Modified Latency Associated Protein Construct

Abstract

The present invention provides a fusion protein comprising a latency associated peptide (LAP), a pharmaceutically active agent and an amino acid sequence comprising a dimerisation domain, wherein the LAP and the pharmaceutically active agent are connected by an amino acid sequence comprising a proleolytic cleavage site. Also provided are nucleic acids enclosing such fusion proteins, process for their preparation, pharmaceutical compositions, kits and uses thereof in medicine.

Description

The present invention relates to the use of proteins, protein derivatives and DNA constructs that confer latency to pharmaceutically active agents. The present invention also relates to improved methods of providing latency to pharmaceutically active agents.

Most cytokines and growth factors are expressed under tight control mechanisms. Their gene expression is regulated by environmental stimuli such as infection, cell-cell interactions, change in extracellular matrix composition and interactions with adhesion molecules or via stimulation with other cytokines.

In addition to the control at the transcriptional and post-transcriptional level, some cytokines are not released into the medium unless a second signal activates the cell. A third level of regulation for cytokine activity is found in molecules which are secreted in a latent form and become “activated” by releasing the cytokine moiety where processes of inflammation, wound healing and tissue repair takes place (Khalil N, Microbes and Infection, 1, 1255-1263 (1999). In this latter respect, transforming growth factor beta (TGFβ) has received greatest attention.

TGFβ is synthesized as a dimeric latent cytokine composed of an amino terminal latency associated protein (LAP) and the active TGFβ cytokine at its COOH terminal end (Roberts and Sporn, Peptide Growth Factors and their Receptors: Sporn, M B and Roberts, AB, Springer-Verlag, 419-472 (1996); Roth-Eicchorn et al., Hepatology, 28 1588-1596 (1998)). The precursor peptide contains a signal peptide (residues 1-29) necessary for protein secretion and guiding the molecule through the Golgi apparatus to become processed by proteolytic cleavage and glycosylation. The LAP domain is separated from TGFβ by proteolytic cleavage at arginines (277-278). Mature TGFβ begins at alanine 279. The LAP, in addition to protect TGFβ, contains important residues necessary for the interaction with other molecules. Mutations in the LAP domain have recently been associated with the autosomal dominant Camurati-Engelmann disease (Janssens et al., Nature Genetics, 26, 273-275 (2000). Cysteines 224 and 226 are important in the intermolecular disulphide bond between two LAPs. Their mutation to serine renders the molecule “active” (Sanderson et al., Proc. Natl. Acad. Sci. USA, 92, 2572-2576 (1995); Brunner et al., Mol. Endocrinol. 6, 1691-1700 (1992); Brunner et al., J. Biol. Chem, 264, 13660-13664 (1989)). The RGD motif (245-247) facilitates the interaction with integrins (Munger et al., Mol, Biol. of the Cell, 9, 2627-2638 (1998; Derynck R, TIBS, 19, 548-553 (1994)). Nucleic acid encoding TGFβ is described in U.S. Pat. No. 5,801,231.

In most cell types studied, including those of mesenchymal, epithelial and endothelial origin, TGFβ is secreted in a latent form consisting of TGFβ and its latency associated peptide (LAP) propeptide dimers, covalently linked to latent TGFβ-binding proteins (LTBPs). LTBPs are also needed for the secretion and folding of TGFβ (Miyazano et al., EMBO J. 10, 1091-1101 (1991); Miyazano et al., J. Biol. Chem. 267, 5668-5675 (1992); Eklov et al., Cancer Res. 53, 3193-3197 (1993)). Cysteine 33 is important for the disulphide bridge with the third 8 cysteine-rich repeat of latent TGFβ binding protein (LTBP) (Saharinen et al., The EMBO Journal, 15, 245-253 (1996). Modification of LTBP by enzymes such as thrombospondin (Schultz et al., The Journal of Biological Chemistry, 269, 26783-26788 (1994); Crawford et al., Cell, 93, 1159-1170 (1998)), transglutaminase (Nunes et al., J. Cell, Biol. 136, 1151-1163 (1997); Kojima et al., The Journal of Cell Biology, 121, 439-448 (1993)) and MMP9, MMP2 (Yu and Stamenkovic, Genes and Dev, 14, 163-176 (2000)) could release the active portion of TGFβ from the latent complex.

Cytokines are natural products serving as soluble local mediators of cell-cell interactions. They have a variety of pleiotropic actions, some of which can be harnessed for therapeutic purposes. Targeting of cytokines to specific cell types using scFv (Lode et al., Pharmacol. Ther, 80, 277-292 (1998)) and vWF (Gordon et al., Human Gene Therapy, 8, 1385-1394 (1997)) have focused entirely on the active cytokine moiety of the cytokine complex.

Pharmacologically active proteins or other medicines based on such agents, which have to be administered at very high concentrations systemically in order to achieve biologically effective concentrations in the tissue being targeted, tend to give rise to undesirable systemic effects, for example toxicity, which limit their use and efficacy.

The principles underlying the construction of such a system for providing latency to pharmaceutically active agents using the LAP of TGF-β was described in WO 02/055098 and WO 2009/077755. In the naturally occurring LAP-TGF-β complex, the latency associated peptide forms a protective shell around TGF preventing it from being degraded. The closed nature of the shell is guaranteed because of internal interactions between TGF with LAP. These interactions are not necessarily expected when the ‘payload’ is another cytokine, growth factor or peptide or pharmaceutically active compound, and may result in a permeable shell which allows entry of mobile target molecules into the shell. For example, if the target molecule is a soluble receptor, the receptor may be able to enter the shell and interact with the pharmaceutically active agent even when the pharmaceutically active agent is bound to the LAP. This could lead to off-site activity which may have undesirable side effects. Furthermore, while improving protein production utilizing suspension cell cultures according to WO 2009/077755, the inventors found that, along with dimers, the LAP fusion proteins also tended to form active monomers.

The present inventors have now developed an improved means for providing pharmaceutically active agents in latent form based on this system.

According to the first aspect of the invention there is provided a fusion protein comprising a latency associated peptide (LAP), a pharmaceutically active agent and an amino acid sequence comprising a dimerisation domain wherein the LAP and pharmaceutically active agent are connected by an amino acid sequence comprising a proteolytic cleavage site.

The fusion protein comprising a LAP, a proteolytic cleavage site, a pharmaceutically active agent and a dimerisation domain may provide for site specific activation of the latent pharmaceutically active agent. The term “site specific activation” as used herein means, in general terms and not limited to the removal or reduction of latency, conferred on a pharmaceutically active agent, by site-specific cleavage at the proteolytic cleavage site.

Site-specific cleavage at the proteolytic cleavage site is expected to take place concomitantly with the restored activation of the pharmaceutically active agent.

The term “latent pharmaceutically active agent” as used herein may include, but is not limited to, pharmaceutically active agents which are latent due to their association with LAP and a proteolytic cleavage site. Specifically, the pharmaceutically active agent may be latent by virtue of its fusion to a LAP associated proteolytic cleavage site to form a latent fusion protein. The pharmaceutically active agent may be of natural or synthetic origin.

The fusion protein may be constructed as shown in FIG. 4(c) in which the dimerisation domain is fused to the LAP. An additional proteolytic cleavage site and/or linker sequence may be inserted also between the dimerisation domain and the LAP. A secretory signal peptide (i.e. the precursor peptide) may be fused to the dimerisation domain also at the N-terminal of the dimerisation domain.

The term “protein” in this text means, in general terms, a plurality of amino acid residues joined together by peptide bonds. It is used interchangeably and means the same as peptide, oligopeptide, oligomer or polypeptide, and includes glycoproteins and derivatives thereof. The term “protein” is also intended to include fragments, analogues and derivatives of a protein wherein the fragment, analogue or derivative retains essentially the same biological activity or function as a reference protein.

The fragment, analogue or derivative of the protein as defined in this text, may be at least 6, preferably 10 or 20, or up to 50 or 100 amino acids long.

The fragment, derivative or analogue of the protein may be (i) one in which one or more of the amino acid residues are substituted with a conserved or non-conserved amino acid residue (preferably, a conserved amino acid residue) and such substituted amino acid residue may or may not be one encoded by the genetic code, or (ii) one in which one or more of the amino acid residues includes a substituent group, or (iii) one in which the mature polypeptide is fused with another compound, such as a compound to increase the half life of the polypeptide (for example, polyethylene glycol), or (iv) one in which the additional amino acids are fused to the mature polypeptide, such as a leader or secretory sequence which is employed for purification of the polypeptide. Such fragments, derivatives and analogues are deemed to be within the scope of those skilled in the art from the teachings herein.

Particularly preferred are variants, analogues, derivatives and fragments having the amino acid sequence of the protein in which several e.g. 5 to 10, or 1 to 5, or 1 to 3, 2, 1 or no amino acid residues are substituted, deleted or added in any combination. Especially preferred among these are silent substitutions, additions and deletions, which do not alter the properties and activities of the protein of the present invention. Also especially preferred in this regard are conservative substitutions.

