GAG binding protein

The present invention relates to methods and tools for the inhibition of the interaction of chemokines and their high-affinity receptors on leukocytes and methods for the therapeutic treatment of inflammatory diseases.

Chemokines, originally derived from chemoattractant cytokines, actually comprise more than 50 members and represent a family of small, inducible, and secreted proteins of low molecular weight (6-12 kDa in their monomeric form) that play a decisive role during immunosurveillance and inflammatory processes. Depending on their function in immunity and inflammation, they can be distinguished into two classes. Inflammatory chemokines are produced by many different tissue cells as well as by immigrating leukocytes in response to bacterial toxins and inflammatory cytokines like IL-1, TNF and interferons. Their main function is to recruit leukocytes for host defence and in the process of inflammation. Homing chemokines, on the other hand, are expressed constitutively in defined areas of the lymphoid tissues. They direct the traffic and homing of lymphocytes and dendritic cells within the immune system. These chemokines, as illustrated by BCA-1, SDF-1 or SLC, control the relocation and recirculation of lymphocytes in the context of maturation, differentiation, activation and ensure their correct homing within secondary lymphoid organs.

Despite the large number of representatives, chemokines show remarkably similar structural folds although the sequence homology varies between 20 to 70 percent. Chemokines consist of roughly 70-130 amino acids with four conserved cysteine residues. The cysteines form two disulphide bonds (Cys 1→Cys 3, Cys 2→Cys 4) which are responsible for their characteristic three-dimensional structure. Chemotactic cytokines consist of a short amino terminal domain (3-10 amino acids) preceding the first cysteine residue, a core made of β-strands and connecting loops found between the second and the fourth cysteine residue, as well as a carboxy-terminal α-helix of 20-60 amino acids. The protein core has a well ordered structure whereas the N- and C-terminal parts are disordered. As secretory proteins they are synthesised with a leader sequence of 20-25 amino acids which is cleaved off before release.

The chemokines have been subdivided into four families on the basis of the relative position of their cysteine residues in the mature protein. In the α-chemokine subfamily, the first two of the four cysteines are separated by a single amino acid (CXC), whereas in the β-chemokines the corresponding cysteine residues are adjacent to each other (CC). The α-chemokines can be further classified into those that contain the ELR sequence in the N-terminus, thereby being chemotactic for neutrophils (IL-8 for example), and those that lack the ELR motif and act on lymphocytes (I-TAC for example). Structurally the β-chemokines can be subdivided into two families: the monocyte-chemoattractant protein eotaxin family, containing the five monocyte chemoattractant proteins (MCP) and eotaxin which are approximately 65 percent identical to each other, and the remaining β-chemokines. As with the CXC-family, the N-terminal amino acids preceding the CC-residues are critical components for the biologic activity and leukocyte selectivity of the chemokines. The β-chemokines, in general, do not act on neutrophils but attract monocytes, eosinophils, basophils and lymphocytes with variable selectivity.

Only a few chemokines do not fit into the CC- or the CXC-family. Lymphotactin is so far the only chemokine which shows just two instead of the four characteristic cysteines in its primary structure, and is thus classified as γ- or C-chemokine. On the other hand, by concluding this classification, fractalkine has to be mentioned as the only representative of the δ- or CXXXC-subfamily with three amino acids separating the first two cysteines. Both of them, Lymphotaxin and fractalkine, induce chemotaxis of T-cells and natural killer cells.

Chemokines induce cell migration and activation by binding to specific cell surface, seven transmembrane-spanning (7TM) G-protein-coupled receptors on target cells. Eighteen chemokine receptors have been cloned so far including six CXC, ten CC, one CX3C and one XC receptor. Chemokine receptors are expressed on different types of leukocytes, some of them are restricted to certain cells (e.g. CXCR1 is restricted to neutrophils) whereas others are more widely expressed (e.g. CCR2 is expressed on monocytes, T cells, natural killer cells and basophils). Similar to chemokines, the receptors can be constitutively expressed on certain cells, whereas some are inducible. Some of them can even be down-regulated making the cells unresponsive to a certain chemokine but remaining responsive to another. Most receptors recognise more than one chemokine and vice versa but recognition is restricted to chemokines of the corresponding subfamily (see Table 1).

TABLE 1

Inflammatory

Chemokine
Receptor
Chemotactic for
Diseases

CXC-
IL-8
CXCR1
Neutrophils
Acute respiratory distress

Chemokine

CXCR2

syndrome [71];

(+ELR-motif)

Bacterial pneumonia [72];

Rheumathoid

arthritis [73];

Inflammatory bowel

disease [74];

Psoriasis [75];

Bacterial meningitis [76]

CC-
MCP-1
CCR2
Basophils; Monocytes;
Asthma [77];

Chemokine

Activated T cells;
Glomerulonephritis [78];

Dentritic cells; Natural
Atheroscleosis [79];

killer cells
Inflammatory bowel

disease [80];

Psoriasis [81];

Bacterial and viral

meningitis [82, 83]

RANTES
CCR1
Eosinophils; Monocytes;
Asthma [84];

Activated T cells;
Glomerulonephritis [85]

Dentritic cells

CCR3
Eosinophils; Basophils;

Dentritic cells

CCR5
Monocytes; Activated T

cells; Dentritic cells;

Natural killer cells

Chemokines have two main sites of interaction with their receptors, one in the amino-terminal domain and the other within an exposed loop of the backbone that extends between the second and the third cysteine residue. Both sites are kept in close proximity by the disulphide bonds. The receptor recognises first the binding site within the loop region which appears to function as a docking domain. This interaction restricts the mobility of the chemokine thus facilitating the proper orientation of the amino-terminal domain. Studies have been performed with mutant chemokines that still bound effectively to their receptors but did not signal. These mutants were obtained by amino acid deletion or modification within the N-termini of, for example, IL-8, RANTES and MCP-1.

Multiple intracellular signalling pathways occur after receptor activation as a result of chemokine binding. Chemokines also interact with two types of nonsignalling molecules. One is the DARC receptor which is expressed on erythrocytes and on endothelial cells and which binds CC- as well as CXC-chemokines to prevent them from circulation. The second type are heparan sulphate glycosaminoglycans (GAGs) which are part of proteoglycans and which serve as co-receptors of chemokines. They capture and present chemokines on the surface of the homing tissue (e.g. endothelial cells) in order to establish a local concentration gradient. In an inflammatory response, such as in rheumatoid arthritis, leukocytes rolling on the endothelium in a selectin-mediated process are brought into contact with the chemokines presented by the proteoglycans on the cell surface. Thereby, leukocyte integrins become activated which leads to firm adherence and extravasation. The recruited leukocytes are activated by local inflammatory cytokines and may become desensitised to further chemokine signalling because of high local concentration of chemokines. For maintaining a tissue bloodstream chemokine gradient, the DARC receptor functions as a sink for surplus chemokines.

Heparan sulphate (HS) proteoglycans, which consist of a core protein with covalently attached glycosaminoglycan sidechains (GAGs), are found in most mammalian cells and tissues. While the protein part determines the localisation of the proteoglycan in the cell membrane or in the extracellular matrix, the glycosaminoglycan component mediates interactions with a variety of extracellular ligands, such as growth factors, chemokines and adhesions molecules. The biosynthesis of proteoglycans has previously been extensively reviewed. Major groups of the cell surface proteoglycans are the syndecan family of transmembrane proteins (four members in mammals) and the glypican family of proteins attached to the cell membrane by a glycosylphosphatidylinositol (GPI) tail (six members in mammals). While glypicans are expressed widely in the nervous system, in kidney and, to a lesser extent, in skeletal and smooth muscle, syndecan-1 is the major HSPG in epithelial cells, syndecan-2 predominates in fibroblasts and endothelial cells, syndecan-3 abounds in neuronal cells and syndecan-4 is widely expressed. The majority of the GAG chains added to the syndecan core proteins through a tetrasaccharide linkage region onto particular serines are HS chains. Although the amino acid sequences of the extracellular domains of specific syndecan types are not conserved among different species, contrary to the transmembrane and the cytoplasmic domains, the number and the positions of the GAG chains are highly conserved. The structure of the GAGs, however, is species-specific and is, moreover, dependent upon the nature of the HSPG-expressing tissue.

Heparan sulphate (HS) is the most abundant member of the glycosaminoglycan (GAG) family of linear polysaccharides which also includes heparin, chondroitin sulphate, dermatan sulphate and keratan sulphate. Naturally occurring HS is characterised by a linear chain of 20-100 disaccharide units composed of N-acetyl-D-glucosamine (GlcNAc) and D-glucuronic acid (GlcA) which can be modified to include N- and O-sulphation (6-0 and 3-0 sulphation of the glucosamine and 2-0 sulphation of the uronic acid) as well as epimerisation of β-D-gluronic acid to α-L-iduronic acid (IdoA).

