RECOMBINANT FACTOR VIII HAVING INCREASED STABILITY
The present invention relates to a recombinant factor VIII that includes one or more mutations that result in enhanced stability of both factor VIII and factor VIIIa. Methods of making and using the recombinant factor VIII, and pharmaceutical compositions containing the same are also disclosed. The present invention further relates to an isolated nucleic acid molecule that encodes the recombinant factor VIII, as well as DNA expression systems and host cells containing the isolated nucleic acid molecule.
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This application is a division of U.S. patent application Ser. No. 13/691,474, filed Nov. 30, 2012, which is a continuation of U.S. patent application Ser. No. 12/179,801, filed Jul. 25, 2008, issued as U.S. Pat. No. 8,338,571 on Dec. 25, 2012, which claims the priority benefit of U.S. Provisional Patent Application Ser. No. 60/984,518, filed Nov. 1, 2007, and U.S. Provisional Patent Application Ser. No. 60/991,304, filed Nov. 30, 2007, each of which is hereby incorporated by reference in its entirety.
This invention was made with government support under grant numbers HL 76213 and HL 38199 awarded by the National Institutes of Health. The government has certain rights in the invention.
BACKGROUND OF THE INVENTIONHemophilia A, the most common of the severe, inherited bleeding disorders, results from a deficiency or defect in the plasma protein factor VIII. There is no cure for Hemophilia A and treatment consists of replacement therapy using preparations of (purified) plasma or the recombinant protein.
Factor VIII circulates as a non-covalent, metal ion-dependent heterodimer. This procofactor form of the protein contains a heavy chain (HC) comprised of A1(a1)A2(a2)B domains and a light chain (LC) comprised of (a3)A3C1C2 domains, with the lower case a representing short (˜30-40 residue) segments rich in acidic residues (see Fay, “Activation of Factor VIII and Mechanisms of Cofactor Action,” Blood Rev. 18:1-15 (2004)). Factor VIII is activated by proteolytic cleavages at the A1A2, A2B and A3A3 junctions catalyzed by thrombin or factor Xa. The product of this reaction, factor VIIIa, is a heterotrimer comprised of subunits designated A1, A2, and A3C1C2 that functions as a cofactor for the serine protease factor IXa in the membrane-dependent conversion of zymogen factor X to the serine protease, factor Xa (see Fay, “Activation of Factor VIII and Mechanisms of Cofactor Action,” Blood Rev. 18:1-15 (2004)).
Reconstitution studies have shown that the factor VIII heterodimeric structure is supported by both electrostatic and hydrophobic interactions (Fay, “Reconstitution of Human Factor VIII from Isolated Subunits,” Arch Biochem Biophys. 262:525-531 (1988); Ansong et al., “Factor VIII A1 Domain Residues 97-105 Represent a Light Chain-interactive Site,” Biochemistry. 45:13140-13149 (2006), and the inter-chain affinity is further strengthened by factor VIII binding von Willebrand factor (Fay, “Reconstitution of Human Factor VIII from Isolated Subunits,” Arch Biochem Biophys. 262:525-531 (1988); Kaufman et al., “Regulation of Factor VIII Expression and Activity by von Willebrand Factor,” Thromb Haemost. 82:201-208 (1999)). Metal ions also contribute to the inter-chain affinity and activity parameters (Wakabayashi et al., “Metal Ion-independent Association of Factor VIII Subunits and the Roles of Calcium and Copper Ions for Cofactor Activity and Inter-subunit Affinity,” Biochemistry 40:10293-10300 (2001)). Calcium is required to yield the active factor VIII conformation. Mutagenesis studies mapped a calcium-binding site to a segment rich in acidic residues within the A1 domain (residues 110-126) and identified specific residues within this region prominent in the coordination of the ion (Wakabayashi et al., “Residues 110-126 in the A1 Domain of Factor VIII Contain a Ca2+ Binding Site Required for Cofactor Activity,” J Biol Chem. 279:12677-12684 (2004)). A recent intermediate resolution X-ray structure (Shen et al., “The Tertiary Structure and Domain Organization of Coagulation Factor VIII,” Blood 111:1240-1247 (2008)) confirmed this calcium-binding site as well as suggested a second potential site within the A2 domain. This structure also showed occupancy of the two type 1 copper ion sites within the A1 and A3 domains. Earlier functional studies have shown that copper ions facilitate the association of the heavy and light chains to form the heterodimer, increasing the inter-chain affinity by several-fold at physiologic pH (Fay et al., “Human Factor VIIIa Subunit Structure: Reconstruction of Factor VIIIa from the Isolated A1/A3-C1-C2 Dimer and A2 Subunit,” J Biol Chem. 266:8957-8962 (1991); Wakabayashi et al., “pH-dependent Association of Factor VIII Chains: Enhancement of Affinity at Physiological pH by Cu2+,” Biochim Biophys Acta. 1764:1094-1101 (2006); Ansong et al., “Factor VIII A3 Domain Residues 1954-1961 Represent an A1 Domain-Interactive Site,” Biochemistry 44:8850-8857 (2005)).
The instability of factor VIIIa results from weak electrostatic interactions between the A2 subunit and the A1/A3C1C2 dimer (Fay et al., “Human Factor VIIIa Subunit Structure: Reconstruction of Factor VIIIa from the Isolated A1/A3-C1-C2 Dimer and A2 Subunit,” J Biol Chem. 266:8957-8962 (1991); Lollar et al., “pH-dependent Denaturation of Thrombin-activated Porcine Factor VIII,” J Biol Chem. 265:1688-1692 (1990)) and leads to dampening of factor Xase activity (Lollar et al., “Coagulant Properties of Hybrid Human/Porcine Factor VIII Molecules,” J Biol Chem. 267:23652-23657 (1992); Fay et al., “Model for the Factor VIIIa-dependent Decay of the Intrinsic Factor Xase: Role of Subunit Dissociation and Factor IXa-catalyzed Proteolysis,” J Biol Chem. 271:6027-6032 (1996)). Limited information is available regarding the association of the A2 subunit in factor VIIIa, and residues in both the A1 and A3 domains appear to make contributions to the retention of this subunit. Several factor VIII point mutations have been shown to facilitate the dissociation of A2 relative to WT and these residues localize to either the A1-A2 domain interface (Pipe et al., “Mild Hemophilia A Caused by Increased Rate of Factor VIII A2 Subunit Dissociation: Evidence for Nonproteolytic Inactivation of Factor VIIIa in vivo,” Blood 93:176-183 (1999); Pipe et al., “Hemophilia A Mutations Associated with 1-stage/2-stage Activity Discrepancy Disrupt Protein-protein Interactions within the Triplicated A Domains of Thrombin-activated Factor VIIIa,” Blood 97:685-691 (2001)) or the A2-A3 domain interface (Hakeos et al., “Hemophilia A Mutations within the Factor VIII A2-A3 Subunit Interface Destabilize Factor VIIIa and Cause One-stage/Two-stage Activity Discrepancy,” Thromb Haemost. 88:781-787 (2002)). These factor VIII variants demonstrate a characteristic one-stage/two-stage assay discrepancy (Duncan et al., “Familial Discrepancy Between the One-stage and Two-stage Factor VIII Methods in a Subgroup of Patients with Haemophilia A,” Br J Haematol. 87:846-848 (1994); Rudzki et al., “Mutations in a Subgroup of Patients with Mild Haemophilia A and a Familial Discrepancy Between the One-stage and Two-stage Factor VIII:C Methods,” Br J Haematol. 94:400-406 (1996)), with significant reductions in activity values determined by the latter assay as a result of increased rates of A2 subunit dissociation.
Examination of the ceruloplasmin-based homology model for the A domains of factor VIII (Pemberton et al., “A Molecular Model for the Triplicated A Domains of Human Factor VIII Based on the Crystal Structure of Human Ceruloplasmin,” Blood 89:2413-2421 (1997)) suggests an extended interface between the A2 domain and each of the A1 and A3 domains, with multiple potential contacts contributing to binding interactions.
Significant interest exists in stabilizing factor VIIIa, since a more stable form of the protein would represent a superior therapeutic for hemophilia A, potentially requiring less material to treat the patient (Fay et al., “Mutating Factor VIII: Lessons from Structure to Function,” Blood Reviews 19:15-27 (2005)). To this end, preparations of factor VIII have been described where mutations have been made in the recombinant protein to prevent the dissociation of the A2 subunit by introducing novel covalent bonds between A2 and other factor VIII domains (Pipe et al., “Characterization of a Genetically Engineered Inactivation-resistant Coagulation Factor VIIIa,” Proc Natl Acad Sci USA 94:11851-11856 (1997); Gale et al., “An Engineered Interdomain Disulfide Bond Stabilizes Human Blood Coagulation Factor VIIIa,” J. Thromb. Haemostasis 1:1966-1971 (2003)). However, it has since been suggested that these types of mutation may not be desirable in a therapeutic factor VIII, because they substantially eliminate means for down-regulation. This situation could yield a prothrombotic condition, which may cause harm. Thus, it would be desirable to enhance the stability of both factor VIII and factor VIIIa, but in a manner that minimizes the likelihood of promoting prothrombotic conditions.
The present invention is directed to overcoming these and other deficiencies in the art.
SUMMARY OF THE INVENTIONA first aspect of the present invention relates to a recombinant factor VIII that includes one or more mutations that result in enhanced stability of both factor VIII and factor VIIIa.
Preferably, the one or more mutations constitute a replacement of one or more charged amino acid residues with a hydrophobic amino acid residue at either or both of the A1A2 or A2A3 domain interfaces. Particularly preferred recombinant factor VIII of the present invention includes a substitution of a Glu287 residue of wildtype factor VIII, a substitution of an Asp302 residue of wildtype factor VIII, a substitution of an Asp519 residue of wildtype factor VIII, a substitution of a Glu665 residue of wildtype factor VIII, a substitution of a Glu1984 residue of wildtype factor VIII, or combinations thereof.
A second aspect of the present invention relates to a pharmaceutical composition that includes the recombinant factor VIII according to the first aspect of the present invention.
A third aspect of the present invention relates to an isolated nucleic acid molecule encoding a recombinant factor VIII according to the first aspect of the present invention. Also included within this aspect of the present invention are recombinant DNA expression systems that contain a DNA molecule encoding the recombinant factor VIII of the present invention, and recombinant host cells that contain the DNA molecule and/or recombinant expression system.
A fourth aspect of the present invention relates to a method of making a recombinant factor VIII that includes: growing a host cell according to the third aspect of the present invention under conditions whereby the host cell expresses the recombinant factor VIII; and isolating the recombinant factor VIII.
A fifth aspect of the present invention relates to a method of treating an animal for hemophilia A. This method of treatment includes: administering to an animal exhibiting hemophilia A an effective amount of the recombinant factor VIII according to the first aspect of the present invention, whereby the animal exhibits effective blood clotting following vascular injury.
The present invention demonstrates that a number of charged residues at the A1A2 and A2A3 domain interfaces do not participate in hydrogen bonding, but instead may be destabilizing to factor VIII structure and/or may facilitate the dissociation of the A2 subunit following activation of the factor VIII procofactor. Replacement of these charged residues with hydrophobic residues—with the aim of increasing the buried hydrophobic area and reducing the buried hydrophilic area—was shown in the accompanying Examples to enhance inter-domain binding affinity. Stability parameters were assessed following the activity of the factor VIII variants at elevated temperature and time courses for the decay of factor VIIIa activity resulting from A2 subunit dissociation. Results from these studies demonstrated that a number of mutations yielded increased stability parameters consistent with the elimination of destabilizing forces likely due to buried charge at the A2 domain interface. These stabilized variants of factor VIII and activated cofactor VIIIa should afford an improved therapeutic for treatment of hemophilia A.
