Factor VIII Lacking the C2 Domain Retains Cofactor Activity in Vitro

Wakabayashi, Hironao; Griffiths, Amy E.; Fay, Philip J.

doi:10.1074/jbc.m110.106906

Cited by 28 publications

(39 citation statements)

References 32 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…6, B and D, and 7B), suggesting that membrane binding cannot be fully mediated by the C2 domain alone under these conditions of limiting PS exposure. This supports the view that both C domains support membrane interaction in a cooperative manner (15) and is also compatible with the finding that a FVIII deletion mutant lacking the C2 domain still displays substantial FVIII cofactor activity (37).…”

Section: Discussionsupporting

confidence: 78%

Factor VIII C1 Domain Spikes 2092–2093 and 2158–2159 Comprise Regions That Modulate Cofactor Function and Cellular Uptake

Bloem

Biggelaar

Wroblewska

et al. 2013

Journal of Biological Chemistry

View full text Add to dashboard Cite

Background: Antibody KM33 blocks factor VIII (FVIII) endocytosis and phospholipid binding. Results: Hydrogen-deuterium exchange mass spectrometry reveals that KM33 binds C1 domain spikes 2092-2093 and 2158 -2159. Glycosylated FVIII-R2159N shows reduced endocytosis and decreased binding to phospholipid membranes with low phosphatidylserine content. Conclusion: Spikes 2092-2093 and 2158 -2159 modulate FVIII endocytosis and phospholipid binding. Significance: Novel insight is obtained about the role of the C1 domain for FVIII biology. The C1 domain of factor VIII (FVIII) has been implicated in binding to multiple constituents, including phospholipids, vonWillebrand factor, and low-density lipoprotein receptor-related protein (LRP). We have previously described a human monoclonal antibody called KM33 that blocks these interactions as well as cellular uptake by LRP-expressing cells. To unambiguously identify the apparent "hot spot" on FVIII to which this antibody binds, we have employed hydrogen-deuterium exchange mass spectrometry. The results showed that KM33 protects FVIII regions 2091-2104 and 2157-2162 from hydrogen-deuterium exchange. These comprise the two C1 domain spikes 2092-2093 and 2158 -2159. Spike 2092-2093 has been demonstrated recently to contribute to assembly with lipid membranes with low phosphatidylserine (PS) content. Therefore, spike 2158 -2159 might serve a similar role. This was assessed by replacement of Arg-2159 for Asn, which introduces a motif for N-linked glycosylation. Binding studies revealed that the purified, glycosylated R2159N variant had lost its interaction with antibody KM33 but retained substantial binding to von Willebrand factor and LRP. Cellular uptake of the R2159N variant was reduced both by LRP-expressing U87-MG cells and by human monocytederived dendritic cells. FVIII activity was virtually normal on membranes containing 15% PS but reduced at low PS content. These findings suggest that the C1 domain spikes 2092-2093 and 2158 -2159 together modulate FVIII membrane assembly by a subtle, PS-dependent mechanism. These findings contribute evidence in favor of an increasingly important role of the C1 domain in FVIII biology.Activated coagulation factor VIII (FVIIIa) is a cofactor that assembles with activated factor IX (FIXa) 3 on lipid membranes that expose phosphatidylserine (PS) in the outer leaflet (1). This complex effectively generates activated factor X, ultimately leading to blood clot formation at sites of vascular injury. Current treatment of hemophilia A patients, who lack functional factor VIII (FVIII), involves intravenous infusion with either recombinant or plasma-derived FVIII (2). This treatment is, however, limited by the particularly effective clearance of FVIII from the circulation. Moreover, about 20% of patients develop antibodies against FVIII (3). The molecular determinants that drive the assembly of FVIII with membranes, including those of cells involved in clearance and immune response, remain incompletely understood.FVIII is a multidomain protein that ...

show abstract

Section: Discussionsupporting

confidence: 78%

Factor VIII C1 Domain Spikes 2092–2093 and 2158–2159 Comprise Regions That Modulate Cofactor Function and Cellular Uptake

Bloem

Biggelaar

Wroblewska

et al. 2013

Journal of Biological Chemistry

View full text Add to dashboard Cite

show abstract

“…As a rule, missense mutations cause CRM-positive haemophilia A with varying severity, depending on the mutation in question and the parts of the gene it affects. Recently, Wakabayashi et al demonstrated that Factor VIII devoid of its C2 domain remains functional, at least in vitro, but is less stable (Wakabayashi et al, 2010). In our practice, we have had two (related) patients with exon 24 missense mutation (the C2 domain) and with mild haemophilia A (40 %), supporting the notion of decreased stability of the protein.…”

Section: Point Mutationssupporting

confidence: 52%

From Genotype to Phenotype - When the Parents Ask the Question

Petkova¹,

Chakarov²,

Ganev³

2012

Hemophilia

View full text Add to dashboard Cite

“…The positioning of the C1 domain relative to the C2 domain supports previous data indicating that the C1 domain contributes to membrane association and the C2 domain is not essential for function. [29][30][31] Lastly, the x-ray crystal structure of the C2 domain/3E6/G99 complex is remarkably similar to the previously modeled ternary complex from low-resolution SAXS data ( Figure 1B). 41 These structural findings suggest that using rapid, low-resolution techniques such as SAXS may be effective tools for characterizing other antibody epitopes for fVIII inhibitor antibodies as well as other antigen/antibody interactions.…”

mentioning

confidence: 54%

“…[26][27][28] Recent studies also suggest that the C1 domain contributes to binding both VWF and PS, 29,30 and deletion studies of the C2 domain indicate that it is not essential for PL membrane binding, factor IXa binding, or clotting activity. 31 The C2 domain of fVIII is a major antigenic determinant for recognition by inhibitor antibodies. 32,33 Initial mechanistic investigations of anti-C2 inhibitor antibodies suggested that these antibodies There is an Inside Blood commentary on this article in this issue.…”

Section: Introductionmentioning

confidence: 99%