Clusters of N- and O-sulphated sugar residues, separated by regions of low sulphation, are assumed to be mainly responsible for the numerous protein binding and regulatory properties of HS. In addition to the electrostatic interactions of the HS sulphate groups with basic amino acids, van der Waals and hydrophobic interactions are also thought to be involved in protein binding. Furthermore, the presence of the conformationally flexible iduronate residues seems to favour GAG binding to proteins. Other factors such as the spacing between the protein binding sites play also a critical role in protein-GAG binding interactions: For example γ-interferon dimerisation induced by HS requires GAG chains with two protein binding sequences separated by a 7 kDa region with low sulphation. Additional sequences are sometimes required for full biological activity of some ligands: in order to support FGF-2 signal transduction, HS must have both the minimum binding sequence as well as additional residues that are supposed to interact with the FGF receptor.

Heparin binding proteins often contain consensus sequences consisting of clusters of basic amino acid residues. Lysine, arginine, asparagine, histidine and glutamine are frequently involved in electrostatic contacts with the sulphate and carboxyl groups on the GAG. The spacing of the basic amino acids, sometimes determined by the proteins 3-D structure, are assumed to control the GAG binding specificity and affinity. The biological activity of the ligand can also be affected by the kinetics of HS-protein interaction. Reducing the dimension of growth factor diffusion is one of the suggested HSPG functions for which the long repetitive character of the GAG chains as well as their relatively fast on and off rates of protein binding are ideally suited. In some cases, kinetics rather than thermodynamics drives the physiological function of HS-protein binding. Most HS ligands require GAG sequences of well-defined length and structure. Heparin, which is produced by mast cells, is structurally very similar to heparan sulphate but is characterised by higher levels of post-polymerisation modifications resulting in a uniformly high degree of sulphation with a relatively small degree of structural diversity. Thus, the highly modified blocks in heparan sulphate are sometimes referred to as “heparin-like”. For this reason, heparin can be used as a perfect HS analogue for protein biophysical studies as it is, in addition, available in larger quantities and therefore less expensive than HS. Different cell types have been shown to synthesise proteoglycans with different glycosaminoglycan structure which changes during pathogenesis, during development or in response to extracellular signals such as growth factors. This structural diversity of HSPGs leads to a high binding versatility emphasising the great importance of proteoglycans.

Since the demonstration that heparan sulphate proteoglycans are critical for FGF signalling, several investigations were performed showing the importance of chemokine-GAG binding for promoting chemokine activity. First, almost all chemokines studied to date appear to bind HS in vitro, suggesting that this represents a fundamental property of these proteins. Second, the finding that in vivo T lymphocytes secrete CC-chemokines as a complex with glycosaminoglycans indicates that this form of interaction is physiologically relevant. Furthermore, it is known that the association of chemokines with HS helps to stabilise concentration gradients across the endothelial surface thereby providing directional information for migrating leukocytes. HS is also thought to protect chemokines from proteolytic degradation and to induce their oligomerisation thus promoting local high concentrations in the vicinity of the G-coupled signalling receptors. The functional relevance of oligomerisation, however, remains controversial although all chemokines have a clear structural basis for multimerisation. Dimerisation through association of the β-sheets is observed for all chemokines of the CXC-family (e.g. IL-8), contrary to most members of the CC-chemokine family (e.g. RANTES), which dimerise via their N-terminal strands.

A wealth of data has been accumulated on the inhibition of the interaction of chemokines and their high-affinity receptors on leukocytes by low molecular weight compounds. However, there has been no breakthrough in the therapeutic treatment of inflammatory diseases by this approach.

Interleukin-8 (IL-8) is a key molecule involved in neutrophil attraction during chronic and acute inflammation. Several approaches have been undertaken to block the action of IL-8 so far, beginning with inhibition of IL-8 production by for example glucocorticoids, Vitamin D3, cyclosporin A, transforming growth factor β, interferons etc., all of them inhibiting IL-8 activity at the level of production of IL-8 mRNA. A further approach previously used is to inhibit the binding of IL-8 to its receptors by using specific antibodies either against the receptor on the leukocyte or against IL-8 itself in order to act as specific antagonists and therefore inhibiting the IL-8 activity.

The aim of the present invention is therefore to provide an alternative strategy for the inhibition or disturbance of the interaction of chemokines/receptors on leukocytes. Specifically the action of IL-8, RANTES or MCP-1 should be targeted by such a strategy.

Subject matter of the present invention is therefore a method to produce new GAG binding proteins as well as alternative GAG binding proteins which show a high(er) affinity to a GAG co-receptor (than the wild type). Such modified GAG binding proteins can act as competitors with wild-type GAG binding proteins and are able to inhibit or down-regulate the activity of the wild-type GAG binding protein, however without the side effects which occur with the known recombinant proteins used in the state of the art. The molecules according to the present invention do not show the above mentioned disadvantages. The present modified GAG binding proteins can be used in drugs for various therapeutical uses, in particular—in the case of chemokines—for the treatment of inflammation diseases without the known disadvantages which occur in recombinant chemokines known in the state of the art. The modification of the GAG binding site according to the present invention turned out to be a broadly applicable strategy for all proteins which activity is based on the binding event to this site, especially chemokines with a GAG site. The preferred molecules according to the present invention with a higher GAG binding affinity proved to be specifically advantageous with respect to their biological effects, especially with respect to their anti-inflammatory activity by their competition with wild type molecules for the GAG site.

Therefore, the present invention provides a method for introducing a GAG binding site into a protein characterised in that it comprises the steps:

- identifying a region in a protein which is not essential for structure maintenance
- introducing at least one basic amino acid into said site and/or deleting at least one bulky and/or acidic amino acid in said site,
  
  whereby said GAG binding site has a GAG binding affinity of K_d≦10 μM, preferably ≦1 μM, still preferred ≦0.1 μM. By introducing at least one basic amino acid and/or deleting at least one bulky and/or acidic amino acid in said region, a novel, improved “artificial” GAG binding site is introduced in said protein. This comprises the new, complete introduction of a GAG binding site into a protein which did not show a GAG binding activity before said modification. This also comprises the introduction of a GAG binding site into a protein which already showed GAG binding activity. The new GAG binding site can be introduced into a region of the protein which did not show GAG binding affinity as well as a region which did show GAG binding affinity. However, with the most preferred embodiment of the present invention, a modification of the GAG binding affinity of a given GAG binding protein is provided, said modified protein's GAG binding ability is increased compared to the wild-type protein. The present invention relates to a method of introducing a GAG binding site into a protein, a modified GAG binding protein as well as to an isolated DNA molecule, a vector, a recombinant cell, a pharmaceutical composition and the use of said modified protein.

BRIEF DESCRIPTION OF THE DRAWINGS

FIG. 1 shows a CD spectra.

FIG. 2 shows secondary structure contents of various mutants.

FIG. 3 shows graphics of results from fluorescence anisotropy tests of various mutants.

FIG. 4 shows graphics of results from fluorescence anisotropy tests of two mutants.

FIG. 5 shows the graphic of results from isothermal fluorescence titrations.

FIG. 6 shows the graphic of results from unfolding experiments of various mutants.

FIG. 7 shows chemotaxis index of IL-8 mutants.

FIG. 8 shows the results of the RANTES chemotaxis assay.

The term “introducing at least one basic amino acid” relates to the introduction of additional amino acids as well as the substitution of amino acids. The main purpose is to increase the relative amount of basic amino acids, preferably Arg, Lys, His, Asn and/or Gln, compared to the total amount of amino acids in said site, whereby the resulting GAG binding site should preferably comprise at least 3 basic amino acids, still preferred 4, most preferred 5 amino acids.

The GAG binding site is preferably at a solvent exposed position, e.g. at a loop. This will assure an effective modification.

Whether or not a region of a protein is essential for structure maintenance, can be tested for example by computational methods with specific programmes known to the person skilled in the art. After modification of the protein, the conformational stability is preferably tested in silico.

The term “bulky amino acid” refers to amino acids with long or sterically interfering side chains; these are in particular Trp, Ile, Leu, Phe, Tyr. Acidic amino acids are in particular Glu and Asp. Preferably, the resulting GAG binding site is free of bulky and acidic amino acids, meaning that all bulky and acidic amino acids are removed.

The GAG binding affinity is determined—for the scope of protection of the present application—over the dissociation constant K_d. One possibility is to determine the dissociation constant (K_d) values of any given protein by the structural change in ligand binding. Various techniques are well known to the person skilled in the art, e.g. isothermal fluorescence titrations, isothermal titration calorimetry, surface plasmon resonance, gel mobility assay, and indirectly by competition experiments with radioactively labelled GAG ligands. A further possibility is to predict binding regions by calculation with computational methods also known to the person skilled in the art, whereby several programmes may be used.

A protocol for introducing a GAG binding site into a protein is for example as follows:

- Identify a region of the protein which is not essential for overall structural maintenance and which might be suitable for GAG binding
- Design a new GAG binding site by introducing (replacement or insertion) basic Arg, Lys, His, Asp and Gln residues at any position or by deleting amino acids which interfere with GAG binding
- Check the conformational stability of the resulting mutant protein in silico
- Clone the wild-type protein cDNA (alternatively: purchase the cDNA)
- Use this as template for PCR-assisted mutagenesis to introduce the above mentioned changes into the amino acid sequence
- Subclone the mutant gene into a suitable expression system (prokaryotic or eukaryotic dependent upon biologically required post-translational modifications)
- Expression, purification and characterisation of the mutant protein in vitro
- Criterion for an introduced GAG binding affinity: K_d^GAG(mutant) <10 μM.

