI, suggesting that D3 plays a role in stabilizing the receptor-IgG interaction rather than directly influencing binding specificity.

Article Abstract

Human FcγRI is a high affinity receptor for the Fc portion of human immunoglobulin G (IgG), and has extracellular, transmembrane and cytoplasmic regions. The extracellular region of human FcγRI, which is the part that interacts with human IgG, is comprised of three immunoglobulin-like domains. Unlike low affinity Fcγ receptors (FcγRII and FcγRIII), FcγRI has a unique third extracellular domain (D3). This study investigated the contribution of D3 to the binding between recombinant human FcγRI (rhFcγRI) and human IgG. The three extracellular domains and the first and second extracellular domains of human FcγRI were expressed by Escherichia coli as rhFcγRI and rhFcγRI-D1D2, respectively. The binding specificity of rhFcγRI-D1D2 to human IgG subclasses was the same as that of rhFcγRI. From surface plasmon resonance analysis, the binding affinity of rhFcγRI-D1D2 for human IgG1/κ was high (the equilibrium dissociation constant: KD=8.04 × 10(-10)M), but slightly lower than that of rhFcγRI (KD=2.59 × 10(-10)M). While the association of rhFcγRI-D1D2 with human IgG1/κ was same as that of rhFcγRI, the dissociation of rhFcγRI-D1D2 was faster than that of rhFcγRI. From these results, D3 of rhFcγRI would not contribute directly to the binding specificity and association of rhFcγRI, but to the holding bound human IgG.

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http://dx.doi.org/10.1016/j.molimm.2013.01.007DOI Listing

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