An example of a variant of the present invention is a fusion protein as defined above, apart from the substitution of one or more amino acids with one or more other amino acids. The skilled person is aware that various amino acids have similar properties. One or more such amino acids of a substance can often be substituted by one or more other such amino acids without eliminating a desired activity of that substance.

Thus the amino acids glycine, alanine, valine, leucine and isoleucine can often be substituted for one another (amino acids having aliphatic side chains). Of these possible substitutions it is preferred that glycine and alanine are used to substitute for one another (since they have relatively short side chains) and that valine, leucine and isoleucine are used to substitute for one another (since they have larger aliphatic side chains which are hydrophobic). Other amino acids which can often be substituted for one another include: phenylalanine, tyrosine and tryptophan (amino acids having aromatic side chains); lysine, arginine and histidine (amino acids having basic side chains); aspartate and glutamate (amino acids having acidic side chains); asparagine and glutamine (amino acids having amide side chains); and cysteine and methionine (amino acids having sulphur containing side chains).

Substitutions of this nature are often referred to as “conservative” or “semi-conservative” amino acid substitutions.

Amino acid deletions or insertions may also be made relative to the amino acid sequence for the fusion protein referred to above. Thus, for example, amino acids which do not have a substantial effect on the activity of the polypeptide, or at least which do not eliminate such activity, may be deleted. Such deletions can be advantageous since the overall length and the molecular weight of a polypeptide can be reduced whilst still retaining activity. This can enable the amount of polypeptide required for a particular purpose to be reduced—for example, dosage levels can be reduced.

Amino acid insertions relative to the sequence of the fusion protein above can also be made. This may be done to alter the properties of a substance of the present invention (e.g. to assist in identification, purification or expression, as explained above in relation to fusion proteins).

Amino acid changes relative to the sequence for the fusion protein of the invention can be made using any suitable technique e.g. by using site-directed mutagenesis. It should be appreciated that amino acid substitutions or insertions within the scope of the present invention can be made using naturally occurring or non-naturally occurring amino acids. Whether or not natural or synthetic amino acids are used, it is preferred that only L-amino acids are present.

A protein according to the invention may have additional N-terminal and/or C-terminal amino acid sequences. Such sequences can be provided for various reasons, for example, glycosylation.

The term “fusion protein” in this text means, in general terms, one or more proteins joined together by chemical means, including hydrogen bonds or salt bridges, or by peptide bonds through protein synthesis or both.

The latency associated peptide (LAP) of the present invention may include, but is not limited to, the coding sequence for the precursor domain of TGFβ or a sequence which is substantially identical thereto.

“Identity” as known in the art is the relationship between two or more polypeptide sequences or two or more polynucleotide sequences, as determined by comparing the sequences. In the art, identity also means the degree of sequence relatedness (homology) between polypeptide or polynucleotide sequences, as the case may be, as determined by the match between strings of such sequences. While there exist a number of methods to measure identity between two polypeptide or two polynucleotide sequences, methods commonly employed to determine identity are codified in computer programs. Preferred computer programs to determine identity between two sequences include, but are not limited to, GCG program package (Devereux, et al., Nucleic acids Research, 12, 387 (1984), BLASTP, BLASTN, and FASTA (Atschul et al., J. Molec. Biol. 215, 403 (1990).

The LAP of the present invention may comprise the precursor domain of TGFβ, for example, the precursor peptide of TGFβ-1, 2 or 3 (from human) (Derynck et al., Nature, 316, 701-705 (1985); De Martin et al., EMBO J. 6 3673-3677 (1987); Hanks et al., Proc. Natl. Acad. Sci. 85, 79-82 (1988); Derynck et al., EMBO J. 7, 3737-3743 (1988); Ten Dyke et al., Proc. Natl. Acad. Sci. USA, 85, 4715-4719 (1988)) TGFβ-4 (from chicken) (Jakowlew et al., Mol. Endocrinol. 2, 1186-1195 (1988)) or TGFβ-5 (from xenopus) (Kondaiah et al., J. Biol. Chem. 265, 1089-1093 (1990)). The term “precursor domain” is defined as a sequence encoding a secretory signal peptide (i.e. a precursor peptide) which does not include the sequence encoding the mature protein. The amino acid sequences of the precursor domain of TGFβ1, 2, 3, 4 and 5 (Roberts and Sporn, Peptide Growth Factors and their Receptors: Sporn, M B and Roberts, AB, Springer-Verlag, Chapter 8, 422 (1996)) are shown in FIG. 1.

Preferably, the amino acid sequence of the LAP has at least 50% identity, using the default parameters of the BLAST computer program (Atschul et al., J. Mol. Biol. 215, 403-410 (1990) provided by HGMP (Human Genome Mapping Project), at the amino acid level, to the precursor domain of TGFβ1, 2, 3, 4 or 5 (Roberts and Sporn, Peptide Growth Factors and their Receptors: Sporn, M B and Roberts, AB, Springer-Verlag, Chapter 8, 422 (1996)) as shown in FIG. 1. More preferably, the LAP may have at least 60%, 70%, 80%, 90% and still more preferably 95% (still more preferably at least 99%) identity, at the nucleic acid or amino acid level, to the precursor domain of TGFβ1, 2, 3, 4 or 5 as shown in FIG. 1 which comprises residues 1 to 278.

The LAP may comprise the LAP of TGFβ1, 2, 3, 4, or 5 (Roberts and Sporn, Peptide Growth Factors and their Receptors: Sporn, M B and Roberts, AB, Springer-Verlag, Chapter 8, 422 (1996)) as shown in FIG. 1.

The LAP may contain at least two, for example at least 4, 6, 8, 10 or 20 cysteine residues for the formation of disulphide bonds.

The LAP may also comprise a sequence which has at least 50%, 60%, 70%, 80%, 90%, 95% or 99% identity with a LAP sequence of FIG. 1, using the default parameters of the BLAST computer program provided by HGMP, thereto.

The “dimerisation domain” refers to a peptide having affinity for a second peptide, such that the two peptides associate under physiological conditions to form a dimer. The second peptide may be the same or a different peptide. The dimerisation domain may also refer to polypeptides. The peptides or polypeptides may interact with each other through covalent and/or non-covalent association(s).

The dimerisation domain may be linked to the latency associated peptide by a linker. The linker size can be varied to vary the size of the shell in order to accommodate the pharmaceutically active agent. The linker peptide may comprise the amino acid sequence GGGGS (SEQ ID NO:135) or a multimer thereof (for example a dimer, a trimer, or a tetramer), a suitable linker may be (GGGGS)₃ (SEQ ID NO:136), or a sequence of nucleotides which has at least 50%, 60%, 70%, 80%, 90%, 95% or 99% identity, using the default parameters of the BLAST computer program provided by HGMP, thereto.

Examples of dimerisation domains include antibody fragment polypeptides such as an immunoglobulin Fc polypeptide, an immunoglobulin hinge polypeptide, a CH3 domain polypeptide, a CH4 domain polypeptide, a CH1 domain or CL domain polypeptide; a leucine zipper domain (e.g., a jun/fos leucine zipper domain, see, e.g., Kostelney et al., J. Immunol., 148:1547-1553, 1992; or a yeast GCN4 leucine zipper domain); an isoleucine zipper domain; a dimerising region of a dimerising cell-surface receptor (e.g., interleukin-8 receptor (IL-8R); or an integrin heterodimer such as LFA-1 or GPIllb/111a); a dimerising region of a secreted, dimerising ligand (e.g., nerve growth factor (NGF), neurotrophin-3 (NT-3), interleukin-8 (IL-8), vascular endothelial growth factor (VEGF), or brain-derived neurotrophic factor (BDNF); see, e.g., Arakawa et al., J. Biol. Chem. 269:27833-27839, 1994, and Radziejewski et al., Biochem. 32:1350, 1993); or a polypeptide comprising at least one cysteine residue (e.g., one, two, or three to about ten cysteine residues) such that disulfide bond(s) can form between the polypeptide and a second polypeptide comprising at least one cysteine residue. Suitably the dimerisation domain may be an Fc polypeptide.

An immunogobulin hinge polypeptide typically comprises a region which is rich in proline and cysteine amino acid residues. A common sequence motif present in the hinge polypeptide region may be may be CPXCP (SEQ ID NO:137) where X can be another residue that does not interfere with dimerisation, for example proline (P), arginine (R) or serine (S). The hinge region polypeptide may be from around 10 to 75 amino acid residues. The hinge region polypeptide may contain a plurality of cysteine-cysteine disulphide bonds, for example of from 2 to 15. The hinge region polypeptide may comprise the sequence CPXCP where X can be another residue that does not interfere with dimerisation, for example proline (P), arginine (R) or serine (S). A number of repeats of the sequence CPXCP may be present also, for example 2, 3, 4, or 5 repeats, or greater.