Examples of said engineered proteins with new GAG binding sites are for example the Fc part of IgG as well as the complement factors C3 and C4 modified as follows:

Fc:

(439) KSLSLS (444) -> KSKKLS
(SEQ ID NOS 1 & 2)

C3:

(1297) WIASHT (1302) -> WKAKHK
(SEQ ID NOS 3 & 4)

C4:

(1) MLDAERLK (8) -> MKKAKRLK
(SEQ ID NOS 5 & 6)

A further aspect of the present invention is a protein obtainable by the inventive method as described above. The inventive protein therefore comprises a—compared to the wild-type protein—new GAG binding site as defined above and will therefore act as competitor with natural GAG binding proteins, in particular since the GAG binding affinity of the inventive protein is very high, e.g. K_d≦10 μM.

A further aspect of the present invention is a modified GAG binding protein, whereby a GAG binding region in said protein is modified by substitution, insertion, and/or deletion of at least one amino acid in order to increase the relative amount of basic amino acids in said GAG binding region, and/or reduce the amount of bulky and/or acidic amino acids in said GAG binding region, preferably at a solvent exposed position, and in that the GAG binding affinity of said protein is increased compared to the GAG binding affinity of a respective wild-type protein.

It has been surprisingly shown that by increasing the relative amount of basic amino acids, in particular Arg, Lys, His, Asn and Gln, in the GAG binding region, the modified GAG binding protein shows increased GAG binding affinity compared to the wild-type proteins, in particular when the relative amount of basic amino acids is increased at a solvent exposed position, since a positively charged area on the protein surface has shown to enhance the binding affinity. Preferably, at least 3, still preferred 4, most preferred 5, basic amino acids are present in the GAG binding region.

The term “GAG binding protein” relates to any protein which binds to a GAG co-receptor. Whether or not a protein binds to a GAG co-receptor can be tested with the help of known protocols as mentioned above. Hileman et al. (BioEssays 20 (1998), 156-167) disclose consensus sites in glycosaminoglycan binding proteins. The information disclosed in this article is also useful as starting information for the present invention. The term “protein” makes clear that the molecules provided by the present invention are at least 80 amino acids in length. This is required for making them suitable candidates for the present anti-inflammation strategy. Smaller molecules interacting with a GAG binding site and being physiologically or pathologically relevant due to such an interaction are not known and therefore not relevant for the present invention. Preferably, the molecules according to the present invention are composed of at least 90, at least 100, at least 120, at least 150, at least 200, at least 300, at least 400 or at least 500 amino acid residues.

In the scope of the present application the term “GAG binding region” is defined as a region which binds to GAG with a dissociation constant (K_d-value) of under 100 μM, preferably under 50 μM, still preferred under 20 μM, as determined by isothermal fluorescence titration (see examples below).

Any modifications mentioned in the present application can be carried out with known biochemical methods, for example site-directed mutagenesis. It should also be noted that molecular cloning of GAG binding sites is, of course, prior art (see e.g. WO96/34965 A, WO 92/07935 A, Jayaraman et al. (FEBS Letters 482 (2000), 154-158), WO02/20715 A, Yang et al. (J. Cell. Biochem. 56 (1994), 455-468), wherein molecular shuffling or de novo synthesis of GAG regions are described; Butcher et al., (FEBS Letters 4009 (1997), 183-187) (relates to artificial peptides, not proteins); Jinno-Oue et al, (J. Virol. 75 (2001), 12439-12445) de novo synthesis)).

The GAG binding region can be modified by substitution, insertion and/or deletion. This means that a non-basic amino acid may be substituted by a basic amino acid, a basic amino acid may be inserted into the GAG binding region or a non-basic amino acid may be deleted. Furthermore, an amino acid which interferes with GAG binding, preferably all interfering amino acids binding is deleted. Such amino acids are in particular bulky amino acids as described above as well as acidic amino acids, for example Glu and Asp. Whether or not an amino acid interferes with GAG binding may be examined with for example mathematical or computational methods. The result of any of these modifications is that the relative amount of basic amino acids in said GAG binding region is increased, whereby “relative” refers to the amount of basic amino acids in said GAG binding region compared to the number of all amino acids in said GAG binding region. Furthermore, amino acids which interfere sterically or electrostatically with GAG binding are deleted.

Whether or not an amino acid is present in a solvent exposed position, can be determined for example with the help of the known three dimensional structure of the protein or with the help of computational methods as mentioned above.

Whether or not the GAG binding affinity of said modified protein is increased compared to the GAG binding affinity of the respective wild-type protein, can be determined as mentioned above with the help of, for example, fluorescence titration experiments which determine the dissociation constants. The criterion for improved GAG binding affinity will be K_d(mutant)<K_d(wild-type), preferably by at least 100%. Specifically improved modified proteins have—compared with wild-type K_d—a GAG binding affinity which is higher by a factor of minimum 5, preferably of minimum 10, still preferred of minimum 100. The increased GAG binding affinity will therefore preferably show a K_dof under 10 μM, preferred under 1 μM, still preferred under 0.1 μM.

By increasing the GAG binding affinity the modified protein will act as a specific antagonist and will compete with the wild-type GAG binding protein for the GAG binding.

Preferably, at least one basic amino acid selected from the group consisting of Arg, Lys, and His is inserted into said GAG binding region. These amino acids are easily inserted into said GAG binding region, whereby the term “inserted” relates to an insertion as such as well as substituting any non-basic amino acid with arginine, lysine or histidine. Of course, it is possible to insert more than one basic amino acid whereby the same basic amino acid may be inserted or also a combination of two or three of the above mentioned amino acids.

Still preferred, the protein is a chemokine, preferably IL-8, RANTES or MCP-1. Chemokines are known to have a site of interaction with co-receptor GAG whereby this chemokine binding is often a condition for further receptor activation as mentioned above. Since chemokines are often found in inflammatory diseases, it is of major interest to block the chemokine receptor activation. Such chemokines are preferably IL-8, RANTES or MCP-1, which are well characterised molecules and of which the GAG binding regions are well known (see, for example, Lortat-Jacob et al., PNAS 99 (3) (2002), 1229-1234). By increasing the amount of basic amino acids in the GAG binding region of these chemokines, their binding affinity is increased and therefore the wild-type chemokines will bind less frequently or not at all, depending on the concentration of the modified protein in respect to the concentration of the wild-type protein.

According to an advantageous aspect, said GAG binding region is a C terminal α-helix. A typicial chemical monomer is organised around a triple stranded anti-parallel β-sheet overlaid by a C-terminal α-helix. It has been shown that this C-terminal α-helix in chemokines is to a major part involved in the GAG binding, so that modification in this C-terminal α-helix in order to increase the amount of basic amino acids results in a modified chemokine with an increased GAG binding affinity.

Advantageously, positions 17, 21, 70, and/or 71 in IL-8 are substituted by Arg, Lys, His, Asn and/or Gln. Here it is possible that only one of these aforementioned sites is modified. However, also more than one of these sites may be modified as well as all, whereby all modifications may be either Arg or Lys or His or Asn or Gln or a mixture of those. In IL-8 these positions have shown to highly increase the GAG binding affinity of IL-8 and therefore these positions are particularly suitable for modifications.

Preferably the increased binding affinity is an increased binding affinity to heparan sulphate and/or heparin. Heparan sulphate is the most abundant member of the GAG family of linear polysaccharides which also includes heparin. Heparin is structurally very similar to heparan sulphate characterised by higher levels of post-polymerisation modifications resulting in a uniformly high degree of sulphation with a relatively small degree of structural diversity. Therefore, the highly modified blocks in heparan sulphate are sometimes referred to as heparin-like and heparin can be used as a heparan sulphate analogue for protein biophysical studies. In any case, both, heparan sulphate and heparin are particularly suitable.

Still preferred, a further biologically active region is modified thereby inhibiting or down-regulating a further biological activity of said protein. This further biological activity is known for most GAG binding proteins, for example for chemokines. This will be the binding region to a receptor, for example to the 7TM receptor. The term “further” defines a biologically active region which is not the GAG binding region which, however, binds to other molecules, cells or receptors and/or activates them. By modifying this further biologically active region the further biological activity of this protein is inhibited or down-regulated and thereby a modified protein is provided which is a strong antagonist to the wild-type protein. This means that on the one hand the GAG binding affinity is higher than in the wild-type GAG binding protein, so that the modified protein will to a large extent bind to the GAG instead of the wild-type protein. On the other hand, the further activity of the wild-type protein which mainly occurs when the protein is bound to GAG, is inhibited or down-regulated, since the modified protein will not carry out this specific activity or carries out this activity to a lesser extent. With this modified protein an effective antagonist for wild-type GAG binding proteins is provided which does not show the side effects known from other recombinant proteins as described in the state of the art. This further biologically active region can for example be determined in vitro by receptor competition assays (using fluorescently labelled wt chemokines, calcium influx, and cell migration (performed on native leukocytes or on 7TM stably-transfected cell lines). Examples of such further biologically active regions are, in addition to further receptor binding sites (as in the growth factor family), enzymatic sites (as in hydrolases, lyases, sulfotransferases, N-deacetylases, and copolymerases), protein interaction sites (as in antithrombin III), and membrane binding domains (as in the herpes simplex virus gD protein). With this preferred embodiment of double-modified proteins therefore dominant (concerning GAG binding) negative (concerning receptor) mutants are provided which are specifically advantageous with respect to the objectives set for the present invention.