The present invention relates to a recombinant factor VIII having one or more mutations that result in enhanced stability of both factor VIII and factor VIIIa.
The recombinant factor VIII of the present invention can be prepared by modifying the amino acid sequence of a wild-type factor VIII or a mutant factor VIII that has otherwise been modified to affect other properties of the factor VIII, such as antigenicity, circulating half-life, protein secretion, affinity for factor IXa and/or factor X, altered factor VIII-inactivation cleavage sites, immunogenicity, shelf-life, etc.
Suitable wild-type factor VIII that can be modified in accordance with the present invention can be from various animals including, without limitation, mammals such as humans (see, e.g., GenBank Accession Nos. AAA52484 (amino acid) and K01740 (nucleotide); and GenBank Accession Nos. CAD97566 (amino acid) and AX746360 (nucleotide), which are hereby incorporated by reference in their entirety), rats (see, e.g., GenBank Accession Nos. AAQ21580 (amino acid) and AY362193 (nucleotide), which are hereby incorporated by reference in their entirety), mice (see, e.g., GenBank Accession Nos. AAA37385 (amino acid) and L05573 (nucleotide), which are hereby incorporated by reference in their entirety), guinea pigs, dogs (see, e.g., GenBank Accession Nos. AAB87412 (amino acid) and AF016234 (nucleotide); and GenBank Accession Nos. AAC05384 (amino acid) and AF049489 (nucleotide), which are hereby incorporated by reference in their entirety), cats, monkeys, chimpanzees (see, e.g., GenBank Accession Nos. XP—529212 (amino acid) and XM—529212 (nucleotide), which are hereby incorporated by reference in their entirety), orangutans, cows, horses, sheep, pigs (see, e.g., GenBank Accession Nos. NP—999332 (amino acid) and NM—214167 (nucleotide), which are hereby incorporated by reference in their entirety), goats, rabbits, and chickens. These and other sequences are also available electronically via the Haemophilia A Mutation, Structure, Test and Resource Site (or HAMSTeRS), which further provides an alignment of human, porcine, murine, and canine factor VIII proteins. Thus, the conservation and homology among mammalian factor VIII proteins is well known.
By way of example, the human factor VIII cDNA nucleotide and predicted amino acid sequences are shown below in SEQ ID NOs: 1 and 2, respectively. Human factor VIII is synthesized as an approximately 300 kDa single chain protein with internal sequence homology that defines the “domain” sequence NH2-A1-A2-B-A3-C1-C2-COOH. In a factor VIII molecule, a “domain,” as used herein, is a continuous sequence of amino acids that is defined by internal amino acid sequence identity and sites of proteolytic cleavage by thrombin. Unless otherwise specified, factor VIII domains include the following amino acid residues, when the sequences are aligned with the human amino acid sequence (SEQ ID NO: 2):
A1, residues Ala1-Arg372;
A2, residues Ser373-Arg740;
B, residues Ser741-Arg1648;
A3, residues Ser1690-Ile2032;
C1, residues Arg2033-Asn2172; and
C2, residues Ser2173-Tyr2332.
The A3-C1-C2 sequence includes residues Ser1690-Tyr2332. The remaining sequence, residues Glu1649-Arg1689, is usually referred to as the factor VIII light chain activation peptide. Factor VIII is proteolytically activated by thrombin or factor Xa, which dissociates it from von Willebrand factor, forming factor VIIIa, which has procoagulant function. The biological function of factor VIIIa is to increase the catalytic efficiency of factor IXa toward factor X activation by several orders of magnitude. Thrombin-activated factor VIIIa is a 160 kDa A1/A2/A3-C1-C2 heterotrimer that forms a complex with factor IXa and factor X on the surface of platelets or monocytes. A “partial domain” as used herein is a continuous sequence of amino acids forming part of a domain.
The gene encoding the wild-type human factor VIII has a nucleotide sequence of SEQ ID NO:1, as follows:
The wild-type human factor VIII encoded by SEQ ID NO:1 has an amino acid sequence of SEQ ID NO:2, as follows:
In the above sequence, several charged residues are identified by bold typeface and underlining, including Glu287, Asp302, Asp519, Glu665, and Glu1984
The recombinant factor VIII of the present invention is characterized by the replacement of one or more charged amino acid residues with a hydrophobic amino acid residue at either or both of the A1A2 or A2A3 domain interfaces. Preferably, the charged residue to be replaced is either a Glu or Asp residue that does not participate in hydrogen bonding between the A1A2 or A2A3 domains. The hydrophobic amino acid residue that replaces the charged residue can be any of Ala, Val, Ile, Leu, Met, Phe, or Trp. Particularly preferred recombinant factor VIII of the present invention includes a substitution of the Glu287 residue of wildtype factor VIII, a substitution of the Asp302 residue of wildtype factor VIII, a substitution of the Asp519 residue of wildtype factor VIII, a substitution of the Glu665 residue of wildtype factor VIII, a substitution of the Glu1984 residue of wildtype factor VIII, or combinations thereof. The D302A, E287A, E665A, E665V, D519A, D519V, E1984A, and E1984V substitutions are preferred for achieving a recombinant factor VIII that has enhanced stability of both factor VIII and factor VIIIa. Preferred combinations of these substitutions include, without limitation, D519AE665V, D519VE665V, and D519VE1984A double mutants, as well as D519AE665VE1984A and D519VE665VE1984A triple mutants. The enhanced stability of these mutants is believed to be achieved by stabilizing the inter-domain interface in factor VIII as well as reducing A2 subunit dissociation from A1/A3C1C2 as compared to wildtype factor VIIIa.
Suitable mutant factor VIII sequences that can be modified in accordance with the present invention can also include any previously known or subsequently identified mutant factor VIII sequences that have modified properties with regard to various attributes, including, without limitation, antigenicity, circulating half-life, protein secretion, affinity for factor IXa and/or factor X, altered factor VIII-inactivation cleavage sites, enhanced specific activity of factor VIIIa, immunogenicity, and shelf-life.
One example of a suitable mutant factor VIII that can be modified in accordance with the present invention is a factor VIII having a modified calcium binding site, preferably at residue 113 of SEQ ID NO: 2. This affords a factor VIIIa having enhanced specific activity. Exemplary mutants of this type are described in U.S. patent application Ser. No. 10/581,471 to Fay et al., which is hereby incorporated by reference in its entirety. Preferably, the residue 113 mutant also is modified in accordance with one or more of the mutations described above (e.g., at positions 287, 302, 519, 665, and/or 1984) to afford a high stability/high specific activity factor VIII protein. Exemplary high stability/high specific activity factor VIII proteins include, without limitation: those possessing combined E113AD519A, E113AD519V, E113AE665A, E113AE665V, or E113AE1984V substitutions.
A second example of a suitable mutant factor VIII that can be modified in accordance with the present invention is a B-domainless factor VIII that contains amino acid residues 1-740 and 1690-2332 of SEQ ID NO: 2 (see, e.g., U.S. Pat. No. 6,458,563 to Lollar, which is hereby incorporated by reference in its entirety).
In one embodiment of the B-domainless recombinant factor VIII of the present invention, the B-domain is replaced by a DNA linker segment and at least one codon is replaced with a codon encoding an amino acid residue that has the same charge as a corresponding residue of porcine factor VIII (see, e.g., U.S. Patent Application Publication No. 2004/0197875 to Hauser et al., which is hereby incorporated by reference in its entirety).
In another embodiment of the B-domainless recombinant factor VIII of the present invention, the modified mutant factor VIII is encoded by a nucleotide sequence having a truncated factor IX intron 1 inserted in one or more locations (see, e.g., U.S. Pat. No. 6,800,461 to Negrier and U.S. Pat. No. 6,780,614 to Negrier, each of which is hereby incorporated by reference in its entirety). This recombinant factor VIII can be used for yielding higher production of the recombinant factor VIII in vitro as well as in a transfer vector for gene therapy (see, e.g., U.S. Pat. No. 6,800,461 to Negrier, which is hereby incorporated by reference in its entirety). In a particular example of this embodiment, the recombinant factor VIII can be encoded by a nucleotide sequence having a truncated factor IX intron 1 inserted in two locations, and having a promoter that is suitable for driving expression in hematopoietic cell lines, and specifically in platelets (see, e.g., U.S. Pat. No. 6,780,614 to Negrier, which is hereby incorporated by reference in its entirety).
Regardless of the embodiment, the B-domainless factor VIII preferably contains one or more of the mutations described above (e.g., at positions 287, 302, 519, 665, and/or 1984). Recombinant factor VIII proteins prepared in accordance with the Examples herein are B-domainless.
A third example of a suitable mutant factor VIII that can be modified in accordance with the present invention is a chimeric human/animal factor VIII that contains one or more animal amino acid residues as substitution(s) for human amino acid residues that are responsible for the antigenicity of human factor VIII. In particular, animal (e.g., porcine) residue substitutions can include, without limitation, one or more of the following: R484A, R488G, P485A, L486S, Y487L, Y487A, S488A, S488L, R489A, R4895, R490G, L491S, P492L, P492A, K493A, G494S, V495A, K496M, H497L, L498S, K499M, D500A, F501A, P502L, 1503M, L504M, P505A, G506A, E507G, 1508M, 1508A, M2199I, F2200L, L2252F, V2223A, K2227E, and/or L2251 (U.S. Pat. No. 5,859,204 to Lollar, U.S. Pat. No. 6,770,744 to Lollar, and U.S. Patent Application Publication No. 2003/0166536 to Lollar, each of which is hereby incorporated by reference in its entirety). Preferably, the recombinant chimeric factor VIII contains one or more of the mutations described above (e.g., at positions 287, 302, 519, 665, and/or 1984).
A fourth example of a suitable mutant factor VIII that can be modified in accordance with the present invention is a factor VIII that has enhanced affinity for factor IXa (see, e.g., Fay et al., “Factor VIIIa A2 Subunit Residues 558-565 Represent a Factor IXa Interactive Site,” J. Biol. Chem. 269(32):20522-7 (1994); Bajaj et al., “Factor IXa: Factor VIIIa Interaction. Helix 330-338 of Factor IXa Interacts with Residues 558-565 and Spatially Adjacent Regions of the A2 Subunit of Factor VIIIa,” J. Biol. Chem. 276(19):16302-9 (2001); and Lenting et al., “The Sequence Glu1811-Lys1818 of Human Blood Coagulation Factor VIII Comprises a Binding Site for Activated Factor IX,” J. Biol. Chem. 271(4):1935-40 (1996), each of which is hereby incorporated by reference in its entirety) and/or factor X (see, e.g., Lapan et al., “Localization of a Factor X Interactive Site in the A1 Subunit of Factor VIIIa,” J. Biol. Chem. 272:2082-88 (1997), which is hereby incorporated by reference in its entirety). Preferably, the enhanced-affinity factor VIII contains one or more of the mutations described above (e.g., at positions 287, 302, 519, 665, and/or 1984).