Wypych et al., J. Biol. Chem. 28316194-16205, 2008 defined the following hinge region peptide sequences for IgG antibodies as shown in Table 1 below:

TABLE 1
IgG subtype Core hinge sequences
IgG1        EPKSCDKTHTCPPCP (SEQ ID NO: 138)
IgG2        ERKCCVECPPCP (SEQ ID NO: 139)
IgG3        ELKTPLGDTTHTCPRCP (SEQ ID NO: 140)
            (EPKSCDTPPPCPRCP)3 (SEQ ID NO: 141)
IgG4        ESKYGPPCPSCP (SEQ ID NO: 142)

The terms “antibody” and “immunoglobulin” are used herein interchangeably. An antibody molecule is made up of two identical heavy (H) and two identical light (L) chains held together by disulphide bonds. Each heavy chain comprises an Fc polypeptide. The two Fc polypeptides from the two heavy chains dimerise to form the Fc region of the antibody molecule. The term “Fc region” refers to the constant region of an antibody excluding the first constant region immunoglobulin domain of the heavy chain (CH1) that interacts with the constant portion of the light chain (CL) forming a CH1-CL domain pair. Thus, Fc region comprises the last two constant region immunoglobulin domains (CH2 and CH3) of IgA, IgD, and IgG, and the last three constant region immunoglobulin domains of IgE and IgM (CH2, CH3 and CH4), Any polypeptide of the various immunoglobulin constant domains may therefore be used in accordance with the present invention as a dimerisation domain.

Several antibody effector functions are mediated through the binding of the Fc region to Fc receptors (FcR) found on the surface of many cells for example lymphocytes, macrophages, natural killer cells, etc. FcRs are defined by their specificity for antibody isotypes. For example, Fc receptors for IgG antibodies are referred to as FcγR.

IgG is also bound by the neonatal Fc receptor (FcRn). In humans, IgG exhibits a long serum half-life. Studies indicate that this is due to the protective effect of FcRn which binds to the Fc region of IgG and prevents degradation by allowing intracellular recycling.

The Fc polypeptide may be selected to alter, e.g. increase or decrease the half-life of the fusion protein. As used herein, the term “half-life” refers to a biological half-life of a particular polypeptide or protein in vivo. Half-life may be represented by the time required for half the quantity administered to a subject to be cleared from the circulation and/or other tissues in the animal. In an embodiment of the invention the Fc polypeptide is an IgG Fc polypeptide.

IgG antibodies can be further subdivided into IgG1, IgG2, IgG3 and IgG4. In an embodiment of the invention the Fc polypeptide may be IgG1, IgG2, IgG3 and IgG4 polypeptide, for example an IgG1 polypeptide.

The Fc polypeptide may be selected to target the fusion protein to specific tissues, for example the mucosa. The IgA antibody plays an important role in mucosal immunity for e.g. in the respiratory tract and the gastrointestinal mucosal lining. In its secretory form, IgA is found in mucous secretions such as tears, saliva, colostrum, gastrointestinal and genitourinary fluids. IgA deficiency is associated with a number of autoimmune diseases such as rheumatoid arthritis, systemic lupus erythematosus and immune thrombocytopenic purpura. IgA deficiency is also associated with allergic diseases such as asthma. In another embodiment of the invention the Fc polypeptide may be an IgA polypeptide.

The Fc polypeptides may be derived from the same antibody isotype to form a homodimeric Fc region or from different antibody isotypes to form a heterodimeric Fc region. The Fc polypeptide may be a naturally occurring polypeptide or may be an engineered polypeptide.

The LAP may provide a protective “shell” around the pharmaceutically active agent thereby shielding it and hindering, or preventing, its interaction with other molecules in the cell surface or molecules important for its activity.

The dimerisation domain enables the fusion of the amino terminals of two latency associated proteins thereby effectively closing the LAP shell. The dimerisation domains are therefore complementary and permit dimerisation to occur. The closure of the shell does not depend on the interaction of LAP with the pharmaceutically active agent. The closure also prevents monomer formation of the LAP fusion proteins.

Closure of the shell also prevents any interaction between the pharmaceutically active agent and its target molecule unless the pharmaceutically active agent is released from the LAP fusion protein by proteolytic activity. This ensures site-specific delivery of the pharmaceutically active agent and may reduce off-site activity.

In one alternative embodiment of the invention, therefore, there is provided a protein construct comprising two fusion proteins as defined in the first aspect of the invention which are present as a dimer. The dimer is composed of monomers of the first aspect of the invention which may be the same or different with respect to the latency associated peptide (LAP), the pharmaceutically active agent, and the amino acid sequence comprising a proteolytic cleavage site.

The dimer may therefore be composed of a first monomer and a second monomer, in which the first monomer comprises a latency associated peptide (LAP), a pharmaceutically active agent and an amino acid sequence comprising a dimerisation domain wherein the LAP and pharmaceutically active agent are connected by an amino acid sequence comprising a proteolytic cleavage site, and a second monomer comprising a latency associated peptide (LAP), a pharmaceutically active agent and an amino acid sequence comprising a dimerisation domain wherein the LAP and pharmaceutically active agent are connected by an amino acid sequence comprising a proteolytic cleavage site.

The present invention therefore provides a composition comprising two fusion proteins according to the first aspect, wherein the fusion proteins are associated at the dimerisation domain in each fusion protein.

The proteolytic cleavage site may comprise any protease specific cleavage site. The proteolytic cleavage site may include, but is not limited to, a matrix metalloproteinase (MMP) cleavage site, a serine protease cleavage site, an aggrecanase cleavage site, a site cleavable by a parasitic protease derived from a pathogenic organism (Zhang et al., J. Mol. Biol. 289, 1239-1251 (1999); Voth et al., Molecular and Biochemical Parasitology, 93, 31-41 (1998); Yoshioka et al., Folia Pharmacologica Japonica, 110, 347-355 (1997); Tort et al, Advances in Parasitology, 43, 161-266 (1999); McKerrow, International Journal for Parasitology, 29, 833-837 (1999); Young et al., International Journal for Parasitology, 29, 861-867 (1999); Coombs and Mottram, Parasitology, 114, 61-80 (1997)) or a site cleavable by the proteins of the complement cascade (Carroll, Annu. Rev. Immunol. 16, 545-568 (1998); Williams et al., Ann. Allergy, 60, 293-300 (1988)).

Suitably, the proteolytic cleavage site of the fusion proteins of the present invention is cleaved when the fusion protein is located at or introduced to a site of disease diagnosed as an inflammatory condition, e.g. arthritis, or cancer which can be characterized by inflammation and/or tissue remodelling.

A MMP cleavage site may comprise a number of amino acid residues recognisable by MMP. Preferably, the MMP cleavage site comprises the minimum number of amino acid residues required for recognition and cleavage by MMP. Moreover, the amino acids of the MMP site may be linked by one or more peptide bonds which are cleavable, proteolytically, by MMP. MMPs which may cleave the MMP site include, but are not limited to, MMP1, MMP2, MMP3, MMP7, MMP8, MMP9, MMP10 and MMP13 (Yu and Stamenkovic, Genes and Dev. 14, 163-176 (2000); Nagase and Fields, Biopolymers, 40, 399-416 (1996); Massova et al., J. Mol. Model. 3, 17-30 (1997); reviewed in Vu and Werb; Genes and Dev. 14, 2123-2133 (2000)).

The MMP cleavage site e.g. any one or more of MMP1, MMP2, MMP3, MMP7, MMP8, MMP9 or MMP10 may be as shown in FIG. 2 or a sequence of amino acids which has at least 50%, 60%, 70%, 80%, 90%, 95% or 99% identity with the sequences shown in FIG. 2, using the default parameters of the BLAST computer program provided by HGMP, thereto. In an embodiment the MMP proteolytic cleavage site has the amino acid sequence PLGLWA.

The proteolytic cleavage site may also comprise any aggrecanase specific cleavage site which is cleavable by an aggrecanase. An aggrecanase cleavage site may comprise a number of amino acid residues recognisable by an aggrecanase. Moreover, the amino acids of the aggrecanase site may be linked by one or more peptide bonds which are cleavable, proteolytically, by aggrecanase.

Aggrecanases which may cleave the aggrecanase site include, but are not limited to ADAMTS-4 (aggrecanase-1), ADAMTS-5 (aggrecanase-2) and ADAMTS-11 (Tortorella, M. D., et al Osteoarthritis Cartilage, 2001. 9(6): p. 539-552); Abbaszade, I., et al J Biol Chem, 1999. 274(33): p. 23443-23450).