Still preferred, said further biologically active region is modified by deletion, insertion, and/or substitution, preferably with alanine, a sterically and/or electrostatically similar residue. It is, of course, possible to either delete or insert or substitute at least one amino acid in said further biologically active region. However, it is also possible to provide a combination of at least two of these modifications or all three of them. By substituting a given amino acid with alanine or a sterically/electronically similar residue—“similar” meaning similar to the amino acid being substituted—the modified protein is not or only to a lesser extent modified sterically/electrostatically. This is particularly advantageous, since other activities of the modified protein, in particular the affinity to the GAG binding region, are not changed.

Advantageously, said protein is a chemokine and said further biological activity is leukocyte activation. As mentioned above, chemokines are involved in leukocyte attraction during chronic and acute inflammation. Therefore, by inhibiting or down-regulating leukocyte activation inflammation is decreased or inhibited which makes this particular modified protein an important tool for studying, diagnosing and treating inflammatory diseases.

According to an advantageous aspect, said protein is IL-8 and said further biologically active region is located within the first 10 N-terminal amino acids. The first N-terminal amino acids are involved in leukocyte activation, whereby in particular Glu-4, Leu-5 and Arg-6 were identified to be essential for receptor binding and activation. Therefore, either these three or even all first 10 N-terminal amino acids can be substituted or deleted in order to inhibit or down-regulate the receptor binding and activation.

A further advantageous protein is an IL-8 mutant with the first 6 N-terminal amino acids deleted. As mentioned above, this mutant will not or to a lesser extent bind and activate leukocytes, so that it is particularly suitable for studying, diagnosing and treating inflammatory diseases.

Preferably, said protein is an IL-8 mutant selected from the group consisting of del6F17RE70KN71R, del6F17RE70RN71K and del6E70KN71K. These mutants have shown to be particularly advantageous, since the deletion of the first 6 N-terminal amino acids inhibits or down-regulates receptor binding and activation. Furthermore, the two phenylalanines in position 17 and 21 were found to make first contact with the receptor on its N-terminal extracellular domain to facilitate the later activation of the receptor. In order to prevent any neutrophil contact, these two amino acids 17 and 21 are exchanged, whereby they are exchanged to basic amino acids, since they are in close proximity to the GAG binding motif of the C-terminal α-helix as can be seen on a three dimensional model of a protein. By exchanging the position 17 and/or 21 to either arginine or lysine the GAG binding affinity is therefore increased.

A further aspect of the present invention is an isolated polynucleic acid molecule which codes for the inventive protein as described above. The polynucleic acid may be DNA or RNA. Thereby the modifications which lead to the inventive modified protein are carried out on DNA or RNA level. This inventive isolated polynucleic acid molecule is suitable for diagnostic methods as well as gene therapy and the production of inventive modified protein on a large scale.

Still preferred, the isolated polynucleic acid molecule hybridises to the above defined inventive polynucleic acid molecule under stringent conditions. Depending on the hybridisation conditions complementary duplexes form between the two DNA or RNA molecules, either by perfectly being matched or also comprising mismatched bases (see Sambrook et al., Molecular Cloning: A laboratory manual, 2^nded., Cold Spring Harbor, N.Y. 1989). Probes greater in length than about 50 nucleotides may accommodate up to 25 to 30% mismatched bases. Smaller probes will accommodate fewer mismatches. The tendency of a target and probe to form duplexes containing mismatched base pairs is controlled by the stringency of the hybridisation conditions which itself is a function of factors, such as the concentration of salt or formamide in the hybridisation buffer, the temperature of the hybridisation and the post-hybridisation wash conditions. By applying well-known principles that occur in the formation of hybrid duplexes conditions having the desired stringency can be achieved by one skilled in the art by selecting from among a variety of hybridisation buffers, temperatures and wash conditions. Thus, conditions can be selected that permit the detection of either perfectly matched or partially mismatched hybrid duplexes. The melting temperature (Tm) of a duplex is useful for selecting appropriate hybridisation conditions. Stringent hybridisation conditions for polynucleotide molecules over 200 nucleotides in length typically involve hybridising at a temperature 15-25° C. below the melting temperature of the expected duplex. For oligonucleotide probes over 30 nucleotides which form less stable duplexes than longer probes, stringent hybridisation usually is achieved by hybridising at 5 to 10° C. below the Tm. The Tm of a nucleic acid duplex can be calculated using a formula based on the percent G+C contained in the nucleic acids and that takes chain lengths into account, such as the formula Tm=81.5-16.6 (log [Na⁺)])+0.41 (% G+C)−(600/N), where N=chain length.

A further aspect of the present invention relates to a vector which comprises an isolated DNA molecule according to the present invention as defined above. The vector comprises all regulatory elements necessary for efficient transfection as well as efficient expression of proteins. Such vectors are well known in the art and any suitable vector can be selected for this purpose.

A further aspect of the present application relates to a recombinant cell which is stably transfected with an inventive vector as described above. Such a recombinant cell as well as any therefrom descendant cell comprises the vector. Thereby a cell line is provided which expresses the modified protein either continuously or upon activation depending on the vector.

A further aspect of the present invention relates to a pharmaceutical composition which comprises a protein, a polynucleic acid or a vector according to the present invention as defined above and a pharmaceutically acceptable carrier. Of course, the pharmaceutical composition may further comprise additional substances which are usually present in pharmaceutical compositions, such as salts, buffers, emulgators, colouring agents, etc.

A further aspect of the present invention relates to the use of the modified protein, a polynucleic acid or a vector according to the present invention as defined above in a method for inhibiting or supressing the biological activity of the respective wild-type protein. As mentioned above, the modified protein will act as an antagonist whereby the side effects which occur with known recombinant proteins will not occur with the inventive modified protein. In the case of chemokines this will be in particular the biological activity involved in inflammatory reactions.

Therefore, a further use of the modified protein, polynucleic acid or vector according to the present invention is in a method for producing a medicament for the treatment of an inflammatory condition. In particular, if the modified protein is a chemokine, it will act as antagonist without side effects and will be particularly suitable for the treatment of an inflammatory condition. Therefore, a further aspect of the present application is also a method for the treatment of an inflammatory condition, wherein a modified protein according to the present invention, the isolated polynucleic acid molecule or vector according to the present invention or a pharmaceutical composition according to the present invention is administered to a patient.

Preferably, the inflammatory condition is selected from a group comprising rheumatoid arthritis, psoriasis, osteoarthritis, asthma, Alzheimer's disease, and multiple sclerosis. Since the activation through chemokines can be inhibited with a modified protein according to the present invention, inflammatory reactions can be inhibited or down-regulated whereby the above mentioned inflammatory conditions can be prevented or treated.

The present invention is described in further detail with the help of the following examples and figures to which the invention is, however, not limited whereby FIG. 1 is a CD spectra; FIG. 2 shows secondary structure contents of various mutants; FIGS. 3 and 4 show graphics of results from fluorescence anisotropy tests of various mutants; FIG. 5 shows the graphic of results from isothermal fluorescence titrations; FIG. 6 shows the graphic of results from unfolding experiments of various mutants, FIG. 7 shows chemotaxis index of IL-8 mutants (SEQ ID NOS 1070-1074 are disclosed respectively in order of appearance), and FIG. 8 shows the results of the RANTES chemotaxis assay.