A fifth example of a suitable mutant factor VIII that can be modified in accordance with the present invention is a factor VIII that is modified to enhance secretion of the factor VIII (see, e.g., Swaroop et al., “Mutagenesis of a Potential Immunoglobulin-Binding Protein-Binding Site Enhances Secretion of Coagulation Factor VIII,” J. Biol. Chem. 272(39):24121-4 (1997), which is hereby incorporated by reference in its entirety). Preferably, the secretion enhanced mutant factor VIII contains one or more of the mutations identified above (e.g., at positions 287, 302, 519, 665, and/or 1984).
A sixth example of a suitable mutant factor VIII that can be modified in accordance with the present invention is a factor VIII with an increased circulating half-life. This modification can be made using various approaches, including, without limitation, by reducing interactions with heparan sulfate (Sarafanov et al., “Cell Surface Heparan Sulfate Proteoglycans Participate in Factor VIII Catabolism Mediated by Low Density Lipoprotein Receptor-Related Protein,” J. Biol. Chem. 276(15):11970-9 (2001), which is hereby incorporated by reference in its entirety) and/or low-density lipoprotein receptor-related protein (“LRP”) (Saenko et al., “Role of the Low Density Lipoprotein-Related Protein Receptor in Mediation of Factor VIII Catabolism,” J. Biol. Chem. 274(53):37685-92 (1999); and Lenting et al., “The Light Chain of Factor VIII Comprises a Binding Site for Low Density Lipoprotein Receptor-Related Protein,” J. Biol. Chem. 274(34):23734-9 (1999), each of which is hereby incorporated by reference in its entirety). Preferably, the half-life enhanced mutant factor VIII contains one or more of the mutations described above (e.g., at positions 287, 302, 519, 665, and/or 1984).
A seventh example of a suitable mutant factor VIII that can be modified in accordance with the present invention is a modified factor VIII encoded by a nucleotide sequence modified to code for amino acids within known, existing epitopes to produce a recognition sequence for glycosylation at asparagines residues (see, e.g., U.S. Pat. No. 6,759,216 to Lollar, which is hereby incorporated by reference in its entirety). The mutant factor VIII of this example can be useful in providing a modified factor VIII that escapes detection by existing inhibitory antibodies (low antigenicity factor VIII) and which decreases the likelihood of developing inhibitory antibodies (low immunogenicity factor VIII). In one particular embodiment of this example, the modified factor VIII is mutated to have a consensus amino acid sequence for N-linked glycosylation. An example of such a consensus sequence is N-X-S/T, where N is asparagine, X is any amino acid, and S/T stands for serine or threonine (see U.S. Pat. No. 6,759,216 to Lollar, which is hereby incorporated by reference in its entirety). Preferably, the glycosylation site-modified factor VIII contains one or more of the mutations identified above (e.g., at positions 287, 302, 519, 665, and/or 1984).
An eighth example of a suitable mutant factor VIII that can be modified in accordance with the present invention is a modified factor VIII that is a procoagulant-active factor VIII having various mutations (see, e.g., U.S. Patent Application Publication No. 2004/0092442 to Kaufman et al., which is hereby incorporated by reference in its entirety). One example of this embodiment relates to a modified factor VIII that has been modified to (i) delete the von Willebrand factor binding site, (ii) add a mutation at Arg 740, and (iii) add an amino acid sequence spacer between the A2- and A3-domains, where the amino acid spacer is of a sufficient length so that upon activation, the procoagulant-active factor VIII protein becomes a heterodimer (see U.S. Patent Application Publication No. 2004/0092442 to Kaufman et al., which is hereby incorporated by reference in its entirety). Preferably, procoagulant active factor VIII is also modified to contain one or more of the mutations described above (e.g., at positions 287, 302, 519, 665, and/or 1984).
Further, the mutant factor VIII can be modified to take advantage of various advancements regarding recombinant coagulation factors generally (see, e.g., Saenko et al., “The Future of Recombinant Coagulation Factors,” J. Thrombosis and Haemostasis 1:922-930 (2003), which is hereby incorporated by reference in its entirety).
The recombinant factor VIII of the present invention can be modified at any charged residue that destabilizes the A1 A2 or A2A3 domain interfaces (including positions 287, 302, 519, 665, or 1984), as well as be modified to be B-domainless, to be chimeric, to have modified calcium binding sites that enhance factor VIIIa activity (e.g., at position 113), to have altered inactivation cleavage sites, to have enhanced factor IXa and/or factor X affinity, to have enhanced secretion, to have an increased circulating half-life, or to have mutant glycosylation sites; or to possess any one or more of such modifications in addition to the one or more modifications to charged residues, including a modified calcium-binding site that improves activity of the recombinant factor VIII. A number of exemplary B-domainless, enhanced specific activity, high stability recombinant factor VIII proteins are described in the Examples.
The recombinant factor VIII is preferably produced in a substantially pure form. In a particular embodiment, the substantially pure recombinant factor VIII is at least about 80% pure, more preferably at least 90% pure, most preferably at least 95% pure. A substantially pure recombinant factor VIII can be obtained by conventional techniques well known in the art. Typically, the substantially pure recombinant factor VIII is secreted into the growth medium of recombinant host cells. Alternatively, the substantially pure recombinant factor VIII is produced but not secreted into growth medium. In such cases, to isolate the substantially pure recombinant factor VIII, the host cell carrying a recombinant plasmid is propagated, lysed by sonication, heat, or chemical treatment, and the homogenate is centrifuged to remove cell debris. The supernatant is then subjected to sequential ammonium sulfate precipitation. The fraction containing the substantially pure recombinant factor VIII is subjected to gel filtration in an appropriately sized dextran or polyacrylamide column to separate the recombinant factor VIII. If necessary, a protein fraction (containing the substantially pure recombinant factor VIII) may be further purified by high performance liquid chromatography (“HPLC”).
Another aspect of the present invention relates to an isolated nucleic acid molecule that encodes the recombinant factor VIII of the present invention. The isolated nucleic acid molecule encoding the recombinant factor VIII can be either RNA or DNA.
In one embodiment, the isolated nucleic acid molecule can have a nucleotide sequence encoding a mutation at position 113 that enhances factor VIII specific activity, as modified with one or more of the substitutions of charged residues (e.g., at positions 287, 302, 519, 665, 1984, and/or 332-340 of SEQ ID NO: 2).
In another embodiment, the isolated nucleic acid molecule can have a nucleotide sequence encoding a B-domainless factor VIII of the type described above, as modified with one or more of the substitutions of charged residues (e.g., at positions 287, 302, 519, 665, and/or 1984 of SEQ ID NO:2).
In another embodiment, the isolated nucleic acid molecule can have a nucleotide sequence encoding a chimeric human/porcine of the type described above, as modified with one or more of the substitutions of charged residues (e.g., at positions 287, 302, 519, 665, and/or 1984 of SEQ ID NO:2).
In another embodiment, the isolated nucleic acid molecule can have a nucleotide sequence encoding a factor VIII whose inactivation sites have been modified as described above, as further modified with one or more of the substitutions of charged residues (e.g., at positions 287, 302, 519, 665, and/or 1984 of SEQ ID NO:2).
In yet another embodiment, the isolated nucleic acid molecule can have a nucleotide sequence encoding a factor VIII whose affinity for factor IXa and/or factor X has been enhanced, as further modified with one or more of the substitutions of charged residues (e.g., at positions 287, 302, 519, 665, and/or 1984 of SEQ ID NO:2).
In a still further embodiment, the isolated nucleic acid molecule can have a nucleotide sequence encoding a factor VIII whose affinity for various serum-binding proteins has been altered to increase its circulating half-life, as further modified with one or more of the substitutions of charged residues (e.g., at positions 287, 302, 519, 665, and/or 1984 of SEQ ID NO:2).
In a further embodiment, the isolated nucleic acid molecule can have a nucleotide sequence encoding a factor VIII that has increased secretion in culture, as further modified with one or more of the substitutions of charged residues (e.g., at positions 287, 302, 519, 665, and/or 1984 of SEQ ID NO:2).
In a further embodiment, the isolated nucleic acid molecule can have a nucleotide sequence encoding a factor VIII that possesses one or more non-naturally occurring glycosylation site, as further modified with one or more of the substitutions of charged residues (e.g., at positions 287, 302, 519, 665, and/or 1984 of SEQ ID NO:2).
In yet another embodiment, the isolated nucleic acid molecule encodes a recombinant factor VIII that is modified at any one or more charged residues as described above and is also modified to possess any two or more of the following: modified to be B-domainless, modified to be chimeric, modified to have altered inactivation cleavage sites, modified to have enhanced factor IXa and/or factor X affinity, modified to have enhanced secretion, modified to have an increased circulating half-life, modified to possess one or more non-naturally occurring glycosylation site, and modified within a calcium-binding site (e.g., at position 113) such that the specific activity of the recombinant factor VIII is improved.
Another aspect of the present invention relates to a recombinant DNA expression system that includes an isolated DNA molecule of the present invention, which expression system encodes a recombinant factor VIII. In one embodiment, the DNA molecule is in sense orientation relative to a promoter.
A further aspect of the present invention relates to a host cell including an isolated nucleic acid molecule encoding the recombinant factor VIII of the present invention. In a particular embodiment, the host cell can contain the isolated nucleic acid molecule in DNA molecule form, either as a stable plasmid or as a stable insertion or integration into the host cell genome. In another embodiment, the host cell can contain a DNA molecule in an expression system. Suitable host cells can be, without limitation, animal cells (e.g., baby hamster kidney (“BHK”) cells), bacterial cells (e.g., E. coli), insect cells (e.g., Sf9 cells), fungal cells, yeast cells (e.g., Saccharomyces or Schizosaccharomyces), plant cells (e.g., Arabidopsis or tobacco cells), or algal cells.
The recombinant DNA expression system and host cells can be produced using various recombinant techniques well-known in the art, as further discussed below.
The DNA molecule encoding the recombinant factor VIII of the present invention can be incorporated in cells using conventional recombinant DNA technology. Generally, this involves inserting the DNA molecule into an expression system to which the DNA molecule is heterologous (i.e., not normally present). The heterologous DNA molecule is inserted into the expression system or vector in sense orientation and correct reading frame. The vector contains the necessary elements for the transcription and translation of the inserted protein-coding sequences. Thus, one embodiment of the present invention provides a DNA construct containing the isolated nucleic acid of the present invention, which is operably linked to both a 5′ promoter and a 3′ regulatory region (i.e., transcription terminator) capable of affording transcription and expression of the encoded recombinant factor VIII of the present invention in host cells or host organisms.
With respect to the recombinant expression system of the present invention, an expression vector containing a DNA molecule encoding the recombinant factor VIII of the present invention can be made using common techniques in the art. The nucleic acid molecules of the present invention can be inserted into any of the many available expression vectors using reagents that are well known in the art. In preparing a DNA vector for expression, the various DNA sequences may normally be inserted or substituted into a bacterial plasmid. Any convenient plasmid may be employed, which will be characterized by having a bacterial replication system, a marker which allows for selection in a bacterium, and generally one or more unique, conveniently located restriction sites. The selection of a vector will depend on the preferred transformation technique and target host for transformation.
A variety of host-vector systems may be utilized to express the recombinant factor VIII-encoding sequence(s). Primarily, the vector system must be compatible with the host cell used. Host-vector systems include but are not limited to the following: bacteria transformed with bacteriophage DNA, plasmid DNA, or cosmid DNA; microorganisms such as yeast containing yeast vectors; mammalian cell systems infected with virus (e.g., vaccinia virus, adenovirus, adeno-associated virus, etc.); insect cell systems infected with virus (e.g., baculovirus); and plant cells infected by bacteria (e.g., Agrobacterium). The expression elements of these vectors vary in their strength and specificities. Depending upon the host-vector system utilized, any one of a number of suitable transcription and translation elements can be used.