The sequences of the protein cleavage sites of ADAMTS-4 (aggrecanase-1) are shown in FIG. 3. Suitable ADAMTS-4 sites include:

(SEQ ID NO: 80)
HNEFRQRETYMVF
(SEQ ID NO: 97)
DVQEFRGVTAVIR

The consensus ADAMTS-4 cleavage motif can be represented according to Hills et al (J. Biol. Chem. 282 11101-11109 (2007)) as:

(SEQ ID NO: 129)
E-[AFVLMY]-X-(0,1)-[RK]-X(2,3)-[ST]-[VYIFWMLA]

The aggrecanase proteolytic cleavage site of the present invention may be cleaved by ADAMTS-4 (aggrecanase-1), ADAMTS-5 (aggrecanase-2) or ADAMTS-11.

The amino acid sequence of the aggrecanase cleavage site may include a sequence which has at least 50%, 60%, 70%, 80%, 90%, 95% or 99% identity, using the default parameters of the BLAST computer program provided by HGMP, thereto. Preferably, the nucleic acid sequence encoding the aggrecanase cleavage site comprises the minimum number of residues required for recognition and cleavage by an aggrecanase.

The present invention may further provide a “linker” peptide. Preferably the linker peptide is linked to the amino acid sequence of the proteolytic cleavage site. The linker peptide may be provided at the C terminal or N terminal end of the amino acid sequence encoding the proteolytic cleavage site. Preferably, the linker peptide is continuous with the amino acid sequence of the proteolytic cleavage site. The linker peptide may comprise the amino acid sequence GGGGS (SEQ ID NO:135) or a multimer thereof (for example a dimer, a trimer, or a tetramer), a suitable linker may be (GGGGS)₃ (SEQ ID NO:136), or a sequence of nucleotides which has at least 50%, 60%, 70%, 80%, 90%, 95% or 99% identity, using the default parameters of the BLAST computer program provided by HGMP, thereto.

The term “linker peptide” is intended to define any sequence of amino acid residues which preferably provide a hydrophilic region when contained in an expressed protein. Such a hydrophilic region may facilitate cleavage by an enzyme at the proteolytic cleavage site.

The constructs of the invention may also comprise an additional linker sequence and/or proteolytic cleavage site between the dimerisation domain and the LAP.

The term “latency” as used herein, may relate to a shielding effect which may hinder interaction between the fusion protein and other molecules in the cell surface. Alternatively the term latency may be used to describe a reduction in the activity (up to and including ablation of activity) of a molecule/agent associated with the fusion protein. The term latency may also relate to a stabilising effect of the fusion protein. The effect may be in full or partial, where a partial effect is sufficient to achieve the latency of the active agent.

The term “associating with” in the context of the present invention is intended to include all means of association including, but not limited to, chemical cross-linking or peptide bond linkage.

The pharmaceutically active agent may be a pharmaceutically active protein which can include, but is not limited to, an antibody, a growth factor (e.g. TGFβ, epidermal growth factor (EGF), platelet derived growth factor (PDGF), nerve growth factor (NGF), colony stimulating factor (CSF), hepatocyte growth factor, insulin-like growth factor, placenta growth factor); a differentiation factor; a cytokine e.g. an interleukin, (e.g. IL1, IL-2, IL-3, IL-4, IL-5, IL-6, IL-7, IL-8, IL-9, IL-10, IL-11, IL-12, IL-13, IL-14, IL-15, IL-16, IL-17, IL-18, IL-19, IL-20, IL-21, IL-22, IL-23, IL-24, IL-25, IL-26, IL-27, IL-28, IL-29, IL-30, IL-31, IL-32 or IL-33 or an interferon (e.g. IFN-α, IFN-β and IFN-γ), tumour necrosis factor (TNF), IFN-γ inducing factor (IGIF), a bone morphogenetic protein (BMP, e.g. BMP-1, BMP-2, BMP-3, BMP-4, BMP-4, BMP-5, BMP-6, BMP-7, BMP-8, BMP-9, BMP10, BMP-11, BMP-12, BMP-13); an interleukin receptor antagonist (e.g. IL-1 ra, IL-1R11), a tumor necrosis factor inhibitor (TNF-R or anti-TNF); a chemokine (e.g. MIPs (Macrophage Inflammatory Proteins) e.g. MIPla and MIP113; MCPs (Monocyte Chemotactic Proteins) e.g. MCP1, 2 or 3; RANTES (regulated upon activation normal T-cell expressed and secreted)); a trophic factor; a cytokine inhibitor; a cytokine receptor; a free-radical scavenging enzyme e.g. superoxide dismutase or catalase; a pro-drug converting enzyme (e.g. angiotensin converting enzyme, deaminases, dehydrogenases, reductases, kinases, urate oxidase and phosphatases); a peptide mimetic; a protease inhibitor; a tissue inhibitor of metalloproteinases (TIMPs e.g. TIMP1, TIMP2, TIMP3 or TIMP4) or a serpin (inhibitors of serine proteases). Preferably, the pharmaceutically active agent will be derived from the species to be treated e.g. human origin for the treatment of humans.

Preferably, the pharmaceutically active agent may be a cytokine, e.g. IFNβ, IL-4, or IL-1ra, or a cytokine inhibitor, such as an antibody or antibody fragment, e.g. trastuzumab, and as defined herein below.

The interleukins and cytokines may be anti-inflammatory or pro-inflammatory. Anti-inflammatory cytokines and certain interleukins, such as IL-4 and/or IL-10, are suitable for the treatment of arthritis, whereas pro-inflammatory cytokines and other interleukins, such as IL-1 and IL-2, are suitable for the treatment of cancer.

As used herein “peptide mimetics” includes, but is not limited to, agents having a desired peptide backbone conformation embedded into a non-peptide skeleton which holds the peptide in a particular conformation. Peptide mimetics, which do not have some of the drawbacks of peptides, are of interest in those cases where peptides are not suitable in medicine.

Peptide mimetics may comprise a peptide backbone which is of the L- or D-conformation. Examples of peptides mimetics include melanocortin, adrenocorticotrophin hormone (ACTH) and other peptide mimetic agents which play a role in the central nervous system, endocrine system in signal transduction and in infection and immunity.

The pharmaceutically active agent may comprise a chemical compound such as a chemotherapeutic agent or other synthetic drug. Alternatively, the pharmaceutically active agent may comprise an siRNA or a peptide nucleic acid (PNA) sequence e.g. a poly-lysine sequence which binds to nucleic acids and permeabilises lipid bilayers (Wyman et al., Biological Chemistry, 379, 1045-1052 (1998)) or a KALA peptide which facilitates transfer through lipid bilayers (Wyman et al., Biochemistry, 36, 3008-3017 (1997)) or a protein transduction domain (PTD) that enables polypeptides to enter cells via the plasma membrane (Pi et al Molecular Therapy 2, 339-347 (2000)).

The pharmaceutically active agent may be suitable for interacting with soluble target molecules. Examples of soluble target molecules include cytokines, growth factors, signaling proteins and other ligands and receptors.

The pharmaceutically active agent may be a cytokine inhibitor. The term “cytokine inhibitor” refers to a molecule that can block, reduce, inhibit or neutralise a function, an activity and/or the expression of a cytokine. The cytokine inhibitor may be a protein (for example soluble cytokine receptor protein); an antibody or antibody fragment; nucleic acid (for example siRNA or anti-sense nucleic acid) or organic or inorganic molecules.

Examples of suitable antibodies include but are not limited to anti-TNF (e.g. anti-TNF α, anti-TNF β), anti-interleukins (e.g. anti-IL-1, anti-IL-2, anti-IL-3, anti-IL-4, anti-IL-5, anti-II-6, anti-IL-7, anti-IL-8, anti-IL-9, anti-IL-10, anti-IL-11, anti-IL-12, anti-IL-13, anti-IL-14, anti-IL-15, anti-IL-16, anti-IL-17, anti-IL-18, anti-IL-19, anti-IL-20, anti-IL-21, anti-IL-22, anti-IL-23, anti-IL-24, anti-IL-25, anti-IL-26, anti-IL-27, anti-IL-28, anti-IL-29, anti-IL-30, anti-IL-31, anti-IL-32, anti-IL-33, anti-IL-34, anti-IL-35 and IL-36), anti-interferons (e.g. anti-INF-α, anti-INF-β, anti-INF-γ and anti-INF-ω) and fragments thereof.

Examples of such molecules also include trastuzumab (also known as Herclon™/Herceptin™), a monoclonal antibody to the HER2/neu receptor.

The pharmaceutically active agent may be an antibody or an antibody fragment. An “antibody fragment” as referred to herein means any portion of a full length antibody. Examples of antibody fragments include, but are not limited to, Fab, Fab′, F(ab′)2, scFv, Fv, dsFv diabody and Fd fragments.

The term “single chain variable fragment” or “scFv” refers to an Fv fragment in which the heavy chain domain and the light chain domain are linked. One or more scFv fragments may be linked to other antibody fragments (such as the constant domain of a heavy chain or a light chain) to form antibody constructs having one or more antigen recognition sites.