EXAMPLES
Example 1
Generation of Recombinant IL-8 Genes and Cloning of the Mutants

Polymerase chain reaction (PCR) technique was used to generate the desired cDNAs for the mutants by introducing the mutations using sense and antisense mutagenesis primers. A synthetic plasmid containing the cDNA for wtIL-8 was used as template, Clontech Advantage®2 Polymerase Mix applied as DNA polymerase and the PCR reaction performed using a Mastergradient Cycler of Eppendorf. The mutagenesis primers used are summarised in the table below beginning with the forward sequences (5′ to 3′):

(SEQ ID NO: 7)

CACC ATG TGT CAG TGT ATA AAG ACA TAC TCC

(primer for the mutation Δ6)

(SEQ ID NO: 8)

CACC ATG TGT CAG TGT ATA AAG ACA TAC TCC AAA CCT

AGG CAC CCC AAA AGG ATA

(primer for the mutation Δ6 F17R F21R)

The reverse sequences are (5′ to 3′):

TTA TGA ATT CCT AGC CCT CTT
(SEQ ID NO: 9)

(primer for the mutation E70R)

TTA TGA ATT CTT AGC CCT CTT
(SEQ ID NO: 10)

(primer for the mutation E70K)

TTA TGA CTT CTC AGC CCT CTT
(SEQ ID NO: 11)

(primer for the mutation N71K)

TTA TGA CTT CTT AGC CCT CTT
(SEQ ID NO: 12)

(primer for the mutation E70K

N71K)

TTA TGA CTT CCT AGC CCT CTT
(SEQ ID NO: 13)

(primer for the mutation E70R

N71K)

TTA TGA CCT CTT AGC CCT CTT
(SEQ ID NO: 14)

(primer for the mutation E70K

N71R)

TTA TGA CCT CCT AGC CCT CTT
(SEQ ID NO: 15)

(primer for the mutation E70R

N71R)

The PCR products were purified, cloned into the pCR®T7/NT-TOPO®TA (Invitrogen) vector and transformed into TOP10F competent E. coli (Invitrogen). As a next step a confirmation of the sequence was carried out by double-stranded DNA sequencing using a ABI PRISM CE1 Sequencer.

Example 2
Expression and Purification of the Recombinant Proteins

Once the sequences were confirmed, the constructs were transformed into calcium-competent BL21(DE3) E. coli for expression. Cells were grown under shaking in 1 l Lennox Broth (Sigma) containing 100 μg/ml Ampicillin at 37° C. until an OD₆₀₀of about 0.8 was reached. Induction of protein expression was accomplished by addition of isopropyl-β-D-thiogalactopyranoside (IPTG) to a final concentration of 1 mM. Four hours later the cells were harvested by centrifugation at 6000 g for 20 minutes. The cell pellet was then resuspended in a buffer containing 20 mM TRIS/HCl, 50 mM NaCl, pH 8, sonicated at 100 watts for 5×20 s and finally centrifuged again for 20 min at 10,000 g. Since the main fraction of the recombinant IL-8 proteins was found in inclusion bodies, denaturing conditions were chosen for further purification. So the cell pellet was resuspended in a buffer of 6M Gua/HCl and 50 mM MES, pH 6.5. The suspension was then stirred at 4° C. for 4 hours, followed by a dialysis step against 50 mM MES, pH 6.5. The resulting suspension was then centrifuged and filtered to be loaded on a strong cation exchange column (SP Sepharose from Pharmacia Biotech). The elution was accomplished by a linear gradient from 0M-1M NaCl in a 50 mM MES buffer, pH 6.5 over 60 minutes. After lyophilisation of the fractions containing the desired protein, a second purification step was carried out by reversed-phase HPLC using a C18 column. In this case a non-linear gradient from 10%-90% Acetonitril was chosen to elute the desired protein. Refolding of the denatured protein was finally accomplished by the same cation exchange column under the same conditions as described above.

The protein was then checked for purity and identity by silver stain analysis in the first case and Western Blot analysis, using a specific monoclonal antibody against wtIL-8, in the second. Refolding of the proteins was also confirmed by Circular Dichroism (CD) measurements.

Example 3
Biophysical Characterisation of the Mutants

3.1 Circular Dicroism Measurements and Analysis

In order to investigate secondary structure changes of the mutant protein in the presence and absence of heparan sulphate (HS), CD spectroscopy was carried out. Measurements were recorded on a Jasco J-710 spectropolarimeter over a range of 195-250 nm, and a cell of 0.1 cm path length was used. Spectra of the protein solutions with a concentration of 5 μM were recorded with a response time of 1 s, step resolution of 0.2 nm, speed of 50 nm/min, band width of 1 nm and a sensitivity of 20 mdeg. Three scans were averaged to yield smooth spectra. The protein spectra were then background-corrected relating to the CD-signal either of the buffer itself or buffer/HS. Secondary structure analysis of the protein in the presence and absence of HS was finally accomplished using the programme SELCON.

Since a great number of amino acids were changed in a number of novel combinations, it was tried to find out the dimension of the resulting secondary structure changes by circular dichroism methods.

Different structures were obtained depending on the mutations introduced. Except for one mutant expressed (Δ6 F17R F21R E70K N71R) which didn't show any structure, all mutants exhibited measurable α-helices, β-sheets and loops. Compared to IL-8 wt only one mutant (Δ6 E70R) showed nearly similar structure whereas the others differed mainly in their α-helix which ranged from 17.20 to 45.2% out of the total structure. Nevertheless, this fact suggests that the overall structure of IL-8 wt was maintained despite many changes within the proteins sequence. This could not have been previously predicted. Having already found that heparan sulphate oligosaccharides only, and not heparin, were able to affect IL-8 wt secondary structure, attention was focused on the effects induced by unfractionated heparan sulphate. All examined mutants showed structural changes upon HS binding which can be seen as evidence of complex formation.

To demonstrate the structural changes upon introduced mutations and heparan sulphate addition, some of the data obtained are summarised in the graphs above and below.

3.2 Fluorescence Measurements

For studying concentration and ligand dependent quaternary structure changes fluorescence spectroscopy was performed. Due to its high sensitivity, requiring only nanogram quantities of protein, fluorescence technique was the method of choice for carrying out the desired investigations. Measurements were undertaken using a Perkin-Elmer (Beaconsfield, England) LS50B fluorometer.

3.3 Fluorescence Anisotropy

By recording the concentration dependent fluorescence anisotropy of the chemokine resulting from the extrinsic chromophore bisANS it was aimed to find out the dimerisation constant of the mutants. Measurements were performed in PBS starting with high concentrations (up to 4 μM protein) followed by stepwise dilution. For each data point, the anisotropy signal (r) recorded at 507 nm was averaged over 60 sec.

IL-8 oligomerisation has been reported to relevantly influence the proteins GAG binding properties. Set at monomeric concentration, IL-8 bound size defined oligosaccharides 1000-fold tighter than at dimeric concentration. Therefore, the oligomerisation properties of IL-8 mutants were investigated by fluorescence anisotropy. Since the IL-8 intrinsic fluorophore (Trp57) was not sensitive enough for all of the mutants, the extrinsic fluorophore bis-ANS was used for these measurements.

Again, as already noticed for the secondary structure, the mutant Δ6 E70R showed high resemblance also in the oligomerisation constant (k_oligo=350 nM) to IL-8 wt (k_oligo=379 nM). The mutant with the highest k_oligo(k_oligo=460 μM), which therefore dimerised worst, was Δ6 F17RF21R E70RN71K. Previous studies identified the β-sheets to be mainly involved in the dimerisation process, a fact, which correlates with the results for this mutants' secondary structure, which showed a very low share of β-sheet of only 11.4%. The mutant with the lowest k_oligo(k_oligo=147 nM), was found to be Δ6 F17RF21R E70K, which again showed the highest share of β-sheet structure (29.8%) of all mutants investigated. Also the impact of heparan sulphate addition was observed. As for IL-8 wt, where heparan sulphate caused a shift of the oligomerisation constant to much higher levels (k_oligo=1.075 μM), this was also found for the IL-8 mutants investigated. Δ6 F17RF21R E70K shifted from 0.147 μM to 1.162 μM, and the mutant Δ6 E70R from 0.350 μM to 1.505 μM in the presence of heparan sulphate. Some of the results obtained are demonstrated in FIGS. 3 and 4, whereby FIG. 3 shows the dependence of the fluorescence anisotropy of IL-8 mutants in PBS on the chemokine concentration and FIG. 4 shows the dependence of the fluorescence anisotropy of Δ6 F17RF21R E70K in PBS on the chemokine concentration in the presence (ten fold excess) and absence of HS ((pc=10 xy excess) protein concentration).

3.4 Isothermal Fluorescence Titration (IFT) Experiments

Dissociation constants (K_dvalues) are a measure for the binding affinity of a ligand to a protein and therefore concentration-dependent change in the fluorescence emission properties of the protein (fluorescence quenching) upon ligand binding was used for the determination of K_d. Since these mutants contain an intrinsic tryptophan chromophore which is located at or near the proposed GAG binding site and therefore should be sensitive to structural changes upon ligand binding, IFT experiments seemed to be suitable for this kind of investigation. Fluorescence intensity titration was performed in PBS using a protein concentration of 700 nM. The emission of the protein solution upon excitation at 282 nm was recorded over a range of 300-400 nm following the addition of an aliquot of the respective GAG ligand and an equilibration period of 60 sec.

Binding to unfractionated heparin and heparan sulphate was investigated. The mutants were set at dimeric concentration to assure sufficient sensitivity. A quenching of Trp57 fluorescence intensity upon GAG binding was registered within a range of 25-35%. Significant improvement of ligand binding was observed, especially for heparin binding. Δ6 F17RN71R E70K (K_d=14 nM) and Δ6 F17RF21R N71K (K_d=14.6 nM) showed 2600-fold better binding, and Δ6 E70K N71K (K_d=74 nM) 1760-fold better binding compared to IL-8 wt (K_d=37 μM). Good results were also obtained for heparan sulphate binding. For A6 F17RN71R E70K a K_dof 107 nM was found, for Δ6 F17RF21R N71K the K_dwas 95 nM and the mutant AG E70K N71K showed a K_dof 34 nM. As IL-8 wt binds with a K_dof 4.2 μM, the K_ds found for the mutants represent an extraordinary improvement in binding, see FIG. 5.

