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Differential effects of FcRn antagonists on the subcellular trafficking of FcRn and albumin
Guanglong Ma, Andrew R. Crowley, Liesbeth Heyndrickx, Ilse Rogiers, Eef Parthoens, Jolien Van Santbergen, Raimund J. Ober, Vladimir Bobkov, Hans de Haard, Peter Ulrichts, Erik Hofman, Els Louagie, Bianca Balbino, E. Sally Ward
Guanglong Ma, Andrew R. Crowley, Liesbeth Heyndrickx, Ilse Rogiers, Eef Parthoens, Jolien Van Santbergen, Raimund J. Ober, Vladimir Bobkov, Hans de Haard, Peter Ulrichts, Erik Hofman, Els Louagie, Bianca Balbino, E. Sally Ward
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Research Article Immunology

Differential effects of FcRn antagonists on the subcellular trafficking of FcRn and albumin

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Abstract

The homeostasis of IgG is maintained by the neonatal Fc receptor, FcRn. Consequently, antagonism of FcRn to reduce endogenous IgG levels is an emerging strategy for treating antibody-mediated autoimmune disorders using either FcRn-specific antibodies or an engineered Fc fragment. For certain FcRn-specific antibodies, this approach has resulted in reductions in the levels of serum albumin, the other major ligand transported by FcRn. Cellular and molecular analyses of a panel of FcRn antagonists have been carried out to elucidate the mechanisms leading to their differential effects on albumin homeostasis. These analyses have identified 2 processes underlying decreases in albumin levels during FcRn blockade: increased degradation of FcRn and competition between antagonist and albumin for FcRn binding. These findings have potential implications for the design of drugs to modulate FcRn function.

Authors

Guanglong Ma, Andrew R. Crowley, Liesbeth Heyndrickx, Ilse Rogiers, Eef Parthoens, Jolien Van Santbergen, Raimund J. Ober, Vladimir Bobkov, Hans de Haard, Peter Ulrichts, Erik Hofman, Els Louagie, Bianca Balbino, E. Sally Ward

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Figure 4

Late endosomal/lysosomal trafficking analysis in HEK293-hFcRn-GFP cells.

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Late endosomal/lysosomal trafficking analysis in HEK293-hFcRn-GFP cells....
HEK293-hFcRn-GFP cells were incubated with 50 nM AF647-labeled FcRn antagonist or IgG1-WT (control) for 3 hours. Following incubation, cells were fixed and permeabilized, and detection of late endosomes/lysosomes was carried out using anti–LAMP-1 antibody followed by AF555-labeled goat anti-mouse IgG conjugate. Yellow arrowheads indicate the detection of hFcRn-GFP and AF647 antagonists in anti–LAMP-1–positive compartments. Images for the AF555 channel were adjusted for visualization. Data are representative of 2 independent experiments, each consisting of at least 2 dishes per condition, and at least 6 images for each dish. AF555, AF647, and GFP are pseudocolored red, blue, and green, respectively. Each image represents part of a single cell. Scale bars = 2 μm.

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