The antibody or antibody fragment may be suitable for use in the treatment of inflammatory conditions such as arthritis, gout, atherosclerosis, allograft rejection, Crohn's disease, inflammatory bowel disease, irritable bowel syndrome and colitis.

In an alternative embodiment, the invention further provides the fusion protein of the present invention optionally in association with latent TGFβ binding protein (LTBP). Typically, the fusion protein is covalently linked to LTBP to form a complex. Preferably, the association is mediated by disulphide bond(s) between Cys No. 33 of LAP and the third 8 Cys residue of LTBP. The LTBP associated with the fusion protein may include, but is not limited to, LTBP 1, 2, 3 or 4 (Kanzaki et al., Cell, 61, 1051-1061 (1990); Tsuji et al., Proc. Natl. Acad. Sci. USA, 87, 8835-8839 (1990); Moren et al., J. Biol. Chem. 269, 32469-32478 (1994); Yin et al., J. Biol. Chem. 270, 10147-10160 (1995); Gibson et al., Mol. Cell. Biol. 15, 6932-6942 (1995); Saharinen et al., J. Biol. Chem. 273, 18459-18469 (1998)), or fragments of LTBP such as that containing the third 8 Cys repeat, or homologues having a sequence of amino acids or nucleotides which has at least 50%, 60%, 70%, 80%, 90%, 95% or 99% identity, using the default parameters of the BLAST computer program provided by HGMP, to that of LTBP.

Cleavage of LTBP may release the fusion protein from the LTBP complex. Enzymes which may cleave LTBP in this manner include, but are not limited to, thrombospondin (Schultz et al., The Journal of Biological Chemistry, 269, 26783-26788 (1994); Crawford et al., Cell, 93, 1159-1170 (1998)), transglutaminase (Nunes et al., J. Cell, Biol. 136, 1151-1163 (1997); Kojima et al., The Journal of Cell Biology, 121, 439-448 (1993)) MMP9 and MMP2 (Yu and Stamenkovic, Genes and Dev, 14, 163-176 (2000)).

The invention further provides nucleic acid encoding the fusion protein of the first aspect of the invention as defined above. A second aspect of the invention provides a nucleic acid construct comprising a first nucleic acid sequence encoding a pharmaceutically active agent, a second nucleic acid sequence encoding a LAP and a third nucleic acid sequence encoding a dimerisation domain polypeptide.

The term “nucleic acid construct” generally refers to any length of nucleic acid which may be DNA, cDNA or RNA such as mRNA obtained by cloning or produced by chemical synthesis. The DNA may be single or double stranded. Single stranded DNA may be the coding sense strand, or it may be the non-coding or anti-sense strand. For therapeutic use, the nucleic acid construct is preferably in a form capable of being expressed in the subject to be treated.

The pharmaceutically active agent may be suitable for interacting with soluble target molecules. Examples of soluble target molecules include cytokines, growth factors, signaling proteins and other ligands and receptors.

In an embodiment of the invention, the first nucleic acid sequence encodes a cytokine inhibitor. The term “cytokine inhibitor” refers to a molecule that can block, reduce, inhibit or neutralise a function, an activity and/or the expression of a cytokine. The cytokine inhibitor may be a protein (for example soluble cytokine receptor protein); an antibody or antibody fragment; nucleic acid (for example siRNA or anti-sense nucleic acid).

Where the first nucleic acid construct encodes an antibody or an antibody fragment, the antibody fragment may be, for example, an Fab, Fab′, F(ab′)2, scFv, Fv, dsFv diabody or Fd fragment. Examples of such molecules include trastuzumab (also known as Herclon™/Herceptin™), a monoclonal antibody to the HER2/neu receptor.

In some embodiments, the first nucleic acid sequence encodes the protein IFNβ, IL-4 or IL-1ra. In one embodiment of the invention, the first nucleic acid sequence encodes IFNβ, IL-4 or IL-1ra from a mouse or a human.

The nucleic acid construct of the second aspect of the invention may be in the form of a vector, for example, an expression vector, and may include, among others, chromosomal, episomal and virus-derived vectors, for example, vectors derived from bacterial plasmids, from bacteriophage, from transposons, from yeast episomes, from insertion elements, from yeast chromosomal elements, from viruses such as baculo-viruses, papova-viruses, such as SV40, vaccinia viruses, adenoviruses, fowl pox viruses, pseudorabies viruses and retroviruses, and vectors derived from combinations thereof, such as those derived from plasmid and bacteriophage genetic elements, such as cosmids and phagemids. Generally, any vector suitable to maintain, propagate or express nucleic acid to express a polypeptide in a host, may be used for expression in this regard. The vector may comprise a plurality of the nucleic acid constructs defined above, for example 2 or more.

The invention further provides a protein encoded by the nucleic acid construct of the second aspect of the invention optionally in association with latent TGFβ binding protein (LTBP) described herein. Typically, the protein encoded by the nucleic acid construct is covalently linked to LTBP to form a complex. Preferably, the association is mediated by disulphide bond(s) between Cys No. 33 of LAP and the third 8 Cys residue of LTBP.

The nucleic acid construct of the second aspect of the invention preferably includes a promoter or other regulatory sequence which controls expression of the nucleic acid. Promoters and other regulatory sequences which control expression of a nucleic acid have been identified and are known in the art. The person skilled in the art will note that it may not be necessary to utilise the whole promoter or other regulatory sequence. Only the minimum essential regulatory element may be required and, in fact, such elements can be used to construct chimeric sequences or other promoters. The essential requirement is, of course, to retain the tissue and/or temporal specificity. The promoter may be any suitable known promoter, for example, the human cytomegalovirus (CMV) promoter, the CMV immediate early promoter, the HSV thymidine kinase, the early and late SV40 promoters or the promoters of retroviral LTRs, such as those of the Rous Sarcoma virus (RSV) and metallothionine promoters such as the mouse metallothionine-I promoter. The promoter may comprise the minimum comprised for promoter activity (such as a TATA element without enhancer elements) for example, the minimum sequence of the CMV promoter. Preferably, the promoter is contiguous to the first and/or second nucleic acid sequence.

As stated herein, the nucleic acid construct of the second aspect of the invention may be in the form of a vector. Vectors frequently include one or more expression markers which enable selection of cells transfected (or transformed) with them, and preferably, to enable a selection of cells containing vectors incorporating heterologous DNA. A suitable start and stop signal will generally be present.

One embodiment of the invention relates to a cell comprising the nucleic acid construct of the second aspect of the invention. The cell may be termed a “host” cell, which is useful for the manipulation of the nucleic acid, including cloning. Alternatively, the cell may be a cell in which to obtain expression of the nucleic acid. Representative examples of appropriate host cells for expression of the nucleic acid construct of the invention include virus packaging cells which allow encapsulation of the nucleic acid into a viral vector; bacterial cells, such as Streptococci, Staphylococci, E. coli, Streptomyces and Bacillus subtilis; single cells, such as yeast cells, for example, Saccharomyces cerevisiae, and Aspergillus cells; insect cells such as Drosophila S2 and Spodoptera Sf9 cells, animal cells such as CHO, COS, C127, 3T3, PHK.293, and Bowes Melanoma cells and other suitable human cells; and plant cells e.g. Arabidopsis thaliana.

Introduction of an expression vector into the host cell can be affected by calcium phosphate transfection, DEAE-dextran mediated transfection, microinjection, cationic lipid-mediated transfection, electroporation, transduction, scrape loading, ballistic introduction, infection or other methods. Such methods are described in many standard laboratory manuals, such as Sambrook et al, Molecular Cloning, a Laboratory Manual, Second Edition, Coldspring Harbor Laboratory Press, Coldspring Harbor, N.Y. (1989).

Mature proteins can be expressed in host cells, including mammalian cells such as CHO cells, yeast, bacteria, or other cells under the control of appropriate promoters. Cell-free translation systems can be employed to produce such proteins using RNAs derived from the nucleic acid construct of the second aspect of the present invention. Appropriate cloning and expression vectors for use with prokaryotic and eukaryotic hosts are described by Sambrook et al, Molecular Cloning, a Laboratory Manual, Second Edition, Coldspring Harbor Laboratory Press, Coldspring Harbor, N.Y. (1989).

Proteins can be recovered and purified from recombinant cell cultures by well-known methods including ammonium sulphate or ethanol precipitation, acid extraction, anion or cation exchange chromatography, phosphocellulose chromatography, hydrophobic interaction chromatography, affinity chromatography, hydroxylapatite chromatography, high performance liquid chromatography, lectin and/or heparin chromatography. For therapy, the nucleic acid construct e.g. in the form of a recombinant vector, may be purified by techniques known in the art, such as by means of column chromatography as described in Sambrook et al, Molecular Cloning, a Laboratory Manual, Second Edition, Coldspring Harbor Laboratory Press, Coldspring Harbor, N.Y. (1989).