3.5 Unfolding Experiments

In order to obtain information about the proteins stability and whether this stability would be changed upon GAG ligand binding, unfolding experiments were undertaken. As mentioned above fluorescence techniques are very sensitive for observing quaternary structure changes and therefore are also the method of choice to investigate thermal structural changes of the protein. Measurements were undertaken as described for the IFT in which not the ligand concentration was changed but the temperature. Protein structure was observed at a concentration of 0.7 μM from temperatures of 15-85° C. in the absence and the presence of a 10 fold excess of heparan sulphate or heparin.

The emission maximum of the proteins ranged from 340 nm to 357 nm, values which are typical for a solvent exposed tryptophan residue. Beginning with the unfolding experiments at 15° C., the emission maximum of the mutants varied between 340 nm-351 nm. Compared to IL-8 wt, whose emission maximum was observed at 340 nm, this means slightly higher values. Upon an increase in temperature, the intensity of emission maximum decreased, accompanied by a shift of the maximum to either a higher or lower wavelength. The emission maximum of Δ6 E70R and Δ6 E70K N71K shifted from 352.5 nm-357 nm and 343 nm-345 nm, which is typical for a further exposure of the Trp57 residue to the solvent trough temperature increase, but interestingly the mutants Δ6 F17RN71R E70K and Δ6 F17RF21R E70R N71K showed a blue shift, ranging from 350 nm-343 nm and, less pronounced, from 350 nm-348 nm (see FIG. 6). By slowly decreasing the temperature, the process of unfolding was partially reversible regarding both the wavelength shift and changes of intensity. Addition of a 5 fold excess of heparan sulphate led to an increase of stability of the proteins, probably through complex formation. This could be observed on the one hand by a shift of the melting point to higher temperature, and on the other hand by a significantly less pronounced shift of emission maximum upon temperature increase.

Example 4
Cell-Based Assay of the Receptor-“Negative” Function of the Dominant-Negative IL-8 Mutants

In order to characterise the impaired receptor function of the IL-8 mutants with respect to neutrophil attraction, transfilter-based chemotaxis of neutrophils in response to IL-8 mutants was assayed in a microchemotaxis chamber equipped with a 5 μm PVP-free polycarbonate membrane.

Cell Preparation:

Briefly, a neutrophil fraction was prepared from freshly collected human blood. This was done by adding a 6% dextran solution to heparin-treated blood (1:2) which was then left for sedimentation for 45 min. The upper clear cell solution was collected and washed twice with HBSS w/o Ca and Mg. Cells were counted and finally diluted with HBSS at 2 Mio/ml cell suspension, taking into account that only 60% of the counted cells were neutrophils.

Chemotaxis Assay:

IL-8 mutants were diluted at concentrations of 10 μg/ml, 1 μg/ml and 0.1 μg/ml and put in triplicates in the lower compartment of the chamber (26 μl per well). The freshly prepared neutrophils were seeded in the upper chamber (50 μl per well) and incubated for 30 minutes at 37° C. in a 5% CO₂humidified incubator. After incubation, the chamber was disassembled, the upper side of the filter was washed and wiped off and cells attached to the lower side were fixed with methanol and stained with Hemacolor solutions (Merck). Cells were then counted at 400× magnifications in 4 randomly selected microscopic fields per well. Finally, the mean of three independent experiments was plotted against the chemokine concentration. In FIG. 7, the chemotaxis index for various IL-8 mutants is shown. As expected, all mutants showed significantly decreased receptor binding activity.

Example 5
Generation of Recombinant RANTES Genes, Expression, Biophysical and Activity Characterisation of the Mutants

The concept of dominant-negative “GAG-masking” chemokine mutants was also employed to RANTES, a chemokine involved in type IV hypersensitivity reactions like transplant rejection, atopic dermatitis as well as in other inflammatory disorders like arthritis, progressive glomerulonephritis and inflammatory lung disease.

The receptor binding capability was impaired by introducing into the wt protein an initiating methionine residue. Expression of the wt RANTES in E. Coli lead to the retention of this methionine residue, which renders wt RANTES to a potent inhibitor of monocyte migration, the so-called Met-RANTES. Different mutations enhancing the GAG binding affinity were introduced via PCR-based site-directed mutagenesis methods.

By these means 9 RANTES mutants have so far been cloned, expressed and purified, Met-RANTES A22K, Met-RANTES H23K, Met-RANTES T43K, Met-RANTES N46R, Met-RANTES N46K, Met-RANTES Q48K, Met-RANTES A22K/N46R, Met-RANTES V49R/E66S and Met-RANTES ¹⁵LSLA¹⁸V49R/E66S.

Isothermal fluorescence titration experiments were carried out to measure the relative affinity constants (Kd values) of the RANTES mutants for size defined heparin. As can be seen in the table all RANTES mutant proteins showed higher affinities for this heparin, with Met-RANTES A22K, Met-RANTES H23K, Met-RANTES T43K and Met-RANTES A22K/N46R showing the most promising results.

Kd in nM

Wt Rantes
456.2 ± 8.5

Met-Rantes V49R/E66S
345.5 ± 21.7

Rantes 15LSLA18 V49R/66S
297.3 ± 14.1

Rantes N46R
367.7 ± 11.7

Rantes N46K
257.4 ± 10.2

Rantes H23K
202.5 ± 12.8

Rantes Q48K
383.4 ± 39.6

Rantes T43K
139.2 ± 30.1

Rantes A22K
202.1 ± 9.8

Rantes A22K/N46R
164.0 ± 16.6

RANTES Chemotaxis Assay

RANTES mutant directed cell migration was investigated using the 48-well Boyden chamber system equipped with 5 μm PVP-coated polycarbonate membranes. RANTES and RANTES mutant dilutions in RPMI 1640 containing 20 mM HEPES pH 7.3 and 1 mg/ml BSA were placed in triplicates in the lower wells of the chamber. 50 μl of THP-1 cell suspensions (promonocytic cell line from the European collection of cell cultures) in the same medium at 2×10⁶cells/ml were placed in the upper wells. After a 2 h incubation period at 37° C. in 5% CO₂the upper surface of the filter was washed in HBSS solution. The migrated cells were fixed in methanol and stained with Hemacolor solution (Merck). Five 400× magnifications per well were counted and the mean of three independently conducted experiments was plotted against the chemokine concentration in FIG. 8. The error bars represent the standard error of the mean of the three experiments. Again, as in the case of the IL-8 mutants, all RANTES mutants showed significantly reduced receptor binding activity.

Example 6
Proteins with GAG Binding Regions

By bioinformatical and by proteomical means GAG binding proteins were characterised together with their GAG binding regions. In the following tables 2 and 3 chemokines are shown with their GAG binding regions (table 2) and examples of other proteins are given also with their GAG binding regions (table 3).

TABLE 2

Chemokines and their GAG binding domains

CXC-chemokines

IL-8:

¹⁸HPK²⁰, (R47) ⁶⁰RVVEKFLKR⁶⁸

(residues 60-68 of SEQ ID NO: 16)

SAKELRCQCIKTYSKPFHPKFIKELRVIESGPHCANTEIIVKLSDGRELC

LDPKENWVQRVVEKFLKRAENS

(SEQ ID NO: 16)

MGSA/GROα:

¹⁹HPK²¹, ⁴⁵KNGR⁴⁸

(residues 45-48 of SEQ ID NO: 17),

⁶⁰KKIIEK⁶⁶

(residues 60-66 of SEQ ID NO: 17)

ASVATELRCQCLQTLQGIHPKNIQSVNVKSPGPHCAQTEVIATLKNGRKA

CLNPASPIVKKIIEKMLNSDKSN

(SEQ ID NO: 17)

MIP-2α/GROβ:

¹⁹HLK²¹, K45, ⁶⁰KKIIEKMLK⁶⁸

(residues 60-68 of SEQ ID NO: 18)

APLATELRCQCLQTLQGIHLKNIQSVKVKSPGPHCAQTEVIATLKNGQKA

CLNPASPMVKKIIEKMLKNGKSN

(SEQ ID NO: 18)

NAP-2:

¹⁵HPK¹⁸, ⁴²KDGR⁴⁵

(residues 42-45 of SEQ ID NO: 19),

⁵⁷KKIVQK⁶²

(residues 57-62 of SEQ ID NO: 19)

AELRCLCIKTTSGIHPKNIQSLEVIGKGTHCNQVEVIATLKDGRKICLDP

DAPRIKKIVQKKLAGDESAD

(SEQ ID NO: 19)

PF-4:

²⁰RPRH²³

(residues 20-23 of SEQ ID NO: 20),

⁴⁶KNGR⁴⁹

(residues 46-49 of SEQ ID NO: 20),

⁶¹KKIIKK⁶⁶

(residues 61-66 of SEQ ID NO: 20)