When recombinantly produced, the factor VIII protein or polypeptide (or fragment or variant thereof) is expressed in a recombinant host cell, typically, although not exclusively, a eukaryote.
Suitable vectors for practicing the present invention include, but are not limited to, the following viral vectors such as lambda vector system gt11, gtWES.tB, Charon 4, and plasmid vectors such as pCMV, pBR322, pBR325, pACYC177, pACYC184, pUC8, pUC9, pUC18, pUC19, pLG339, pR290, pKC37, pKC101, SV 40, pBluescript II SK+/− or KS+/− (see “Stratagene Cloning Systems” Catalog (1993)), pQE, pIH821, pGEX, pET series (Studier et al, “Use of T7 RNA Polymerase to Direct Expression of Cloned Genes,” Methods in Enzymology 185:60-89 (1990), which is hereby incorporated by reference in its entirety), and any derivatives thereof. Any appropriate vectors now known or later described for genetic transformation are suitable for use with the present invention.
Recombinant molecules can be introduced into cells via transformation, particularly transduction, conjugation, mobilization, or electroporation. The DNA sequences are cloned into the vector using standard cloning procedures in the art, as described by Maniatis et al., Molecular Cloning: A Laboratory Manual, Cold Springs Harbor, N.Y.: Cold Springs Laboratory, (1982), which is hereby incorporated by reference in its entirety.
U.S. Pat. No. 4,237,224 issued to Cohen and Boyer, which is hereby incorporated by reference in its entirety, describes the production of expression systems in the form of recombinant plasmids using restriction enzyme cleavage and ligation with DNA ligase. These recombinant plasmids are then introduced by means of transformation and replicated in unicellular cultures including prokaryotic organisms and eukaryotic cells grown in tissue culture.
Different genetic signals and processing events control many levels of gene expression (e.g., DNA transcription and messenger RNA (mRNA) translation).
Transcription of DNA is dependent upon the presence of a promoter which is a DNA sequence that directs the binding of RNA polymerase and thereby promotes mRNA synthesis. The DNA sequences of eukaryotic promoters differ from those of prokaryotic promoters. Furthermore, eukaryotic promoters and accompanying genetic signals may not be recognized in or may not function in a prokaryotic system, and, further, prokaryotic promoters are not recognized and do not function in eukaryotic cells.
Similarly, translation of mRNA in prokaryotes depends upon the presence of the proper prokaryotic signals which differ from those of eukaryotes. Efficient translation of mRNA in prokaryotes requires a ribosome binding site called the Shine-Dalgarno (“SD”) sequence on the mRNA. This sequence is a short nucleotide sequence of mRNA that is located before the start codon, usually AUG, which encodes the amino-terminal methionine of the protein. The SD sequences are complementary to the 3′-end of the 16S rRNA (ribosomal RNA) and probably promote binding of mRNA to ribosomes by duplexing with the rRNA to allow correct positioning of the ribosome. For a review on maximizing gene expression, see Roberts and Lauer, Methods in Enzymology 68:473 (1979), which is hereby incorporated by reference in its entirety.
Promoters vary in their “strength” (i.e., their ability to promote transcription). For the purposes of expressing a cloned gene, it is generally desirable to use strong promoters in order to obtain a high level of transcription and, hence, expression of the gene. Depending upon the host cell system utilized, any one of a number of suitable promoters may be used. For instance, when cloning in Escherichia coli, its bacteriophages, or plasmids, promoters such as the T7 phage promoter, lac promoter, trp promoter, recA promoter, ribosomal RNA promoter, the PR and PL promoters of coliphage lambda and others, including but not limited, to lacUV5, ompF, bla, lpp, and the like, may be used to direct high levels of transcription of adjacent DNA segments. Additionally, a hybrid trp-lacUV 5 (tac) promoter or other E. coli promoters produced by recombinant DNA or other synthetic DNA techniques may be used to provide for transcription of the inserted gene.
Bacterial host cell strains and expression vectors may be chosen which inhibit the action of the promoter unless specifically induced. In certain operations, the addition of specific inducers is necessary for efficient transcription of the inserted DNA. For example, the lac operon is induced by the addition of lactose or IPTG (isopropylthio-beta-D-galactoside). A variety of other operons, such as trp, pro, etc., are under different controls.
Specific initiation signals are also required for efficient gene transcription and translation in prokaryotic cells. These transcription and translation initiation signals may vary in “strength” as measured by the quantity of gene specific messenger RNA and protein synthesized, respectively. The DNA expression vector, which contains a promoter, may also contain any combination of various “strong” transcription and/or translation initiation signals. For instance, efficient translation in E. coli requires an SD sequence about 7-9 bases 5′ to the initiation codon (“ATG”) to provide a ribosome binding site. Thus, any SD-ATG combination that can be utilized by host cell ribosomes may be employed. Such combinations include but are not limited to the SD-ATG combination from the cro gene or the N gene of coliphage lambda, or from the E. coli tryptophan E, D, C, B or A genes. Additionally, any SD-ATG combination produced by recombinant DNA or other techniques involving incorporation of synthetic nucleotides may be used.
In one embodiment, the nucleic acid molecule of the present invention is incorporated into an appropriate vector in the sense direction, such that the open reading frame is properly oriented for the expression of the encoded protein under control of a promoter of choice. This involves the inclusion of the appropriate regulatory elements into the DNA-vector construct. These include non-translated regions of the vector, useful promoters, and 5′ and 3′ untranslated regions which interact with host cellular proteins to carry out transcription and translation. Such elements may vary in their strength and specificity. Depending on the vector system and host utilized, any number of suitable transcription and translation elements, including constitutive and inducible promoters, may be used.
A constitutive promoter is a promoter that directs expression of a gene throughout the development and life of an organism.
An inducible promoter is a promoter that is capable of directly or indirectly activating transcription of one or more DNA sequences or genes in response to an inducer. In the absence of an inducer, the DNA sequences or genes will not be transcribed.
The DNA construct of the present invention can also include an operable 3′ regulatory region, selected from among those which are capable of providing correct transcription termination and polyadenylation of mRNA for expression in the host cell of choice, operably linked to a DNA molecule which encodes for a protein of choice.
The vector of choice, promoter, and an appropriate 3′ regulatory region can be ligated together to produce the DNA construct of the present invention using well known molecular cloning techniques as described in Sambrook et al., Molecular Cloning: A Laboratory Manual, Second Edition, Cold Spring Harbor Press, NY (1989), and Ausubel, F. M. et al. Current Protocols in Molecular Biology, New York, N.Y: John Wiley & Sons (1989), each of which is hereby incorporated by reference in its entirety.
As noted, one alternative to the use of prokaryotic host cells is the use of eukaryotic host cells, such as mammalian cells, which can also be used to recombinantly produce the recombinant factor VIII of the present invention. Mammalian cells suitable for carrying out the present invention include, among others: COS (e.g., ATCC No. CRL 1650 or 1651), BHK (e.g., ATCC No. CRL 6281), CHO (e.g., ATCC No. CCL 61), HeLa (e.g., ATCC No. CCL 2), 293 (ATCC No. 1573), CHOP, and NS-1 cells.
Suitable expression vectors for directing expression in mammalian cells generally include a promoter, as well as other transcription and translation control sequences known in the art. Common promoters include SV40, MMTV, metallothionein-1, adenovirus E1a, CMV, immediate early, immunoglobulin heavy chain promoter and enhancer, and RSV-LTR.
Once the DNA construct of the present invention has been prepared, it is ready to be incorporated into a host cell. Accordingly, another aspect of the present invention relates to a method of making a recombinant cell. Basically, this method is carried out by transforming a host cell with a DNA construct of the present invention under conditions effective to yield transcription of the DNA molecule in the host cell. Recombinant molecules can be introduced into cells via transformation, particularly transduction, conjugation, mobilization, or electroporation.
In view of the recombinant technology discussed herein, another aspect of the present invention relates to a method of making a recombinant factor VIII of the present invention. This method involves growing a host cell of the present invention under conditions whereby the host cell expresses the recombinant factor VIII. The recombinant factor VIII is then isolated. In one embodiment, the host cell is grown in vitro in a growth medium. In a particular embodiment, suitable growth media can include, without limitation, a growth medium containing a von Willebrand Factor (referred to herein as “VWF”). In this embodiment, the host cell can contain a transgene encoding a VWF or the VWF can be introduced to the growth medium as a supplement. VWF in the growth medium will allow for greater expression levels of the recombinant factor VIII. Once the recombinant factor VIII is secreted into the growth medium, it can then be isolated from the growth medium using techniques well-known by those of ordinary skill in the relevant recombinant DNA and protein arts (including those described herein). In another embodiment, the method of making the recombinant factor VIII of the present invention further involves disrupting the host cell prior to isolation of the recombinant factor VIII. In this embodiment, the recombinant factor VIII is isolated from cellular debris.
The modifications at positions 287, 302, 519, 665, and/or 1984 are particularly preferred, because they result in enhanced stability of both factor VIII and factor VIIIa. This increased stability is important with regard to circulating half-life of factor VIII and the activity of factor VIIIa during blood clotting. Furthermore, this property is significant in terms of enhancing the recovery of usable factor VIII during the purification and preparation of the protein for therapeutic use.
When an expression vector is used for purposes of in vivo transformation to induce factor VIII expression in a target cell, promoters of varying strength can be employed depending on the degree of enhancement desired. One of skill in the art can readily select appropriate mammalian promoters based on their strength as a promoter. Alternatively, an inducible promoter can be employed for purposes of controlling when expression or suppression of factor VIII is desired. One of skill in the art can readily select appropriate inducible mammalian promoters from those known in the art. Finally, tissue specific mammalian promoters can be selected to restrict the efficacy of any gene transformation system to a particular tissue. Tissue specific promoters are known in the art and can be selected based upon the tissue or cell type to be treated.
Another aspect of the present invention relates to a method of treating an animal for a blood disorder such as hemophilia, particularly hemophilia A. This method involves administering to an animal exhibiting hemophilia A an effective amount of the recombinant factor VIII of the present invention, whereby the animal exhibits effective blood clotting following vascular injury. A suitable effective amount of the recombinant factor VIII can include, without limitation, between about 10 to about 50 units/kg body weight of the animal. The animal can be any mammal, but preferably a human, a rat, a mouse, a guinea pig, a dog, a cat, a monkey, a chimpanzee, an orangutan, a cow, a horse, a sheep, a pig, a goat, or a rabbit.
The recombinant factor VIII of the present invention can be used to treat uncontrolled bleeding due to factor VIII deficiency (e.g., intraarticular, intracranial, or gastrointestinal hemorrhage) in hemophiliacs with and without inhibitory antibodies and in patients with acquired factor VIII deficiency due to the development of inhibitory antibodies. In a particular embodiment, the recombinant factor VIII, alone, or in the form of a pharmaceutical composition (i.e., in combination with stabilizers, delivery vehicles, and/or carriers) is infused into patients intravenously according to the same procedure that is used for infusion of human or animal factor VIII.