According to a third aspect of the invention, there is provided a composition in accordance with the first aspect of the invention for use in the treatment of inflammatory conditions or cancer. This aspect of the invention therefore extends to and includes a method for the treatment of inflammatory conditions or cancer comprising the administration to a subject of a composition comprising a fusion protein comprising a latency associated protein, a dimerisation domain and a pharmaceutically active agent.

The present invention provides a composition as described above for use in the treatment of inflammatory conditions or cancer. Inflammatory conditions include, without limitation, atherosclerosis, acute and chronic lung inflammation (e.g., chronic bronchitis, asthma, lung infection including bacterial and viral infections such as SARS and influenza, cystic fibrosis, etc.), inflammation of virus-infected tissues (e.g., viral lung infections, viral myocarditis, viral meningitis, etc.), ulcerative colitis, endotoxic shock, arthritis (e.g., rheumatoid arthritis, juvenile arthritis, osteoarthritis, psoriatic arthritis, reactive arthritis, viral or post-viral arthritis, ankylosing spondylarthritis, etc.), psoriasis, Crohn's disease, inflammatory bowel disease, insulin dependent diabetes mellitus, injury independent type II diabetes, ischemia induced inflammation, otitis media (middle ear infection), gout, multiple sclerosis, cachexia, and Ataxia Telangiectasia. Arthritis defines a group of disease conditions (or arthropathies) where damage is caused to the joints of the body and includes osteoarthritis (also known as degenerative joint disease) which can occur following trauma to the joint, following an infection of the joint or as a result of aging. Other forms of arthritis include rheumatoid arthritis and psoriatic arthritis, which are autoimmune diseases, and septic arthritis is caused by infection in the joints. Cancer defines a group of diseases characterized by an abnormal proliferation of cells in the body, which can be defined as tumors, for example glioma. Types of gliomas include ependymomas, astrocytomas, oligodendrogliomas and mixed gliomas. A Grade 4 astrocytoma is also known as a glioblastoma.

In a fourth aspect, the invention provides a nucleic acid sequence in accordance with the second aspect of the invention for use in the treatment of inflammatory conditions or cancer. This aspect therefore extends to and includes a method for the treatment of inflammatory conditions or cancer comprising the administration to a subject a nucleic acid construct of the second aspect of the invention. Where the nucleic acid construct is used in the therapeutic method of the invention, the construct may be used as part of an expression construct, e.g. in the form of an expression vector such as a plasmid or virus. In such a method, the construct may be administered intravenously, intradermally, intramuscularly, orally or by other routes.

The nucleic acid construct of the second aspect of the invention, and proteins derived therefrom, may be employed alone or in conjunction with other compounds, such as therapeutic compounds, e.g. anti-inflammatory drugs, cytotoxic agents, cytostatic agents or antibiotics. The nucleic acid constructs and proteins useful in the present invention are preferably provided in an isolated form, and preferably are purified to homogeneity.

As used herein, the term “treatment” includes any regime that can benefit a human or a non-human animal. The treatment of “non-human animals” extends to the treatment of domestic animals, including horses and companion animals (e.g. cats and dogs) and farm/agricultural animals including members of the ovine, caprine, porcine, bovine and equine families. The treatment may be in respect of any existing condition or disorder, or may be prophylactic (preventive treatment). The treatment may be of an inherited or an acquired disease. The treatment may be of an acute or chronic condition. Preferably, the treatment is of a condition/disorder associated with inflammation. The first nucleic acid sequence of the nucleic acid construct of the third aspect of the invention may encode a protein for use in the treatment of the disorder, including, but not limited to osteoarthritis, scleroderma, renal disease, rheumatoid arthritis, inflammatory bowel disease, multiple sclerosis, atherosclerosis, cancer, or any inflammatory disease.

The nucleic acid construct of the second aspect of the invention may be used therapeutically in a method of the invention by way of gene therapy. Alternatively, protein encoded by the nucleic acid construct may be directly administered as described herein.

Administration of the nucleic acid construct of the second aspect may be directed to the target site by physical methods. Examples of these include topical administration of the “naked” nucleic acid in the form of a vector in an appropriate vehicle, for example, in solution in a pharmaceutically acceptable excipient, such as phosphate buffered saline, or administration of a vector by physical method such as particle bombardment according to methods known in the art.

Other physical methods for administering the nucleic acid construct or proteins of the third aspect of the invention directly to the recipient include ultrasound, electrical stimulation, electroporation and microseeding. Further methods of administration include oral administration or administration through inhalation.

Particularly preferred is the microseeding mode of delivery which is a system for delivering genetic material into cells in situ in a patient. This method is described in U.S. Pat. No. 5,697,901.

The nucleic acid construct according to the second aspect of the invention may also be administered by means of delivery vectors. These include viral delivery vectors, such as adenovirus, retrovirus or lentivirus delivery vectors known in the art. Other non-viral delivery vectors include lipid delivery vectors, including liposome delivery vectors known in the art.

Administration may also take place via transformed host cells. Such cells include cells harvested from the subject, into which the nucleic acid construct is transferred by gene transfer methods known in the art. Followed by the growth of the transformed cells in culture and grafting to the subject.

As used herein the term “gene therapy” refers to the introduction of genes by recombinant genetic engineering of body cells (somatic gene therapy) for the benefit of the patient. Furthermore, gene therapy can be divided into ex vivo and in vivo techniques. Ex vivo gene therapy relates to the removal of body cells from a patient, treatment of the removed cells with a vector i.e., a recombinant vector, and subsequent return of the treated cells to the patient. In vivo gene therapy relates to the direct administration of the recombinant gene vector by, for example, intravenous or intravascular means. Preferably the method of gene therapy of the present invention is carried out ex vivo.

Preferably in gene therapy, the expression vector of the present invention is administered such that it is expressed in the subject to be treated. Thus for human gene therapy, the promoter is preferably a human promoter from a human gene, or from a gene which is typically expressed in humans, such as the promoter from human CMV.

For gene therapy, the present invention may provide a method for manipulating the somatic cells of human and non-human mammals.

The present invention also provides a gene therapy method which may involve the manipulation of the germ line cells of a non-human mammal.

The present invention therefore provides a method for providing a human with a therapeutic protein comprising introducing mammalian cells into a human, the human cells having been treated in vitro to insert therein a nucleic acid construct according to the second aspect of the invention.

Each of the individual steps of the ex vivo somatic gene therapy method are also covered by the present invention. For example, the step of manipulating the cells removed from a patient with the nucleic acid construct of the third aspect of the invention in an appropriate vector. As used herein, the term “manipulated cells” covers cells transfected with a recombinant vector. Also contemplated is the use of the transfected cells in the manufacture of a medicament for the treatment of inflammatory conditions, such as arthritis or cancer, as defined herein above.

The present invention may also find application in veterinary medicine for treatment/prophylaxis of domestic animals including horses and companion animals (e.g. cats and dogs) and farm animals which may include mammals of the ovine, porcine, caprine, bovine and equine families.

The present invention also relates to compositions comprising the nucleic acid construct or proteins of the first or second aspects of the invention. Therefore, the fusion protein or nucleic acid constructs of the present invention may be employed in combination with the pharmaceutically acceptable carrier or carriers. Such carriers may include, but are not limited to, saline, buffered saline, dextrose, liposomes, water, glycerol, ethanol and combinations thereof.

The pharmaceutical compositions of the invention may comprise two fusion proteins according to the first aspect of the invention, wherein the fusion proteins are associated at the dimerisation domain in each fusion protein, or a nucleic acid sequence encoding two fusion proteins according to the first aspect of the invention.

The pharmaceutical compositions may be administered in any effective, convenient manner effective for treating a patient's disease including, for instance, administration by oral, topical, intravenous, intramuscular, intranasal, or intradermal routes among others. In therapy or as a prophylactic, the active agent may be administered to an individual as an injectable composition, for example as a sterile aqueous dispersion, preferably isotonic.

For administration to mammals, and particularly humans, it is expected that the daily dosage of the active agent will be from 0.01 mg/kg up to 10 mg/kg body weight, typically around 1 mg/kg. The physician in any event will determine the actual dosage which will be most suitable for an individual which will be dependent on factors including the age, weight, sex and response of the individual. The above dosages are exemplary of the average case. There can, of course, be instances where higher or lower dosages are merited, and such are within the scope of this invention

References to uses of the fusions proteins, nucleic acid constructs, vectors, or host cells of the present invention in the treatment of diseases, such as inflammatory diseases or cancer, includes embodiments relating to the use of the fusion protein, nucleic acid construct, vector, or host cell in the manufacture of a medicament for the treatment of said diseases.

A fifth aspect of the invention provides a fusion protein comprising a LAP, a pharmaceutically active agent and an amino acid sequence comprising a dimerisation domain, wherein the LAP and the pharmaceutically active agent are connected by an amino acid sequence comprising a proteolytic cleavage site for use in the treatment of inflammatory conditions or cancer. The pharmaceutically active agent may be as described above. In some embodiments of this aspect of the invention, the pharmaceutically active agent may be an siRNA or PNA molecule.