EAEEDGDLQCLCVKTTSQVRPRHITSLEVIKAGPHCPTAQLIATLKNGRK

ICLDLQAPLYKKIIKKLLES

(SEQ ID NO: 20)

SDF-1α:

K1, ²⁴KHLK²⁷

(residues 24-27 of SEQ ID NO: 21),

⁴¹RLK⁴³

KPVSLSYRCPCRFFESHVARANVKHLKILNTPNCALQIVARLKNNNRQVC

IDPKLKWIQEYLEKALN

(SEQ ID NO: 21)

CC-chemokines

RANTES:

(¹⁷RPLPRAH²³(residues 17-23 of SEQ ID NO: 22))

⁴⁴RKNR⁴⁷

(residues 44-47 of SEQ ID NO: 22)

SPYSSDTTPCCFAYIARPLPRAHIKEYFYTSGKCSNPAVVFVTRKNRQVC

ANPEKKWVREYINSLEMS

(SEQ ID NO: 22)

MCP-2:

¹⁸RKIPIQR²⁴

(residues 18-24 of SEQ ID NO: 23),

⁴⁶KRGK⁴⁹

(residues 46-49 of SEQ ID NO: 23)

QPDSVSIPITCCFNVINRKIPIQRLESYTRITNIQCPKEAVIFKTKRGKE

VCADPKERWVRDSMKHLDQIFQNLKP

(SEQ ID NO: 23)

MCP-3:

²²KQR^{24 ,}⁴⁷KLDK⁵⁰

(residues 47-50 of SEQ ID NO: 24),

⁶⁶KHLDKK⁷¹

(residues 66-71 of SEQ ID NO: 24)

QPVGINTSTTCCYRFINKKIPKQRLESYRRTTSSHCPREAVIFKTKLDKE

ICADPTQKWVQDFMKHLDKKTQTPKL

(SEQ ID NO: 24)

MIP-1α:

R17, ⁴⁴KRSR⁴⁷

(residues 44-47 of SEQ ID NO: 25)

SLAADTPTACCFSYTSRQIPQNFIADYFETSSQCSKPGVIFLTKRSRQVC

ADPSEEWVQKYVSDLELSA

(SEQ ID NO: 25)

MIP-1β:

R18, ⁴⁵KRSK⁴⁸

(residues 45-48 of SEQ ID NO: 26)

APMGSDPPTACCFSYTARKLPRNFVVDYYETSSLCSQPAVVFQTKRSKQV

CADPSESWVQEYVYDLELN

(SEQ ID NO: 26)

MPIF-1:

R18, ⁴⁵KKGR⁴⁸

(residues 45-48 of SEQ ID NO: 27)

MDRFHATSADCCISYTPRSIPCSLLESYFETNSECSKPGVIFLTKKGRRF

CANPSDKQVQVCMRMLKLDTRIKTRKN

(SEQ ID NO: 27)

MIP-5/HCC-2:

⁴⁰KKGR⁴³

(residues 40-43 of SEQ ID NO: 28)

HFAADCCTSYISQSIPCSLMKSYFETSSECSKPGVIFLTKKGRQVCAKPS

GPGVQDCMKKLKPYSI

(SEQ ID NO: 28)

TABLE 3

SEQ ID

NO:

