| Literature DB >> 26718855 |
Stian Foss1, Algirdas Grevys1, Kine Marita Knudsen Sand1, Malin Bern1, Pat Blundell2, Terje E Michaelsen3, Richard J Pleass2, Inger Sandlie1, Jan Terje Andersen4.
Abstract
Monoclonal IgG antibodies (Abs) are used extensively in the clinic to treat cancer and autoimmune diseases. In addition, therapeutic proteins are genetically fused to the constant Fc part of IgG. In both cases, the Fc secures a long serum half-life and favourable pharmacokinetics due to its pH-dependent interaction with the neonatal Fc receptor (FcRn). FcRn also mediates transport of intact IgG across polarized epithelial barriers, a pathway that is attractive for delivery of Fc-containing therapeutics. So far, no study has thoroughly compared side-by-side how IgG and different Fc-fusion formats are transported across human polarizing epithelial cells. Here, we used an in vitro cellular transport assay based on the human polarizing epithelial cell line (T84) in which both IgG1 and Fc-fusions were transported in an FcRn-dependent manner. Furthermore, we found that the efficacy of transport was dependent on the format. We demonstrate that transepithelial delivery could be enhanced by Fc-engineering for improved FcRn binding as well as by Fc-polymerization. In both cases, transport was driven by pH-dependent binding kinetics and the pH at the luminal side. Hence, efficient transcellular delivery of IgG-based drugs across human epithelial cells requires optimal pH-dependent FcRn binding that can be manipulated by avidity and Fc-engineering, factors that should inspire the design of future therapeutics targeted for transmucosal delivery.Entities:
Keywords: Epithelial; Fc-fusion; FcRn; IgG; Mucosal barrier; Transcytosis; pH-dependent binding
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Year: 2015 PMID: 26718855 DOI: 10.1016/j.jconrel.2015.12.033
Source DB: PubMed Journal: J Control Release ISSN: 0168-3659 Impact factor: 9.776