Alternatively, or in addition thereto, the recombinant factor VIII can be administered by administering a viral vector such as an adeno-associated virus (Gnatenko et al., “Human Factor VIII Can Be Packaged and Functionally Expressed in an Adeno-associated Virus Background: Applicability to Hemophilia A Gene Therapy,” Br. J. Haematol. 104:27-36 (1999), which is hereby incorporated by reference in its entirety), or by transplanting cells genetically engineered to produce the recombinant factor VIII, typically via implantation of a device containing such cells. Such transplantation typically involves using recombinant dermal fibroblasts, a non-viral approach (Roth et al., “Nonviral Transfer of the Gene Encoding Coagulation Factor VIII in Patients with Sever Hemophilia,” New Engl. J. Med. 344:1735-1742 (2001), which is hereby incorporated by reference in its entirety).
The treatment dosages of recombinant factor VIII that should be administered to a patient in need of such treatment will vary depending on the severity of the factor VIII deficiency. Generally, dosage level is adjusted in frequency, duration, and units in keeping with the severity and duration of each patient's bleeding episode. Accordingly, the recombinant factor VIII is included in a pharmaceutically acceptable carrier, delivery vehicle, or stabilizer in an amount sufficient to deliver to a patient a therapeutically effective amount of the protein to stop bleeding, as measured by standard clotting assays.
Factor VIII is classically defined as that substance present in normal blood plasma that corrects the clotting defect in plasma derived from individuals with hemophilia A. The coagulant activity in vitro of purified and partially-purified forms of factor VIII is used to calculate the dose of recombinant factor VIII for infusions in human patients and is a reliable indicator of activity recovered from patient plasma and of correction of the in vivo bleeding defect. There are no reported discrepancies between standard assay of novel factor VIII molecules in vitro and their behavior in the dog infusion model or in human patients, according to Lusher et al., “Recombinant Factor VIII for the Treatment of Previously Untreated Patients with Hemophilia A—Safety, Efficacy, and Development of Inhibitors,” New Engl. J. Med. 328:453-459 (1993); Pittman et al., “A2 Domain of Human Recombinant-derived Factor VIII is Required for Procoagulant Activity but not for Thrombin Cleavage,” Blood 79:389-397 (1992); and Brinkhous et al., “Purified Human Factor VIII Procoagulant Protein: Comparative Hemostatic Response After Infusions into Hemophilic and von Willebrand Disease Dogs,” Proc. Natl. Acad. Sci. 82:8752-8755 (1985), which are hereby incorporated by reference in their entirety.
Usually, the desired plasma factor VIII activity level to be achieved in the patient through administration of the recombinant factor VIII is in the range of 30-100% of normal. In one embodiment, administration of the therapeutic recombinant factor VIII is given intravenously at a preferred dosage in the range from about 5 to 50 units/kg body weight, and particularly in a range of 10-50 units/kg body weight, and further particularly at a dosage of 20-40 units/kg body weight; the interval frequency is in the range from about 8 to 24 hours (in severely affected hemophiliacs); and the duration of treatment in days is in the range from 1 to 10 days or until the bleeding episode is resolved. See, e.g., Roberts and Jones, “Hemophilia and Related Conditions—Congenital Deficiencies of Prothrombin (Factor II, Factor V, and Factors VII to XII),” Ch. 153, 1453-1474, 1460, in Hematology, Williams, W. J., et al., ed. (1990), which is hereby incorporated by reference in its entirety. Patients with inhibitors may require a different amount of recombinant factor VIII than their previous form of factor VIII. For example, patients may require less recombinant factor VIII because of its higher specific activity than the wild-type VIII and its decreased antibody reactivity. As in treatment with human or plasma-derived factor VIII, the amount of therapeutic recombinant factor VIII infused is defined by the one-stage factor VIII coagulation assay and, in selected instances, in vivo recovery is determined by measuring the factor VIII in the patient's plasma after infusion. It is to be understood that for any particular subject, specific dosage regimens should be adjusted over time according to the individual need and the professional judgment of the person administering or supervising the administration of the compositions, and that the concentration ranges set forth herein are exemplary only and are not intended to limit the scope or practice of the claimed recombinant factor VIII.
Treatment can take the form of a single intravenous administration of the recombinant factor VIII or periodic or continuous administration over an extended period of time, as required. Alternatively, therapeutic recombinant factor VIII can be administered subcutaneously or orally with liposomes in one or several doses at varying intervals of time.
The recombinant factor VIII can also be used to treat uncontrolled bleeding due to factor VIII deficiency in hemophiliacs who have developed antibodies to human factor VIII.
It has been demonstrated herein that the recombinant factor VIII of the present invention can differ in specific activity from the wild-type factor VIII. Factor VIII proteins having greater procoagulant activity from wild-type factor VIII are useful in treatment of hemophilia because lower dosages will be required to correct a patient's factor VIII deficiency. This will not only reduce medical expense for both the patient and the insurer, but also reduce the likelihood of developing an immune response to the factor VIII (because less antigen is administered).
EXAMPLESThe following examples are provided to illustrate embodiments of the present invention but they are by no means intended to limit its scope.
Materials & Methods ReagentsRecombinant factor VIII (Kogenate™) was a generous gift from Dr. Lisa Regan of Bayer Corporation (Berkeley, Calif.). Phospholipid vesicles containing 20% phosphatidylcholine (PC), 40% phosphatidylethanolamine (PE), and 40% phosphatidylserine (PS) were prepared using octylglucoside as described previously (Mimms et al., “Phospholipid Vesicle Formation and Transmembrane Protein Incorporation Using Octyl Glucoside,” Biochemistry 20:833-840 (1981), which is hereby incorporated by reference in its entirety). The reagents α-thrombin, factor Vila, factor IXaβ, factor X, and factor Xa (Enzyme Research Laboratories, South Bend, Ind.), hirudin and phospholipids (DiaPharma, West Chester, Ohio), the chromogenic Xa substrate, Pefachrome Xa (Pefa-5523, CH3OCO-D-CHA-Gly-Arg-pNA.AcOH; Centerchem Inc. Norwalk Conn.), recombinant human tissue factor (rTF), Innovin (Dade Behring, Newark, Del.), fluorogenic substrate, Z-Gly-Gly-Arg-AMC (Calbiochem, San Diego, Calif.), and thrombin calibrator (Diagnostica Stago, Parsippany, N.J.) were purchased from the indicated vendors.
Construction, Expression and Purification of WT and Variant Factor VIII:Ala mutants (at D27, H281, R282, E287, D302, S313, H317, T522, S524, R531, N538, E540, S650, S654, D666, E683, N684, S695, D696, S1791, D1795, Q1820, E1829, S1949, N1950, and R1966); Phe mutants (at Y476, Y664, Y1786, and Y1792); Ala and Val mutants (at charged residues E272, D519, E665, and E1984); and WT factor VIII forms were individually constructed as a B-domainless factor VIII, lacking residues Gln744-Ser1637 in the B-domain (Doering et al., “Expression and Characterization of Recombinant Murine Factor VIII,” Thromb Haemost. 88:450-458 (2002), which is hereby incorporated by reference in its entirety). The cloning and expression constructs were generous gifts from Dr. Pete Lollar and John Healey. Recombinant WT and variant factor VIII forms were stably expressed in BHK cells and purified as described previously (Wakabayashi et al., “Residues 110-126 in the A1 Domain of Factor VIII Contain a Ca2+ Binding Site Required for Cofactor Activity,” J Biol Chem. 279:12677-12684 (2004), which is hereby incorporated by reference in its entirety). After transfection there were no significant differences in the amounts of factor VIII secretion among the variants. Protein yields for the variants ranged from >10 to −100 μg from two 750 cm2 culture flasks, with purity from ˜85% to >95% as judged by SDS-PAGE. The primary contaminant in the factor VIII preparations was albumin and at the concentrations present in the factor VIII showed no effect on stability of activity parameters. Factor VIII concentration was measured using an Enzyme-Linked Immunoadsorbant Assay (ELISA) and factor VIII activity was determined by an one-stage clotting assay and a two-stage chromogenic factor Xa generation assay as described below.
SDS-PAGE and Western BlottingFactor VIII proteins (0.77 μg for gel staining and 0.34 μg for Western blot) were electrophoresed on 8% polyacrylamide gel at constant voltage (100V). Gels were stained with Gelcode Blue (Thermo Scientific, Rockford, Ill.) or transferred to a polyvinylidene fluoride membrane and probed with biotinylated anti-A2 antibody (R8B12, Green Mountain Antibodies, Burlington, Vt.) followed by the incubation with peroxidase-conjugated streptoavidin (Calbiochem, San Diego, Calif.). The chemifluorescence substrate (ECF substrate, GE Healthcare, Piscataway, N.J.) was reacted and the fluorescence signal scanned using a phosphoimager (Storm 860, GE Healthcare). The density of single chain factor VIII form (170 kDa) and heavy chain (HC, 90 kDa) were quantified using ImageQuant software (GE Healthcare) and the amount ratios were calculated.
ELISAA sandwich ELISA was performed to measure the concentration of factor VIII proteins as previously described (Wakabayashi et al., “A Glu113Ala Mutation within a Factor VIII Ca2+-Binding Site Enhances Cofactor Interactions in Factor Xase,” Biochemistry 44:10298-10304 (2005), which is hereby incorporated by reference in its entirety) using purified commercial recombinant factor VIII (Kogenate, Bayer Corporation) as a standard. Factor VIII capture used the anti-C2 antibody (ESH-8, American Diagnostica Inc., Stamford, Conn.) and a biotinylated R8B12 antibody, was employed for factor VIII detection.
One-Stage Clotting AssayOne-stage clotting assays were performed using substrate plasma chemically depleted of factor VIII (Over, “Methodology of the One-stage Assay of Factor VIII (VIII:C),” Scand J Haematol Suppl. 41:13-24 (1984), which is hereby incorporated by reference in its entirety) and assayed using a Diagnostica Stago clotting instrument. Plasma was incubated with APTT reagent (General Diagnostics) for 6 min at 37° C. after which a dilution of factor VIII was added to the cuvette. After 1 min the mixture was recalcified, and clotting time was determined and compared to a pooled normal plasma standard.
Two-Stage Chromogenic Factor Xa Generation AssayThe rate of conversion of factor X to factor Xa was monitored in a purified system (Lollar et al., “Factor VIII and Factor VIIIa,” Methods Enzymol. 222:128-143 (1993), which is hereby incorporated by reference in its entirety) according to methods previously described (Wakabayashi et al., “Metal Ion-independent Association of Factor VIII Subunits and the Roles of Calcium and Copper Ions for Cofactor Activity and Inter-subunit Affinity,” Biochemistry 40:10293-10300 (2001); Wakabayashi et al., “Ca2+ Binding to Both the Heavy and Light Chains of Factor VIII Is Required for Cofactor Activity,” Biochemistry 41:8485-8492 (2002), each of which is hereby incorporated by reference in its entirety). Factor VIII (1 nM) in buffer containing 20 mM N-[2-hydroxyethyl]piperazine-N′-[2-ethanesulfonic acid] (HEPES), pH 7.2, 0.1 M NaCl, 0.01% Tween 20, 0.01% BSA, 5 mM CaCl2, and 10 μM PSPCPE vesicles (Buffer A) was activated with 20 nM α-thrombin for 1 min. The reaction was stopped by adding hirudin (10 U/ml) and the resulting factor VIIIa was reacted with factor IXa (40 nM) for 1 mM. Factor X (300 nM) was added to initiate reactions which were quenched after 1 mM by the addition of 50 mM EDTA. Factor Xa generated was determined following reaction with the chromogenic substrate Pefachrome Xa (0.46 mM final concentration). All reactions were run at 23° C.
