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The structural basis for the functional comparability of factor VIII and the long‐acting variant recombinant factor VIII Fc fusion protein
Author(s) -
Leksa N. C.,
Chiu P.L.,
BouAssaf G. M.,
Quan C.,
Liu Z.,
Goodman A. B.,
Chambers M. G.,
Tsutakawa S. E.,
Hammel M.,
Peters R. T.,
Walz T.,
Kulman J. D.
Publication year - 2017
Publication title -
journal of thrombosis and haemostasis
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.947
H-Index - 178
eISSN - 1538-7836
pISSN - 1538-7933
DOI - 10.1111/jth.13700
Subject(s) - fusion protein , recombinant dna , domain (mathematical analysis) , chemistry , c terminus , crystallography , mathematics , biochemistry , amino acid , gene , mathematical analysis
Essentials Recombinant factor VIII (rFVIII) Fc fusion protein has a 1.5‐fold longer half‐life than rFVIII. Five orthogonal methods were used to characterize the structure of rFVIIIFc compared to rFVIII. The C‐terminal Fc fusion does not perturb the structure of FVIII in rFVIIIFc. The FVIII and Fc components of rFVIIIFc are flexibly tethered and functionally independent.Summary Background Fusion of the human IgG 1 Fc domain to the C‐terminal C2 domain of B‐domain‐deleted ( BDD ) factor VIII (FVIII) results in the recombinant FVIII F c (r FVIIIF c) fusion protein, which has a 1.5‐fold longer half‐life in humans. Objective To assess the structural properties of r FVIIIF c by comparing its constituent FVIII and Fc elements with their respective isolated components, and evaluating their structural independence within r FVIIIF c. Methods r FVIIIF c and its isolated FVIII and Fc components were compared by the use of hydrogen–deuterium exchange mass spectrometry ( HDX ‐ MS ). The structure of r FVIIIF c was also evaluated by the use of X‐ray crystallography, small‐angle X‐ray scattering ( SAXS ), and electron microscopy ( EM ). The degree of steric interference by the appended Fc domain was assessed by EM and surface plasmon resonance ( SPR ). Results HDX ‐ MS analysis of r FVIIIF c revealed that fusion caused no structural perturbations in FVIII or Fc. The r FVIIIF c crystal structure showed that the FVIII component is indistinguishable from published BDD FVIII structures. The Fc domain was not observed, indicating high mobility. SAXS analysis was consistent with an ensemble of rigid‐body models in which the Fc domain exists in a largely extended orientation relative to FVIII . Binding of Fab fragments of anti‐C2 domain antibodies to BDD FVIII was visualized by EM , and the affinities of the corresponding intact antibodies for BDD FVIII and r FVIIIF c were comparable by SPR analysis. Conclusions The FVIII and Fc components of r FVIIIF c are structurally indistinguishable from their isolated constituents, and show a high degree of structural independence, consistent with the functional comparability of r FVIIIF c and unmodified FVIII.