The invention further provides a nucleic acid construct encoding the fusion protein of the fifth aspect of the invention. The nucleic acid construct preferably comprises a nucleic acid sequence encoding a LAP adjacent a nucleic acid sequence encoding a proteolytic cleavage site. Preferably, the nucleic acid sequence encoding a LAP is suitably operably linked to a nucleic acid sequence encoding a proteolytic cleavage site.

The invention further provides the fusion protein of the fifth aspect of the invention optionally in association with latent TGFβ binding protein (LTBP) described herein.

The fusion protein of the fifth aspect of the invention may be associated with the pharmaceutically active agent by means of a peptide bond linkage. Alternatively, the fusion protein may be associated with the pharmaceutically active agent by means of a chemical linkage e.g. by cross-linking the fusion protein to a chemical compound such as a chemotherapeutic agent, synthetic drug or PNA.

Preferably, the pharmaceutically active agent is linked to the C-terminal end of the amino acid sequence of the proteolytic cleavage site in the fusion protein of the seventh aspect of the invention. More preferably, the pharmaceutically active agent is continuous with the C-terminal residue of the amino acid sequence of the proteolytic cleavage site.

The fusion protein, and associated pharmaceutically active agent of the fifth aspect of the invention may be employed alone or in conjunction with other compounds, such as therapeutic compounds, e.g. anti-inflammatory drugs, cytotoxic agents, cytostatic agents or antibiotics. Such administration may be simultaneous, separate or sequential. The components may be prepared in the form of a kit which may comprise instructions as appropriate.

Preferably, the fusion protein and associated pharmaceutically active agent of the fifth aspect of the invention are directly administered to a patient as described herein.

The present invention also relates to compositions comprising the fusion protein and associated pharmaceutically active agent of the fifth aspect of the invention. Therefore, the fusion protein and associated pharmaceutically active agent may be employed in combination with the pharmaceutically acceptable carrier or carriers. Such carriers may include, but are not limited to, saline, buffered saline, dextrose, liposomes, water, glycerol, polyethylene glycol, ethanol and combinations thereof.

The pharmaceutical compositions may be administered in any effective, convenient manner effective for treating a disease of a patient including, for instance, administration by oral, topical, intravenous, intramuscular, intranasal, or intradermal routes among others. In therapy or as a prophylactic, the active agent may be administered to an individual as an injectable composition, for example as a sterile aqueous dispersion, preferably isotonic.

A sixth aspect of the invention provides a kit of parts comprising a fusion protein of the first aspect of the invention, a nucleic acid construct of the second aspect of the invention, or a fusion protein and associated pharmaceutically active agent according to the fifth aspect of the invention, and an administration vehicle including, but not limited to, tablets for oral administration, inhalers for lung administration and injectable solutions for intravenous administration.

A seventh aspect of the invention provides a process for preparing the fusion protein, of the first aspect of the invention comprising production of the fusion protein recombinant by expression in a host cell, purification of the expressed fusion protein and association of the pharmaceutically active agent to the purified fusion protein by means of peptide bond linkage, hydrogen or salt bond or chemical cross linking. In some embodiments of this aspect of the invention where the pharmaceutically active agent is a peptide, the fusion protein could be prepared using hydrogen or salt bonds where the peptide is capable or multimerisation, for example dimerisation or trimerisation.

An eighth aspect of the invention provides a process for preparing a nucleic acid construct of the second aspect of the invention comprising ligating together nucleic acid sequences encoding a latency associated peptide, a proteolytic cleavage sequence, and a pharmaceutically active agent, optionally including a linker sequence on either side of the proteolytic cleavage site.

One embodiment of the present invention provides a method of providing latency to a pharmaceutically active agent which is a cytokine, preferably interferon or an interleukin or a cytokine inhibitor such as a scFV or soluble cytokine receptor, the method comprising constructing a fusion protein having a latency associated peptide, preferably from TGFβ, associated with a proteolytic cleavage site, preferably an ADAM-TS4 cleavage site, and the pharmaceutically active agent. For example, the pharmaceutically active agent may be followed by the proteolytic cleavage site and the LAP as follows: Ig-LAP-cleavage site-active agent.

The present invention therefore enables the formation of a dimer which solves a problem of protein production in suspension cultures. The invention also enables (due to the closure of the “shell” of the LAP construct) the production of latent antibody fragments (e.g. inhibitors of cytokine action) as therapeutic agents. Previously, the fusion of a single peptide therapeutic agent with LAP left the “shell” partially open and thus potentially exposed without the need for release by protease action at the site of disease i.e. MMP/aggrecanase cleavage. For example, where the therapeutic peptide was a cytokine inhibitor, such as a scFv, it could interact if exposed with the cytokine before release at the site of disease.

The present invention can use any type of immunoglobulin (Ig) from any species (as their structure is extremely similar), but for certain clinical applications particular isotypes may be advantageous for example for in mucosal tissues IgA may be used, for binding to Fc receptors IgG2 may be used. Additionally, mutated forms of Fc that prevent them from binding to Fc receptors or activating cell mediated immunity or complement activation could be used if it was desirable for a particular clinical application.

All preferred features of the second and subsequent aspects of the invention are as for the first aspect mutatis mutandis.

The present invention will now be described by way of example only with reference to the accompanying figures wherein:

FIG. 1 shows amino acid sequences of the precursor domain of TGFβ1, 2 and 3 (human, Hu) (SEQ ID NOs:1-3), TGFβ4 (chicken, Ck) (SEQ ID NO:4), TGFβ (frog, Fg) (SEQ ID NO:5). Arrows indicate the position of the proteolytic processing resulting in cleavage of the signal peptide of TGFβ1 and of the mature TGFβs. N-linked glycosylation sites are underlined, as is the integrin cellular recognition sequence (Roberts and Sporn, Peptide Growth Factors and their Receptors: Sporn, M B and Roberts, AB, Springer-Verlag, Chapter 8, 422 (1996)).

FIG. 2 shows the sequences of protein cleavage sites of matrix metalloproteinases (MMPs) (Nagase and Fields, Biopolymers, 40, 399-416 (1996)) (SEQ ID NOs:6-78).

FIG. 3 shows a multiple sequence alignment of the ADAMTS-4 epitope sequences with corresponding average percentage of phagemid cleavage and the derived ADAMTS-4 cleavage motif. Predominant amino acids found at a frequency of greater than 40% in a particular position are illustrated with a black background, in contrast to related amino acids which are shown with a grey background (reproduced from Hills et al J. Biol. Chem. 282 11101-11109 (2007)) (SEQ ID NOs:79-129).

FIG. 4A shows the theoretical structure of LAP. FIG. 4B shows the theoretical structure of Ig-LAP. FIG. 4C shows a schematic representation of Ig-LAP.

FIG. 5 shows the DNA sequence (SEQ ID NO:130) and predicted amino acid sequence (SEQ ID NO:131) of mouse IgG1 (Fc)-LAP-MMP-IFN. Initiator ATG is at position 10 and stop codon at position 2025.

FIG. 6 shows the expression of Ig-LAP-IFN in CHO cells. Western blotting of LAP-IFN (slot 1) or Ig-LAP-IFN (slot 2). 20 μl supernatant from suspension CHO cells was run on 4-12% SDS-PAGE in non-denaturing conditions and blotted onto PDVF membrane. Then probed with goat anti-LAP antibodies. The bands were detected using HRP-conjugated anti-goat antibody by chemiluminescence (ECL, Amersham) and exposed to autoradiography.

FIG. 7 shows the cleavage of Ig-LAP-IFN by MMP1. 20 μl of CHO cell supernatant was incubated at 37° C. overnight without (slot 1) or with MMP1 (slot 2). The products were then run on a 4-12% SDS-PAGE gradient gel in non-denaturing conditions and blotted to a PDVF membrane. Anti-LAP antibodies were used to detect the uncleaved (slot 1) and cleaved product (slot 2). The molecular weight of the cleaved Ig-LAP corresponds to the expected size of about 160 kDa.

FIG. 8 shows the DNA sequence of human Ig-LAP with anti-herNeu2 (Herceptin™) antibody (SEQ ID NOs:132-134). The cleavage site in this construct is an aggrecanase-specific site. The secretory signal peptide is derived from IL-2 (nucleotides 1-54), the human CH2 and CH3 domains are derived from IgG1 (nucleotides 55-757) and is followed by a spacer with unique restriction sites HindIII and Nco1 (nucleotides 758-771) and the human LAP sequence (nucleotides 772-1515) is followed by the aggrecanase cleavage site which is flanked by GGGGS (SEQ ID NO:135) linkers (nucleotides 1516-1584) and finally the Herceptin™ scFv ending in a poly His tail (nucleotides 1585-2370).