Thrombin Generation AssayThe amount of thrombin generated in plasma was measured by Calibrated Automated Thrombography (Hemker et al., “Calibrated Automated Thrombin Generation Measurement in Clotting Plasma,” Pathophysiol Haemost Thromb. 33:4-15 (2003); Hemker et al., “Thrombin Generation in Plasma: Its Assessment via the Endogenous Thrombin Potential,” Thromb Haemost. 74:134-138 (1995), each of which is hereby incorporated by reference in its entirety). In a 96-well plate, 80 μl of factor VIII deficient plasma (<1% residual activity, platelet-poor) from severe hemophilia A patient lacking factor VIII inhibitor (George King Bio-Medical, Overland Park, Kans.) was mixed with factor VIII samples (20 μl; 6 nM) in HEPES-BSA buffer (20 mM HEPES, pH 7.35, 0.15 M NaCl, 6% BSA) containing 3 pM rTF (the concentration of rTF stock was determined by factor Xa generation assay using known concentrations of factor VIIa), PSPCPE vesicles (24 μM) or 20 μl thrombin calibrator (630 nM) and reactions were immediately started by mixing with 20 μl fluorogenic substrate (2.5 mM, Z-Gly-Gly-Arg-AMC) in HEPES-BSA buffer including 0.1 M CaCl2. All reagents were pre-warmed at 37° C. Final concentrations of reagents were 1 nM factor VIII (except as otherwise noted), 0.5 pM rTF, 4 μM PSPCPE vesicles, 433 μM fluorogenic substrate, 13.3 mM CalCl2, and 105 nM thrombin calibrator. The development of a fluorescent signal at 37° C. was monitored at 8 second intervals using a Microplate Spectrofluorometer (Spetramax Gemini, Molecular Devices, Sunnyvale, Calif.) with a 355 nm (excitation)/460 nm (emission) filter set. Fluorescent signals were corrected by the reference signal from the thrombin calibrator samples (Hemker et al., “Calibrated Automated Thrombin Generation Measurement in Clotting Plasma,” Pathophysiol Haemost Thromb. 33:4-15 (2003), each of which is hereby incorporated by reference in its entirety) and actual thrombin generation in nM was calculated as previously described (Hemker et al., “Thrombin Generation in Plasma: Its Assessment via the Endogenous Thrombin Potential,” Thromb Haemost. 74:134-138 (1995), which is hereby incorporated by reference in its entirety).
Factor VIII Activity at Elevated TemperatureWT factor VIII or factor VIII variants (4 nM) in buffer A were incubated at 52-60° C. Aliquots were removed at the indicated times and residual factor VIII activity was determined using a two-stage chromogenic factor Xa generation assay.
Factor VIIIa Activity Time Course
WT and mutant factor VIII (4 nM) in buffer A containing 10 μM PSPCPE vesicles were activated by 20 nM thrombin for 1 min at 23° C. Reactions were immediately quenched by hirudin (10 U/ml), aliquots removed at the indicated times, and activity was determined using the factor Xa generation assay following addition of factor IXa (40 nM) and factor X (300 nM). For decay measurements run in the presence of factor IXa, factor IXa (40 nM) was added to reactions prior to thrombin addition.
Factor VIII Stability in PlasmaWT or variant factor VIII (1 nM) was added to factor VIII deficient plasma (<1% residual activity) from severe hemophilia A patient lacking factor VIII inhibitor (George King Bio-Medical). Plasma was supplemented with 0.02% NaN3 to prevent the growth of microorganisms and samples were incubated at 37° C. Aliquots were removed at the indicated times and residual activity was determined by a one-stage clotting assay.
Data AnalysisFactor VIIIa activity values as a function of time were fitted to a single exponential decay curve by non-linear least squares regression using the equation,
A=A0×e−k−t
where A is residual factor VIIIa activity (nM/min/nM factor VIII), A0 is the initial activity, k is the apparent rate constant, and t is the time (minutes) of reaction of either factor VIII at elevated temperature (for factor VIII decay experiments) or after thrombin activation was quenched (for factor VIIIa decay measurements). Nonlinear least-squares regression analysis was performed by Kaleidagraph (Synergy, Reading, Pa.). Comparison of average values was performed by the Student's t-test. The factor VIII A domain modeled structure (Pemberton et al., “A Molecular Model for the Triplicated A Domains of Human Factor VIII Based on the Crystal Structure of Human Ceruloplasmin,” Blood 89:2413-2421 (1997), which is hereby incorporated by reference in its entirety) was analyzed using Swiss PDB Viewer to identify charged residues that were located at the A2 domain interface and that showed little potential for hydrogen bonding interactions based on a threshold of >2.8 Å separating the polar atoms of the complementary domains (Weiner et al., “A New Force Field for Molecular Mechanical Simulation of Nucleic Acids Proteins,” J Am Chem Soc. 106:765-784 (1984), which is hereby incorporated by reference in its entirety).
Example 1 Activity Values for Factor VIII Mutants Targeting Hydrogen Bonding InteractionsBonding interactions involving the A2 domain in factor VIII remain poorly understood yet represent a primary mechanism for the regulation of cofactor activity. The factor VIII homology model (Pemberton et al., “A Molecular Model for the Triplicated A Domains of Human Factor VIII Based on the Crystal Structure of Human Ceruloplasmin,” Blood 89:2413-2421 (1997), which is hereby incorporated by reference in its entirety) identifies the potential for many hydrogen bonds linking residues in the A2 domain with those in the A1 or A3 domains. Using a criterion for a spatial separation of <2.8 Å between hydrogen donor and acceptor atoms (Weiner et al., “A New Force Field for Molecular Mechanical Simulation of Nucleic Acids Proteins,” J Am Chem Soc. 106:765-784 (1984), which is hereby incorporated by reference in its entirety) thirty residues were identified as having a side chain atom that may be involved in hydrogen bonding with an atom from a complementary A domain (see Table 1 below). In approximately half of the residues identified, side chain atoms were juxtaposed with either backbone carbonyl oxygen or amide hydrogen atoms, while the remainder represented possible interactions between neighboring side chains. Target residues in the factor VIII A domains were individually mutated to Ala, with the exception that Tyr residues were replaced with Phe, and the point mutations were stably expressed as B-domainless factor VIII.
Factor VIII activity was measured for the purified proteins using a one-stage clotting assay and a (two-stage) factor Xa generation assay. Results from the one-stage assay (
To assess the heat-stability of the WT procofactor and variants, a temperature at 55° C. was employed based upon factor VIII inactivation results described in an earlier study (Ansong et al., “Factor VIII A3 Domain Residues 1954-1961 Represent an A1 Domain-Interactive Site,” Biochemistry 44:8850-8857 (2005), which is hereby incorporated by reference in its entirety). For these reactions, factor VIII was incubated for indicated times at the elevated temperature, after which the reaction mixture was immediately cooled to room temperature, and factor VIII reacted with thrombin and assayed for cofactor activity using a factor Xa generation assay. Rates of loss for factor VIII activity to the heat treatment, as judged by residual cofactor function, was determined as described in Methods.
Table 2 (below) summarizes the results obtained from factor VIII thermostability assays for the 30 variants. Overall, these activity data fit well to a single exponential decay function with correlation coefficients in most cases >0.98. While a number of mutations were benign with respect to the amino acid replacement (21 showing <2-fold differences in rates of decay), several residues including Arg282 (A1 domain), and A2 domain residues Ser524, Asn684 and Ser650 showed ˜5- to ˜20-fold increased rates in factor VIII decay suggesting an important role for these residues in maintaining factor VIII stability. Furthermore, the R282A and N684A variants showed significantly reduced specific activity values suggesting both activity and stability parameters were affected by the single point mutations. On the other hand, replacement of E287 and D302 with Ala yielded reduced rates for factor VIII decay at the elevated temperature. This apparent increase in protein stability following mutation is consistent with these acidic side chains destabilizing inter-domain interactions in the WT cofactor.
Factor VIIIa activity is labile due to A2 subunit dissociation (Fay et al., “Human Factor VIIIa Subunit Structure: Reconstruction of Factor VIIIa from the Isolated A1/A3-C1-C2 Dimer and A2 Subunit,” J Biol Chem. 266:8957-8962 (1991); Lollar et al., “pH-dependent Denaturation of Thrombin-activated Porcine Factor VIII,” J Biol Chem. 265:1688-1692 (1990), each of which is hereby incorporated by reference in its entirety). Results from earlier studies showed that inclusion of factor IXa and phospholipid vesicles with factor VIIIa to form the Xase complex reduced the lability of the cofactor (Lollar et al., “Stabilization of Thrombin-activated Porcine Factor VIII:C by Factor IXa Phospholipid,” Blood 63:1303-1308 (1984); Lamphear et al., “Factor IXa Enhances Reconstitution of Factor VIIIa from Isolated A2 Subunit and A1/A3-C1-C2 Dimer,” J. Biol. Chem. 267:3725-3730 (1992), each of which is hereby incorporated by reference in its entirety) by partially stabilizing the A2 subunit within factor Xase (Fay et al., “Model for the Factor VIIIa-dependent Decay of the Intrinsic Factor Xase: Role of Subunit Dissociation and Factor IXa-catalyzed Proteolysis,” J Biol Chem. 271:6027-6032 (1996), which is hereby incorporated by reference in its entirety). This approach was recently used to examine the decay rate for an E1829A factor VIIIa mutant (Wakabayashi et al., “A3 Domain Residue Glu1829 Contributes to A2 Subunit Retention in Factor VIIIa,” J. Thromb. Haemost. 5:996-1001 (2007), which is hereby incorporated by reference in its entirety) since the activity decay of this variant factor VIIIa, in the absence of factor IXa and membrane, was too rapid to measure accurately. This approach was similarly employed to assess rates for factor VIIIa decay for the panel of variants described in this Example. Factor VIII (4 nM) was incubated with a molar excess of factor IXa (40 nM) and phospholipid vesicles, rapidly activated with thrombin and subsequent factor Xase activity was measured over a time course at 23° C. Rates of decay of factor Xase activity was attributed to A2 subunit dissociation and data were fitted using a single exponential decay. Given the high Kd value for the affinity of A2 subunit within factor VIIIa (144 nM) and the low factor VIIIa concentration (4 nM) used in the reactions, the effect of re-association of dissociated A2 subunit is negligible, supporting use of a simple single exponential applied for this regression analysis.
Results are presented in
Conversely, the variants E287A and D302A that possessed greater thermostabilities than WT factor VIII also yielded enhanced stability of factor VIIIa as judged by reductions in the rates of cofactor decay following activation by thrombin. Results with the D302A variant were more pronounced and showed an ˜2-fold reduced rate of cofactor decay relative to WT factor VIIIa, retaining ˜90% of its original activity after 40 min. This observation was consistent with the mutations primarily altering conformation at the inter-domain interface in the procofactor.
Taken together, these results in Examples 1-3 identify contributions of multiple residues to inter-A2 (domain) subunit interactions in the procofactor and cofactor forms of factor VIII, with selected residues making disparate contributions to protein stability. While the observed effects of mutation at the target residues were for the most part either benign or detrimental, the mutations at two A1 domain acidic residues, D302 and E287, yielded modest enhancement in stability in both pro- and active cofactor forms. The relative activity of E287 was somewhat reduced compared with WT, whereas the activity values for the D302 variant were indistinguishable from the WT protein, and suggest the latter represents a gain-of-function mutation. These results indicate that some destabilization may result from burying the (negative) charge at the interface and/or an increase in stability when these residue side chains are hydrophobic.
