Identification of Porcine Coagulation Factor VIII Domains Responsible for High Level Expression via Enhanced Secretion

Doering, Christopher B.; Healey, John F.; Parker, Ernest T.; Barrow, Rachel T.; Lollar, Pete

doi:10.1074/jbc.m312451200

Cited by 61 publications

(95 citation statements)

References 39 publications

(41 reference statements)

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“…1) in the mammalian expression vector ReNeo has been described previously (27,28). These constructs contain nucleotide sequence between the A2 and ap-A3 domains encoding a linker region of human or porcine origin that includes the Arg-His-Gln-Arg recognition sequence for PACE/furin processing (29,30).…”

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confidence: 99%

A1 Subunit-mediated Regulation of Thrombin-activated Factor VIII A2 Subunit Dissociation

Parker

Doering

Lollar

2006

Journal of Biological Chemistry

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Factor VIII (fVIII) is the plasma protein that is missing or deficient in hemophilia A. In contrast, elevated levels of fVIII are associated with an increased risk of arterial and venous thrombosis. fVIII is activated by thrombin to form a non-covalently linked A1/A2/A3-C1-C2 heterotrimer. At physiological concentrations, fVIIIa decays as a result of A2 subunit dissociation, which may help regulate the balance between hemostasis and thrombosis. A2 subunit dissociation is faster in human fVIIIa than in porcine fVIIIa, which may represent an evolutionary adaptation associated with the development of the upright posture and venous stasis in the lower extremities. To investigate the basis for the different decay kinetics of human and porcine fVIIIa, hybrid fVIII molecules representing all possible combinations of human and porcine A domains were isolated. The kinetics of fVIIIa decay were measured and fit to a model describing a reversible bimolecular reaction in which the dissociation rate constant, k, and dissociation constant, K d , were the fitted parameters. Substitution of the porcine A1 domain into human fVIIIa produced a dissociation rate constant indistinguishable from porcine fVIIIa. Subsequently, substitution of the second cupredoxin-like A1 subdomain resulted in a dissociation rate constant similar to porcine fVIIIa, whereas substitution of the first cupredoxin-like A1 subdomain resulted in a dissociation rate constant intermediate between human and porcine fVIIIa. We propose that cupredoxin-like A1 subdomains in fVIII contain inter-species differences that are a result of selective pressure on the dissociation rate constant.Factor VIII (fVIII) 2 contains internal homology that defines a sequence of domains designated A1-A2-B-ap-A3-C1-C2 (1). The B domain undergoes limited intracellular proteolysis at several sites prior to secretion of fVIII into the circulation. As a result, a series of 160 -300-kDa heterodimers are produced that contain a common ap-A3-C1-C2 light chain and A1-A2-B heavy chains in which the amount of B domain is variable. The B domain can be deleted with little or no change in the function of fVIII. fVIII circulates non-covalently bound to von Willebrand factor (vWf) and is proteolytically activated by thrombin, which catalyzes cleavages at Arg 372 between the A1 and A2 domains, at Arg 740 between the A2 and B domains, and at Arg 1689 between the ap and A3 domains (2). The product, fVIIIa, is a 160-kDa A1/A2/A3-C1-C2 heterotrimer whose subunits are held together non-covalently (3-5).fVIIIa functions in blood coagulation as a cofactor for factor IXa during the proteolytic activation of factor X on the phospholipid surface of platelets and monocytes. Cleavage at Arg 372 activates the factor IXa cofactor function of fVIIIa, as judged by naturally occurring mutations at this site that result in hemophilia A (6, 7) and by site-directed mutagenesis of this site, which produces loss of function (8). Cleavage at Arg 740 releases the B domain. However, removal of the B domain does not activate ...