FIG. 9 shows the detection of Herceptin™ by anti-His antibody labelled with a fluorophore. Ig-LAP Herceptin™ was produced in CHO cells in suspension and the fusion protein was purified from cell supernatants by affinity chromatography using a Protein A column. A fraction from the purified material was applied to breast cancer cells expressing Her/neu2 (SKBR3) or non-expressing (MDA-MD-231) before or after cleavage by aggrecanase. Herceptin™ scFv binds to the P185 Her Neu2 on breast cancer cells only after aggrecanase release of Herceptin™ from the hulg-LAP fusion.

The invention is now described with reference to the following non-limiting examples:

Example 1: Cloning the IgG1 Fc Between the Signal Peptide of IL-2 and Mouse LAP

An example of the preparation of a construct of the invention is as follows. PCR of mouse IgG1 was used for cloning the IgG1 Fc into an EcoR1 site after the signal peptide of muLAP-MMP-IFN. The following oligonucleotides were designed for linking in frame the coding regions.

Sense oligo:
(SEQ ID NO: 143)
5′ ATG AAT TCC GGT TGT AAG CCTTGCATA
Anti-sense oligo:
(SEQ ID NO: 144)
5′ GT GA ATT CCT CCA TGG AAG CTT TTT ACC AGG AGA
GTG GGA GAG

The EcoR1 sites in the oligos are underlined and the Nco1 and HindIII sites are in bold. These latter sites were introduced to allow for direct cloning of additional MMP or aggrecanase cleavage sites. Because the IgG1 fragment could be inserted on the opposite orientation needed for in-frame translation, the resulting clones were analysed by restriction analysis and these containing the IgG1 fragment in the right orientation sent for DNA sequencing. FIG. 5 depicts the DNA sequence of a representative positive clone.

Ig-LAP-MMP-IFN is effectively secreted from CHO cells grown in suspension:

Supernatant from transiently transfected CHO cells was analysed after non-reducing SDS-PAGE by western blotting using a goat anti-LAP antibody (R&D systems) (FIG. 6). The molecular weight of the Ig-LAP-IFN was bigger than that of LAP-IFN (i.e. above 200 kDa as expected from a glycosylated dimerised protein).

Id-LAP-Fusion is Cleaved by Recombinant MMP1:

In order to establish whether the Ig-LAP-IFN fusion is still cleavable by MMP the inventors digested the protein in the CHO supernatant with recombinant MMP-1 overnight at 37° C. The reaction was stopped with 25 mM EDTA and then analysed by western blotting after non-denaturing SDS-PAGE (FIG. 7).

After Cleavage with MMP, Ig-LAP-IFN Releases IFN Biological Activity:

Mouse L929 cells were plated at 104 cells/well in 96 well plates. The cells were incubated overnight with supernatants of Ig-LAP-IFN transfected CHO cell cultures that was treated or untreated with MMP-1 at double dilutions starting at 1:10. Then the medium was removed and the cells were infected with encephalomyocarditis virus in a volume of 50 μl for 16 hours as described (Adams et al. 2003). Cells were washed in PBS and 100 ml of Cell titer-Glo (Promega) cell lysis buffer. After 20 minutes and room temperature, 50 μl were transferred to an opaque plate and the luminescence (endogenous ATP levels) read in a Luminometer. 50% cell viability was assessed as half of luciferase activity compared to uninfected L929 cells (see Table 2 which shows MMP cleavage releases IFN activity from Ig-LAP-IFN).

	TABLE 2
		Luciferase	IFN biological
	Treatment	activity	activity (U/ml)
	Control No infection	10973	N/A
	Control (+EMC)	64
	Ig-LAP-IFN (no MMP1) + EMC	64	0
	IgLAP-IFN (+MMP) + EMC	5068	30

Example 2: Human IQ-Human LAP with Anti-herNeu2 (Herceptin™) Antibody

Human Ig-human LAP with anti-herNeu2 (Herceptin™—Markiv et al. BMC Biotechnology 2011, 11:117) antibody construct was created with an aggrecanase-specific cleavage site in CHO cells in suspension (FIG. 8). The secretory signal peptide was derived from IL-2 (nucleotides 1-54), the human CH2 and CH3 domains were derived from IgG1 (nucleotides 55-757). In the construct the human CH2 and CH3 domains are followed by a spacer with unique restriction sites HindIII and Nco1 (nucleotides 758-771). The human LAP sequence (nucleotides 772-1515) is followed by the aggrecanase cleavage site which is flanked by GGGGS linkers (nucleotides 1516-1584). The Herceptin™ scFv ends in a poly His tail (nucleotides 1585-2370). The fusion protein was purified from cell supernatants by affinity chromatography using a Protein A column. A fraction from the purified material was applied to breast cancer cells expressing Her/neu2 (SKBR3) or non-expressing (MDA-MD-231) before or after cleavage by aggrecanase. The bound Herceptin™ was detected by anti-His antibody labelled with a fluorophore (FIG. 9).

Claims

1-30. (canceled)

31. A protein dimer comprising a pair of fusion proteins, each fusion protein comprising a latency associated peptide (LAP) which is the precursor domain of TGFβ-1, -2, -3, -4, or -5, a pharmaceutically active agent and an amino acid sequence comprising a dimerisation domain comprising an antibody fragment polypeptide, wherein the LAP and the pharmaceutically active agent are connected by an amino acid sequence comprising a proteolytic cleavage site, and the dimerisation domain is linked to the N-terminus of the LAP, and wherein the fusion proteins are associated at the dimerisation domain in each fusion protein and form a closed shell around the pharmaceutically active agent, wherein the pharmaceutically active agent is an antibody or antibody fragment.

32. The protein dimer as claimed in claim 31, wherein the antibody fragment polypeptide is an Fc region polypeptide, an immunoglobulin hinge polypeptide, a CH3 domain polypeptide, a CH4 domain polypeptide, a CH1 domain polypeptide, or a CL domain polypeptide.

33. The protein dimer as claimed in claim 31, wherein the antibody fragment polypeptide is an Fc region polypeptide.

34. The protein dimer as claimed in claim 33, wherein the Fc region polypeptide is derived from an IgG or IgA antibody.

35. The protein dimer as claimed in claim 31, wherein the dimerisation domain is linked to the latency associated peptide by a linker sequence.

36. The protein dimer as claimed in claim 31, wherein the proteolytic cleavage site is a matrix metalloproteinase or an aggrecanase cleavage site.

37. The protein dimer as claimed in claim 31, wherein the antibody fragment is an scFv, Fab, Fab′, F(ab′)2, Fv, dsFv diabody, or Fd fragment.

38. The protein dimer as claimed in claim 31, wherein the antibody or antibody fragment thereof is an anti-TNF antibody, anti-interleukin antibody, anti-interferon antibody, anti-cytokine antibody, or fragment thereof.

39. The protein dimer as claimed in claim 31, wherein the antibody or antibody fragment thereof is an antibody against the HER2/neu receptor.

40. The protein dimer as claimed in claim 31, wherein the antibody fragment is a trastuzumab scFv.

41. A pharmaceutical composition comprising a protein dimer of claim 31.

42. A nucleic acid construct encoding a fusion protein as defined in claim 31 comprising a nucleic acid sequence encoding a pharmaceutically active agent, a nucleic acid sequence encoding a LAP, and a nucleic acid sequence encoding a dimerisation domain composed of an antibody fragment polypeptide, wherein the pharmaceutically active agent is an antibody or an antibody fragment.

43. The nucleic acid construct as claimed in claim 42, wherein the dimerisation domain polypeptide is an Fc region polypeptide derived from an IgG or IgA antibody.

44. The nucleic acid construct as claimed in claim 42, wherein the nucleic acid construct further comprises a nucleic acid sequence encoding a proteolytic cleavage site.

45. The nucleic acid construct as claimed in claim 42, which is in the form of a vector.

46. A fusion protein encoded by the nucleic acid construct of claim 42.

47. A cell comprising a nucleic acid construct of claim 42.

48. A pharmaceutical composition comprising a nucleic acid construct as claimed in claim 42.

49. A method for the treatment of an inflammatory condition or cancer comprising the administration to a subject of a composition comprising a protein dimer of claim 31.

50. A method for the treatment of an inflammatory condition or cancer comprising the administration to a subject of a composition comprising a nucleic acid construct of claim 42.

51. A kit comprising a protein dimer as claimed in claim 31 as an administration vehicle.

52. A process for preparing the protein dimer as claimed in claim 31, comprising producing the fusion proteins recombinantly by expression in a host cell, purifying the expressed fusion proteins, and associating the dimerisation domain of the fusion proteins at the N-terminus of the LAP to form a closed shell around the pharmaceutically active agent.

53. A process for preparing a nucleic acid construct of claim 42, comprising ligating together nucleic acid sequences encoding a latency associated peptide, a dimerisation domain, a proteolytic cleavage sequence, and a pharmaceutically active agent, optionally including a linker sequence on either side of the proteolytic cleavage site.