Example 4 Identification of Additional Target Residues and Generation of Point Mutants at Glu272, Asp519, Glu665, and Glu1984Based on the results of the preceding Examples, the substitution of other charged residues was explored. Using the ceruloplasmin-based homology model (Pemberton et al., “A Molecular Model for the Triplicated A Domains of Human Factor VIII Based on the Crystal Structure of Human Ceruloplasmin,” Blood 89:2413-2421 (1997), which is hereby incorporated by reference in its entirety) for the A domains of factor VIII, four charged residues were identified (Glu272, Asp519, Glu665, and Glu1984). These four residues appear to be buried at the interface of the A2 domain with either the A1 domain (Glu272 and Asp519) or the A3 domain (Glu665, and Glu1984), but did not appear to contribute to H-bonding interactions based upon spatial separations of >2.8 Å with potential bonding neighbors. These residues were mutated to either Ala or Val to eliminate charge as well as provide for potential hydrophobic interactions with similar side chains from other buried residues. Factor VIII variants were prepared as B-domainless factor VIII in stable-expressing BHK cell lines.
Factor VIII was expressed as a mixture of single chain and heterodimer forms. The purified proteins ranged from ˜85% to >95% as judged by SDS-PAGE (
Purified proteins were assessed for specific activity using both one-stage and two-stage assays (
The purified factor VIII mutant proteins were assessed for stability at elevated temperatures as judged by rates of activity loss. Factor VIII (4 nM) was incubated at 52-60° C. and at the indicated times an aliquot was removed, cooled to room temperature, reacted with thrombin, and residual cofactor activity was measured using a factor Xa generation assay as described in the Materials and Methods. Results shown in
Results assessing a range of temperatures (
To test the effects of the mutations on factor VIII stability under more native conditions, a near physiological concentration of the proteins (1 nM) was incubated in (anti-coagulated) factor VIII deficient plasma from a hemophilia A patient free from factor VIII inhibitor activity at 37° C. for up to 4 days. Residual factor VIII was assayed daily using a one-stage clotting assay. Activity of the WT factor VIII was reduced to ˜50% after 2 days as was that of the Asp519Val variant, while the Glu665Ala variant showed a modest (˜15%) reduction in the rate of activity decay (
The above results indicate that mutations consistent with replacing buried charged residues with hydrophobic residues in general yielded factor VIII protein showing enhanced stability. Inasmuch as these mutations are at or near the interface of the A2 domain with A1 or A3, it was predicted that they could positively impact the lability of factor VIIIa by reducing rates for dissociation of the A2 subunit. Rates of loss of factor VIIIa activity resulting from this mechanism were assessed under two conditions. In the first, the WT and factor VIII variants were activated with thrombin and at indicated times the remaining cofactor activity was determined following addition of factor IXa and factor X and monitoring rates of factor Xa generation. In the second method, the above assay was modified to include addition of factor IXa prior to factor VIII activation to allow for immediate formation of factor Xase. Incorporation of factor VIIIa in the factor Xase complex has been shown to partially stabilize cofactor activity by reducing its decay rate as much as 10-fold by a mechanism consistent with factor IXa tethering the A2 and A3C1C2 subunits with Xase (Fay et al., “Model for the Factor VIIIa-dependent Decay of the Intrinsic Factor Xase: Role of Subunit Dissociation and Factor IXa-catalyzed Proteolysis,” J Biol Chem. 271:6027-6032 (1996), which is hereby incorporated by reference in its entirety).
Results obtained in the absence or presence of added factor IXa are shown in
Mutations at the other three sites (Asp519, Glu665 and Glu1984) all resulted in reductions in factor VIIIa decay rates with the degree of reduction variable depending upon the specific residue changed and in one case, the replacement residue. Mutations at Asp519 yielded ˜30% reductions in decay rates that were similar for both the Ala and Val variants when factor IXa was absent. Rates for activity decay of these variants were decreased >2-fold in the presence of factor IXa, suggesting a synergy of the mutations with the stabilizing effects of binding the enzyme. While the Glu665Ala variant showed similar values to the two Asp519 variants, the Glu665Val variant showed 5-fold and 3-fold reductions in decay rates in the absence and presence of factor IXa, respectively, suggesting replacement with the larger hydrophobic residue yielded a more favorable interaction with neighboring residues for A2 subunit retention. Finally, both Glu1984 variants showed-4-fold reductions in factor VIIIa decay compared with WT in the absence of factor IXa, and 5-8-fold reductions when factor IXa was present. The significance of this enhanced stability is observed in
The above Examples demonstrate that substitution of selected charged residues with hydrophobic ones at sites predicted to interface the A2 domain resulted in a general, though variable, increase in the stability of factor VIII. This stability was assessed following activity retention at elevated temperature as well as by reduction in the rate of A2 subunit dissociation in the cofactor.
In the initial analysis of Examples 1-3, 30 residues localized to the factor VIII A2 domain interface were selected for mutational analysis based upon spatial separations of <2.8 Å, which could potentially form hydrogen-bonding partners. The 30 charged/polar residues were mutated to Ala (or Phe for Tyr residues), recombinant proteins stably expressed, and rates of loss of activity were measured. Fourteen of the 30 residues examined showed >2-fold increases in rates of factor VIII decay at 55° C. and/or rates for factor VIIIa decay relative to WT, suggesting that multiple residues at the A1A2 and A2A3 domain interfaces contribute to the stabilization of factor VIII. Interestingly, two acidic residues that were examined, Asp302 and Glu287, yielded modest (<2-fold) enhancement in stability in both the procofactor and active cofactor forms when mutated to Ala. Both of these acidic residues are conserved in human, canine, porcine, mouse, rabbit, rat, and bat factor VIII. These initial results suggested that these acidic side chains did not contribute to stabilizing hydrogen-bonding interactions but rather were somewhat detrimental to factor VIII structure as assessed by functional stability.
Based on these initial studies, the creation of additional hydrophobic interactions were assessed for gain of function. The four acidic residues examined in Examples 4-7 are conserved in human, canine, porcine, mouse, rabbit, and bat factor VIII, while Glu665 is Ala and Glu1984 is Thr in rat factor (see Swiss Institute of Bioinformatics, online analysis UniProtKB/Swiss-Prot Release 55.5 and UniProtKB/TrEMBL Release 38.5 (2008), which is hereby incorporated by reference in its entirety). The results of Examples 4-7 demonstrate that three of these residues, Asp519, Glu665 and Glu1984, when replaced with Ala and/or Val, resulted in enhancements in protein stability. Only one acidic residue evaluated in Examples 4-7 yielded results that were detrimental to activity when mutated. Mutation at Glu272 to Ala yielded a low specific activity factor VIII form with reduced thrombin generation parameters values; and both Ala and Val replacements possessed moderately decreased thermostability and 2-3-fold higher rates of A2 subunit dissociation in the cofactor form as compared with WT. From these observations, it is believed that Glu272 may indeed participate in bonding interaction(s) with neighboring residues, and subsequent mutations at this site disrupt these interactions. This conclusion is consistent with examination of the Hemophilia A database (Kemball-Cook et al., “The Factor VIII Structure and Mutation Resource Site: HAMSTeRS version 4,” Nucleic Acids Res. 26:216-219 (1998); Kemball-Cook (MRC Clinical Sciences Centre), Haemophilia A Mutation Database (accessed Jul. 2, 2008), each of which is hereby incorporated by reference in its entirety), which lists Lys (charge reversal) or Gly (small side chain) at position 272 as a moderate/mild phenotype with reduced factor VIII antigen. The latter observation is consistent with the mutations yielding increased plasma instability. However, there was no significant effect of these mutations on levels of expression in cell culture following mutations at this site to Ala or Val. Conversely, no mutations at Asp519, Glu665 and Glu1984 are listed in the database.
Proteins tend to fold so that the charged or polar moieties remain solvent exposed while hydrophobic groups are buried (Pace et al., “Forces Contributing to the Conformational Stability of Proteins,” FASEB J. 10:75-83 (1996), which is hereby incorporated by reference in its entirety). Therefore, based upon the observed gain-of-function mutations at Glu287, Asp302, Asp519, Glu665 and Glu1984 when these residues are replaced with hydrophobic ones, it is believed that these charged residues are buried at the A2 domain interfaces. Furthermore, these results suggest that these acidic residues do not contribute to electrostatic bonding interactions and are likely destabilizing to WT protein structure and/or subunit interactions.
Because mutagenesis using either Ala or Val resulted in a hydrophobic residue (to replace the charged acidic residues), the Ala or Val substitution would tend to stabilize other hydrophobic contacts at the interface. Furthermore, the Val side chain is larger than Ala, so comparison of effects on activity following replacement at a given site may offer some insights into residue packing and volume at that site. For example, that replacement of Glu1984 with either residue yielded similar results, suggesting both were well-tolerated at that site; whereas Glu665Val showed a 3-fold reduced factor VIIIa decay rate compared with Glu665Ala, suggesting the larger volume side chain of Val was better tolerated in the putative hydrophobic binding pocket.
Overall, the results of Example 1-7 contribute significantly to the understanding of factor VIII A domain structure, which has previously been limited to models derived from homology with a high resolution structure for ceruloplasmin (Pemberton et al., “A Molecular Model for the Triplicated A Domains of Human Factor VIII Based on the Crystal Structure of Human Ceruloplasmin,” Blood 89:2413-2421 (1997), which is hereby incorporated by reference in its entirety) and a recent, intermediate resolution structure (3.75 Å) of human factor VIII (Shen et al., “The Tertiary Structure and Domain Organization of Coagulation Factor VIII,” Blood 111:1240-1247 (2008), which is hereby incorporated by reference in its entirety). While the latter structure does not allow for assignments of hydrogen bonding interactions (<2.8 Å), the authors of that study indicate that the A domains of factor VIII can be superimposed onto those of ceruloplasmin with a high degree of accuracy.
While the ceruloplasmin model suggests Asp302 and Glu287 could contribute hydrogen bonding interactions, the stability studies of Example 1-3 demonstrate that this in unlikely. Instead, these acidic side chains are believed to be buried in a hydrophobic environment. Conversely, results from Examples 4-7 support the belief that Glu272 likely contributes a hydrogen bonding interaction at the A2 domain interface, because loss of this charge reduces factor VIII (VIIIa) stability. The remaining three acidic residues evaluated in Examples 4-7 appear to be buried at the interface as predicted by the model, in that no polar atom from a neighboring residue on a complementary domain appears to localize near the carboxylic groups of these residues. Rather, it is noted that these moieties appear to be proximal with hydrophobic groups. For example, the model predicts that the carboxyloxygen of Asp519 and methyl carbon of Thr275 are separated by ˜4.2 Å, the carboxyloxygen of Glu665 and methyl carbon of Val1982 are separated by ˜8.1 Å, and the carboxyloxygen of Glu1984 and methyl carbon of Val663 are separated by ˜6.2 Å.
Factor VIII variants demonstrating enhanced stability and reduced rates of cofactor activity decay represent positive attributes for a therapeutic preparation. The former property should allow for increased yields of active protein during its purification and formulation, resulting in overall higher specific activity values. These reagents may also possess a longer circulating half-life relative to WT (see
The results of Examples 1-7 using a physiologic factor VIII level (1 nM) showed little difference between WT and the variants demonstrating higher stability, although the Glu272Ala yielded reduced thrombin generation parameters consistent with its lower specific activity. The failure to observe a significant difference with the high stability variants may reflect differences in reaction conditions and/or that these mutations do not covalently bridge the A2 domain and the rates for factor VIIIa decay are not sufficiently reduced.