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A1 Subunit-mediated Regulation of Thrombin-activated Factor VIII A2 Subunit Dissociation

Parker

Doering

Lollar

2006

Journal of Biological Chemistry

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“…9 For many secreted proteins, transit from the endoplasmic reticulum to the Golgi apparatus is rate limiting and the primary determinants of this limitation are believed to be specific amino acid sequences within the molecule itself. 10,11 Using this knowledge, we and others have focused on the development of biobetter FVIII molecules and their implementation into gene transfer vectors that can be used in stem cell gene therapy applications. For example, it was shown by Kaufman et al that coexpression of von Willebrand factor results in the improved accumulation of recombinant FVIII in the culture medium of heterologous cells.…”

Section: Origins and Limitations Of Fviii And Fix Biosynthesismentioning

confidence: 99%

“…For example, we and others have shown that BDD p-FVIII is expressed at 10-fold or greater levels compared with BDD h-FVIII. 11,15,16 This led to the rationale of using a recombinant murine stem cell (␥-retrovirus) viral vector encoding BDD p-FVIII in HSCT gene therapy studies. These studies were highly successful with respect to the plasma FVIII activity levels achieved in transplanted hemophilia A mice conditioned with lethal or sublethal irradiation-based conditioning.…”

Section: Multipotent Adult Stem Cell Therapies: Hscsmentioning

confidence: 99%

“…This bioengineered FVIII transgene demonstrated equivalent transgene product expression to BDD p-FVIII in vitro and in vivo using both SIV-and HIV-based expression vectors. 11,17,18 An alternative, but also successful, preclinical HSCT gene therapy strategy incorporating nonengineered BDD h-FVIII, and more recently FIX, transgenes involves specific targeting of transgene expression to the megakaryocyte/platelet hematopoietic lineage. This approach was first demonstrated by Poncz et al using transplantation of HSCs from transgenic mice to correct the hemophilia A bleeding phenotype.…”

Section: Multipotent Adult Stem Cell Therapies: Hscsmentioning

confidence: 99%

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Replacing bad (F)actors: hemophilia

Doering

Spencer

2014

Hematology

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Hemophilia A and B are bleeding disorders that result from functional deficiencies in specific circulating blood clotting factors termed factor VIII (FVIII) and factor IX (FIX), respectively, and collectively display an incidence of 1 in 4000 male births. Stem cell transplantation therapies hold the promise of providing a cure for hemophilia, but currently available transplantable stem cell products do not confer endogenous FIX or FVIII biosynthesis. Learning Objective• To gain an understanding of the key issues surrounding the implementation of stem cell therapies for hemophilia

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“…Further study using porcine/human hybrids has localized certain protein sequences within porcine FVIII that confer this advantage, although additional studies will be necessary to characterize the mechanism. 10 Bioengineering rFVIII for high-efficiency production could potentially reduce costs and increase the availability of concentrates for therapy.…”

Section: Improved Production Efficiencymentioning

confidence: 99%

Hemophilia: New Protein Therapeutics

Pipe

2010

Hematology

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Therapeutic advances for patients with hemophilia have resulted in reduced mortality, improved joint outcomes, safety from blood-transmitted pathogens, improved quality of life, and a normalized life span in the developed world. The production of recombinant coagulation factors has increased the worldwide capacity for replacement therapy and facilitated aggressive prophylactic therapy. However, this has come at significant cost, and barriers remain to broad application of prophylaxis. Recombinant DNA technology remains a promising platform to develop novel hemophilia therapeutics with improved functional properties to try to overcome some of these remaining barriers. Bioengineering strategies have produced novel therapeutics with increased production efficiency, increased potency and resistance to inactivation, prolonged plasma half-lives, and reduced immunogenicity. Alternative nonbiologic therapies may lead to new treatment paradigms. The current pipeline of new technologies and products is promising and growing with several agents already advancing from preclinical to clinical trials.

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Identification of Porcine Coagulation Factor VIII Domains Responsible for High Level Expression via Enhanced Secretion

Cited by 61 publications

References 39 publications

A1 Subunit-mediated Regulation of Thrombin-activated Factor VIII A2 Subunit Dissociation

A1 Subunit-mediated Regulation of Thrombin-activated Factor VIII A2 Subunit Dissociation

Replacing bad (F)actors: hemophilia

Hemophilia: New Protein Therapeutics

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