Results presented in Examples 1-7 demonstrate several-fold decreases in rates for cofactor inactivation can be achieved following single point mutations to convert acidic residues to hydrophobic ones. In each of these case, these mutations occur at interfaces where the altered residues are likely buried and not surface exposed, and do not alter covalent interactions within the protein. Based on preliminary results, the cofactor forms of the Glu1984Val and -Ala variants and the WT cofactor show similar rates of inactivation as measured by activated protein C-catalyzed cleavages at Arg336 and Arg562 (Varfaj et al., “Residues Surrounding Arg336 and Arg562 Contribute to the Disparate Rates of Proteolysis of Factor VIIIa Catalyzed by Activated Protein C,” J. Biol. Chem. 282(28):20264-72 (2007), which is hereby incorporated by reference in its entirety). This supports the belief that down-regulation of these higher stability variants should also proceed via the protein C pathway in much the same way as WT cofactor. Thus, the stabilized variants of the present invention should be free from the problems associated with the inactivation-resistant mutants described above.
Example 8 Stability Analysis of Di- and Tri-substituted Factor VIII VariantsTo determine whether additive or synergistic effects will result in further enhancements in factor VIII (VIIIa) stability, combinations of the point mutations described in the preceding Examples have been prepared using the same procedures described in the Materials and Methods. In particular, double or triple combination mutants were prepared with the Ala or Val substitutions of residues Asp519, Glu665, and Glu1984. These combination mutants (amino acids are identified using the single letter code) include: D519AE665A, D519AE665V, D519AE1984A, D519AE1984V, D519VE665V, D519VE1984A, D519VE1984V, E665AE1984A, E665AE1984V, E665VE1984A, E665VE1984V, D519AE665VE1984A, D519VE665VE1984A, D519VE665VE1984V. D519VE665A factor VIII was excluded from this analysis, because this mutant showed atypical characteristics in ELISA and Western blot results.
To produce triple mutants, D519A or D519V was combined with either E665VE1984A or E665VE1984V. The other combinations were eliminated because the E665AE1984A and E665AE1984V double mutants did not enhance both factor VIII and factor VIIIa stability as compared with each single mutant. Results using D519AE665VE1984V were excluded for the same reasons as observed for D519VE665A.
The first group of new mutants (Group A), which combined mutation (Ala or Val) at Asp519 with mutation at either Glu665 or Glu1984, retained normal values for specific activity (>80% the wild type (WT) value,
Interestingly, the enhancement of stability observed for the combination of mutations was more easily observed for the factor VIIIa forms (
A thrombin generation assay was performed on selected mutants and the results are shown in
The E113A mutation is known to enhance factor VIII specific activity as judged by a one-stage clotting assay (U.S. patent application Ser. No. 10/581,471 to Fay et al.; Wakabayashi et al., “A Glu113Ala Mutation within a Factor VIII Ca(2+)-Binding Site Enhances Cofactor Interactions in Factor Xase,” Biochemistry 44:10298-10304 (2005), each of which is hereby incorporated by reference in its entirety). Since the generation of factor VIII with both high stability and high specific activity represents a unique class of reagents for potential therapeutic application in the treatment of hemophilia, the effect of combined mutation of E113A with the high stability mutants described in the preceding Examples was analyzed.
Ala or Val mutants at Asp519, Glu665, and Glu1984 were prepared in combination with the E113A mutation using the same procedures described in the Materials and Methods. These double mutants (amino acids are identified using the single letter code) include: E113AD519A, E113AD519V, E113AE665A, E113AE665V, and E113AE1984V.
Specific activity values determined using the one-stage assay for the combined mutants were ˜2 to ˜3.3 fold higher than WT factor VIII while keeping the normal level of activity by two-stage assay. These results indicate that mutations at Asp519, Glu665, or Glu1984 did not adversely affect the activity enhancement observed for the E113A mutation (
From the foregoing results, the mutation of E113A can be combined with any of the currently described increased stability mutations for the purpose of generating a recombinant factor VIII characterized by both increased specific activity and enhanced factor VIII/factor VIIIa stability. This includes the combination of E113A (or other suitable E113 substitutions as described in U.S. patent application Ser. No. 10/581,471 to Fay et al., which is hereby incorporated by reference in its entirety) with single or multiple stability-enhanced mutants of the type described herein.
Although preferred embodiments have been depicted and described in detail herein, it will be apparent to those skilled in the relevant art that various modifications, additions, substitutions, and the like can be made without departing from the spirit of the invention and these are therefore considered to be within the scope of the invention as defined in the claims which follow.
Claims
1. An isolated nucleic acid molecule encoding a recombinant factor VIII, wherein said recombinant factor VIII comprises one or more mutations that result in enhanced stability of both factor VIII and factor VIIIa, wherein the one or more mutations comprise substitution of one or more charged amino acid residues with a hydrophobic amino acid residue at either or both of the A1 A2 or A2A3 domain interfaces.
2. The isolated nucleic acid molecule according to claim 1, wherein the one or more mutations comprise a substitution of a Glu287 residue of wildtype factor VIII, a substitution of an Asp302 residue of wildtype factor VIII, a substitution of an Asp519 residue of wildtype factor VIII, a substitution of a Glu665 residue of wildtype factor VIII, a substitution of a Glu1984 residue of wildtype factor VIII, or combinations thereof.
3. The isolated nucleic acid molecule according to claim 2, wherein the substitution of the Asp302 residue is D302A.
4. The isolated nucleic acid molecule according to claim 2, wherein the substitution of the Glu287 residue is E287A.
5. The isolated nucleic acid molecule according to claim 2, wherein the substitution of the Glu665 residue is E665A or E665V.
6. The isolated nucleic acid molecule according to claim 2, wherein the substitution of the Asp519 residue is D519A or D519V.
7. The isolated nucleic acid molecule according to claim 2, wherein the substitution of the Glu1984 residue is E1984A or E1984V.
8. The isolated nucleic acid molecule according to claim 1, wherein the one or more mutations comprise two or more substitutions selected from the Glu665 residue, the Asp519 residue, and the Glu1984 residue.
9. The isolated nucleic acid molecule according to claim 8, wherein the two or more substitutions include D519V/E665V, D519A/E665V, D519V/E1984A, E665V/E1984A, E665A/E1984V, D519A/E665V/E1984A, D519V/E665V/E1984A, or D519V/E665V/E1984V.
10. The isolated nucleic acid molecule according to claim 1, wherein the recombinant factor VIII further comprises one or more of (i) factor IXa and/or factor X binding domains modified to enhance the affinity of the recombinant factor VIII for one or both of factor IXa and factor X; (ii) modified sites that enhance secretion in culture; (iii) modified serum protein binding sites that enhance the circulating half-life thereof; (iv) at least one glycosylation recognition sequence that is effective in decreasing antigenicity and/or immunogenicity thereof; and (v) a modified calcium-binding site that improves activity of the recombinant factor VIIIa.
11. The isolated nucleic acid molecule according to claim 1, wherein the nucleic acid is RNA.
12. The isolated nucleic acid molecule according to claim 1, wherein nucleic acid is DNA.
13. The isolated nucleic acid molecule according to claim 1, wherein the one or more charged amino acid residues is not interdomain hydrogen bonded.
14. A recombinant expression system comprising a DNA molecule of claim 12.
15. The recombinant expression system according to claim 14, wherein the recombinant expression system is a viral vector.
16. The recombinant expression system according to claim 15, wherein the viral vector is an adeno-associated viral vector.
17. A recombinant host cell comprising the isolated nucleic acid molecule according to claim 1.
18. The recombinant host cell according to claim 17, wherein the recombinant host cell is a dermal fibroblast.
19. An implantable device comprising a plurality of the recombinant host cells according to claim 17 contained within the device.
20. A recombinant host cell comprising a DNA molecule of claim 12.
21. A method of treating an animal for hemophilia A, said method comprising:
- administering to an animal exhibiting hemophilia A an effective amount of the nucleic acid molecule of claim 1, whereby the animal expresses the recombinant factor VIII and exhibits effective blood clotting following vascular injury.
22. The method according to claim 21, wherein said animal is a mammal.
23. The method according to claim 22, wherein said mammal is selected from the group consisting of human, rat, mouse, guinea pig, dog, cat, monkey, chimpanzee, orangutan, cow, horse, sheep, pig, goat, rabbit, and chicken.
24. The method according to claim 21, wherein said nucleic acid molecule comprises a viral vector.
25. The method according to claim 24, wherein said viral vector is an adeno-associated viral vector.
26. A method of treating an animal for hemophilia A, said method comprising:
- administering to an animal exhibiting hemophilia A a recombinant host cell of claim 17, whereby the animal expresses the recombinant factor VIII and exhibits effective blood clotting following vascular injury.
27. The method according to claim 26, wherein said administering comprises:
- implanting into the animal a device containing a plurality of said recombinant host cells.
28. The method according to claim 26, wherein the recombinant host cell is a dermal fibroblast.
29. The method according to claim 26, wherein said animal is a mammal.
30. The method according to claim 29, wherein said mammal is selected from the group consisting of human, rat, mouse, guinea pig, dog, cat, monkey, chimpanzee, orangutan, cow, horse, sheep, pig, goat, rabbit, and chicken.
31. An isolated nucleic acid encoding a recombinant factor VIII comprising one or more mutations that result in enhanced stability of both factor VIII and factor VIIIa, wherein the one or more mutations are selected from the group consisting of substitution of a Glu residue with a hydrophobic amino acid residue at a position corresponding to amino acid 287, 665, and/or 1984 of SEQ ID NO: 2, substitution of an Asp residue with a hydrophobic amino acid residue at a position corresponding to amino acid 302 and/or 519 of SEQ ID NO: 2, and combinations of two or more of said substitutions, and wherein the position of the substitution or substitutions of said recombinant factor VIII aligns with amino acids 287, 302, 519, 665, and/or 1984 of SEQ ID NO: 2 upon alignment of the amino acid sequence of the recombinant factor VIII with the amino acid sequence of SEQ ID NO: 2.
32. The isolated nucleic acid molecule according to claim 31, wherein nucleic acid is DNA.
33. A recombinant expression system comprising a DNA molecule of claim 32.
34. A recombinant host cell comprising the isolated nucleic acid molecule according to claim 31.
35. A method of treating an animal for hemophilia A, said method comprising:
- administering to an animal exhibiting hemophilia A an effective amount of the nucleic acid molecule of claim 31, whereby the animal expresses the recombinant factor VIII and exhibits effective blood clotting following vascular injury.
36. A method of treating an animal for hemophilia A, said method comprising:
- administering to an animal exhibiting hemophilia A a recombinant host cell of claim 34, whereby the animal expresses the recombinant factor VIII and exhibits effective blood clotting following vascular injury.
Type: Application
Filed: Oct 11, 2013
Publication Date: Feb 27, 2014
Applicant: University of Rochester (Rochester, NY)
Inventors: Philip J. Fay (Pittsford, NY), Hironao Wakabayashi (Rochester, NY)
Application Number: 14/052,452
International Classification: C12N 15/86 (20060101); A61K 35/12 (20060101);