Peroxisome biogenesis
29
181 TRRAKE 186

factor 1
30
367 QKKIRS 372

31
1263 PKRRKN 1268

32
181 TRRAKE 186

33
367 QKKIRS 372

34
1263 PKRRKN 1268

MLTK-beta
35
415 SKRRGKKV 422

36
312 ERRLKM 317

37
416 KRRGKK 421

38
312 ERRLKM 317

39
416 KRRGKK 421

BHLH factor Hes4
40
43 EKRRRARI 50

41
43 EKRRRA 48

42
43 EKRRRA 48

Protocadherin 11
43
867 MKKKKKKK 874

44
867 MKKKKK 872

45
867 MKKKKK 872

46
899 MKKKKKKK 906

47
899 MKKKKK 904

48
899 MKKKKK 904

catenin (cadherin-
49
315 RRRLRS 320

associated protein),
50
404 VRKLKG 409

delta 1
51
460 LRKARD 465

52
545 RRKLRE 550

53
621 AKKGKG 626

54
787 AKKLRE 792

55
315 RRRLRS 320

56
404 VRKLKG 409

57
460 LRKARD 465

58
545 RRKLRE 550

59
621 AKKGKG 626

60
787 AKKLRE 792

Muscarinic acetylcholine
61
221 EKRTKD 226

receptor MS
62
427 TKRKRV 432

63
514 WKKKKV 519

64
221 EKRTKD 226

65
427 TKRKRV 432

66
514 WKKKKV 519

Alpha-2A adrenergi
67
147 PRRIKA 152

receptor
68
224 KRRTRV 229

69
147 FRRIKA 152

70
224 KRRTRV 229

IL-S promoter
71
440 TKKKTRRR 447

REII-region-binding
72
569 GKRRRRRG 576

protein
73
38 ARKGKR 43

74
437 GKKTKK 442

75
444 TRRRRA 449

76
569 GKRRRR 574

77
38 ARKGKR 43

78
437 GKKTKK 442

79
444 TRRRRA 449

80
569 GKRRRR 574

Mitofusin 1
81
291 ARKQKA 296

82
395 KKKIKE 400

83
291 ARKQKA 296

84
395 KKKIKE 400

N-cym protein
85
71 VRRCKI 76

86
71 VRRCKI 76

Smad ubiquitination
87
672 ERRARL 677

regulatory factor 1
88
672 ERRARL 677

CUG-BP and ETR-3 like
89
468 MKRLKV 473

factor 5
90
475 LKRPKD 480

91
468 MKRLKV 473

92
475 LKRPKD 480

Ewings sarcoma EWS-Fli1
93
347 QRKSKP 352

94
347 QRKSKP 352

NUF2R
95
455 LKRKMFKM 462

96
331 LKKLKT 336

97
347 VKKEKL 352

98
331 LKKLKT 336

99
347 VKKEKL 352

Kruppel-like zinc finger
100
22 EKRERT 27

protein GLIS2
101
22 EKEERT 27

FKSG32
102
15 LKRVRE 20

103
431 VRRGRI 436

104
15 LKRVRE 20

105
431 VRRGRI 436

BARH-LIKE 1 PROTEIN
106
175 LKKPRK 180

107
228 NRRTKW 233

108
175 LKKPRK 180

109
228 NRRTKW 233

Nucleolar GTP-binding
110
393 SRKKRERD 400

protein
111
624 GKRKAGKK 631

112
48 MRKVKF 53

113
141 IKRQKQ 146

114
383 ARRKRM 388

115
393 SRKKRE 398

116
490 KKKLKI 495

117
543 ARRSRS 548

118
550 TRKRKR 555

119
586 VKKAKT 591

120
629 GKKDRR 634

121
48 MRKVKF 53

122
141 IKRQKQ 146

123
383 ARRKRM 388

124
393 SRKKRE 398

125
490 KKKLKI 495

126
543 ARRSRS 548

127
550 TRKRKR 555

128
586 VKKAKT 591

129
629 GKKDRR 634

EVG1
130
17 RRRPKT 22

131
138 ERKRKA 143

132
17 RRRPKT 22

133
138 ERKRKA 143

ASPL
134
282 PKKSKS 287

135
282 PKKSKS 287

Zinc transporter 1
136
477 EKKPRR 482

137
477 EKKPRR 482

Uveal autoantigen
138
603 EKKGRK 608

139
995 ERKFKA 1000

140
1023 VKKNKQ 1028

141
603 EKKGRK 608

142
995 ERKFKA 1000

143
1023 VKKNKQ 1028

RAB39
144
7 VRRDRV 12

145
7 VRRDRV 12

Down syndrome cell
146
320 PRKVKS 325

adhesion molecule
147
387 VRKDKL 392

148
320 PRKVKS 325

149
387 VRKDKL 392

Proteintyrosine
150
139 GRKKCERY 146

phosphatase, non-
151
59 VKKNRY 64

receptor type 12
152
59 VKKNRY 64

WD-repeat protein 11
153
752 VRKIRF 757

154
752 VRKIRF 757

Gastric cancer-related
155
20 SRKRQTRR 27

protein VRG107
156
25 TRRRRN 30

157
25 TRRRRN 30

Early growth response
158
356 ARRKGRRG 363

protein 4
159
452 EKKRHSKV 459

160
357 RRKGRR 362

161
357 RRKGRR 362

Vesicle transport-
162
309 PKRKNKKS 316

related protein
163
226 DKKLRE 231

164
310 KRKNKK 315

165
355 VKRLKS 360

166
226 DKKLRE 231

167
310 KRKNKK 315

168
355 VKRLKS 360

UPF3X
169
140 AKKKTKKR 147

170
141 KKKTKK 146

171
217 ERRRRE 222

172
225 RKRQRE 230

173
233 RRKWKE 238

174
240 EKRKRK 245

175
296 DKREKA 301

176
373 RRRQKE 378

177
393 MKKEKD 398

178
426 VKRDRI 431

179
140 AKKKTKKRD 148

180
141 KKKTKK 146

181
217 ERRRRE 222

182
225 RKRQRE 230

183
233 RRKWKE 238

184
240 EKRKRK 245

185
296 DKREKA 301

186
373 RRRQKE 378

187
393 MKKEKD 398

188
426 VKRDRI 431

CGI-201 protein, type IV
189
49 ARRTRS 54

190
49 ARRTRS 54

RING finger protein 23
191
98 KRKIRD 103

192
98 KRKIRD 103

FKSG17
193
72 EKKARK 77

194
95 IRKSKN 100

195
72 EKKARK 77

196
95 IRKSKN 100

P83
197
681 ARKERE 686

198
681 ARKERE 686

Ovarian cancer-related
199
62 LKRDRF 67

protein 1
200
62 LKRDRF 67

MHC class II
201
407 HRRPRE 412

transactivator CIITA
202
741 PRKKRP 746

203
783 DRKQKV 788

204
407 HRRPRE 412

205
741 PRKKRP 746

206
783 DRKQKV 788

Platelet glycoprotein
207
275 SRRKRLRN 282

VI-2
208
275 SRRKRL 280

209
275 SRRKRL 280

Ubiquitin-like 5 protein
210
11 GKKVRV 16

211
11 GKKVRV 16

Protein kinase D2
212
191 ARKRRL 196

213
191 ARKRRL 196

Homeobox protein GSH-2
214
202 GKRMRT 207

215
252 NRRVKH 257

216
202 GKRMRT 207

217
252 NRRVKH 257

ULBP3 protein
218
166 ARRMKE 171

219
201 HRKKRL 206

220
166 ARRMKE 171

221
201 HRKKRL 206

Type II iodothyronine
222
87 SKKEKV 92

deiodinase
223
87 SKKEKV 92

224
299 SKRCKK 304

225
299 SKRCKK 304

Sperm antigen
226
160 LKKYKE 165

227
478 IKRLKE 483

228
160 LKKYKEKRT 168

229
160 LKKYKE 165

230
478 IKRLKE 483

UDP-GalNAc: polypeptide
231
4 ARKIRT 9

N-acetylgalactosaminyl-
232
44 DRRVRS 49

transferase
233
138 PRKCRQ 143

234
4 ARKIRT 9

235
44 DRRVRS 49

236
138 PRKCRQ 143

NCBE
237
62 HRRHRN 67

238
73 RKRDRE 78

239
1012 SKKKKL 1017

240
62 HRRHRH 67

241
73 RKRDRE 78

242
1012 SKKKKL 1017

WD repeat protein
243
372 LKKKEERL 379

244
384 EKKQRR 389

245
400 AKKMRP 405

246
384 EKKQRR 389

247
400 AKKMRP 405

Phosphodiesterase 11A
248
27 MRKGKQ 32

249
27 MRKGKQ 32

probable cation-
250
891 ERRRRPRD 898

transporting ATPase 2
251
306 SRKWRP 311

252
891 ERRRRP 896

253
306 SRKWRP 311

254
891 ERRRRP 896

HMG-box transcription
255
420 GKKKKRKR 427

factor TCF-3
256
399 ARKERQ 404

257
420 GKKKKR 425

258
420 GKKKKRKRE 428

259
399 ARKERQ 404

260
420 GKKKKR 425

HVPS11
261
793 VRRYRE 798

262
793 VRRYRE 798

PIST
263
165 NKKEKM 170

264
165 NKKEKM 170

FYN-binding protein
265
473 KKREKE 478

266
501 KKKFKL 506

267
682 LKKLKK 687

268
696 RKKFKY 701

269
473 KKREKE 478

270
501 KKKFKL 506

271
682 LKKLKK 687

272
696 RKKFKY 701

Clorf25
273
620 GKKQKT 625

274
620 GKKQKT 625

Clorf14
275
441 LRRRKGKR 448

276
70 LRRWRR 75

277
441 LRRRKG 446

278
70 LRRWRR 75

279
441 LRRRKG 446

T-box transcription
280
144 DKKAKY 149

factor TBX3
281
309 GRREKR 314

282
144 DKKAKY 149

283
309 GRREKR 314

Mitochondrial 39S
284
121 AKRQRL 126

ribosomal protein L47
285
216 EKRARI 221

286
230 RKKAKI 235

287
121 AKRQRL 126

288
216 EKRARI 221

289
230 RKKAKI 235

CGI-203
290
33 VRRIRD 38

291
33 VRRIRD 38

Jaggedl
292
1093 LRKRRK 1098

293
1093 LRKRRK 1098

Secretory carrier-
294
102 DRRERE 107

associated membrane
295
102 DRRERE 107

protein 1

Vitamin D receptor-
296
673 KKKKSSRL 680

interacting protein
297
672 TKKKKS 677

complex component
298
954 QKRVKE 959

DRIP205
299
978 GKRSRT 983

300
995 PKRKKA 1000

301
1338 GKREKS 1343

302
1482 HKKHKK 1487

303
1489 KKKVKD 1494

304
672 TKKKKS 677

305
954 QKRVKE 959

306
978 GKRSRT 983

307
999 PKRKKA 1000

308
1338 GKREKS 1343

309
1482 HKKHKK 1487

310
1489 KKKVKD 1494

Secretory carrier-
311
100 ERKERE 105

associated membrane
312
100 ERKERE 105

protein 2

Nogo receptor
313
420 SRKNRT 425

314
420 SRKNRT 425

FLAMINGO 1
315
169 GRRKRN 174

316
2231 ARRQRR 2236

317
169 GRRKRN 174

318
2231 ARRQRR 2236

CC-chemokine receptor
319
58 CKRLKS 63

320
58 CKRLKS 63

Prolactin regulatory
321
271 HKRLRQ 276

element-binding protien
322
271 HKRLRQ 276

Kappa B and V(D)J
323
17 PRKRLTKG 24

recombination signal
324
713 RKRRKEKS 720

sequences binding
325
903 PKKKRLRL 910

protien
326
180 HKKERK 185

327
629 TKKTKK 634

328
712 LRKRRK 717

329
903 PKKKRL 908

330
1447 QKRVKE 1452

331
1680 SRKPRM 1685

332
180 HKKERK 185

333
629 TKKTKK 634

334
712 LRKRRK 717

335
903 PKKKRL 908

336
1447 QKRVKE 1452

337
1680 SRKPRM 1685

Breast cancer
338
200 SKRKKA 205

metastasis-suppressor 1
339
229 IKKARA 234

340
200 SKRKKA 205

341
229 IKKARA 234

Forkhead box protein P3
342
414 RKKRSQRP 421

343
413 FRKKRS 418

344
413 FRKKRS 418

FAS BINDING PROTEIN
345
228 LKRKLIRL 235

346
391 RKKRRARL 398

347
358 ARRLRE 363

348
390 ERKKRR 395

349
629 CKKSRK 634

350
358 ARRLRE 363

351
390 ERKKRR 395

352
629 CKKSRK 634

Ubiquitin carboxyl-
353
28 HKRMKV 233

terminal hydrolase 12
354
244 LKRFKY 249

355
228 HKRMKV 233

356
244 LKRFKY 249

K1AA0472 protein
357
110 HRKPKL 115

358
110 HRKPKL 115

PNAS-101
359
68 LKRSRP 73

360
106 PRKSRR 111

361
68 LKRSRP 73

362
106 PRKSRR 111

PNAS-26
363
118 DRRTRL 123

364
118 DRRTRL 123

Myelin transcription
365
176 GRRKSERQ 183

factor 2

Sodium/potassium-
366
47 SRRFRC 52

transporting ATPase
367
55 NKKRRQ 60

gamma chain
368
47 SRRFRC 52

369
55 NKKRRQ 60

Mdm4 protein
370
441 EKRPRD 446

371
464 ARRLKK 469

372
441 EKRPRD 446

373
464 ARRLKK 469

G antigen family D 2
374
87 QKKIRI 92

protein
375
87 QKKIRI 92

NipSnap2 protein
376
153 FRKARS 158

377
153 FRKARS 158

Stannin
378
73 ERKAKL 78

379
73 ERKAKL 78

Sodium bicarbonate
380
973 EKKKKKKK 980

cotransporter
381
165 LRKHRH 170

382
666 LKKFKT 671

383
966 DKKKKE 971

384
973 EKKKKK 978

385
165 LRKHRH 170

386
666 LKKFKT 671

387
966 DKKKKE 971

388
973 EKKKKK 978

Myosin X
389
683 YKRYKV 688

390
828 EKKKRE 833

391
1653 LKRIRE 1658

392
1676 LKKTKC 1681

393
683 YKRYKV 688

394
828 EKKKRE 833

395
1653 LKRIRE 1658

396
1676 LKKTKC 1681

PNAS-20
397
21 RKRKSVRG 28

398
20 ERKRKS 25

399
20 ERKRKS 25

Pellino
400
36 RRKSRF 41

401
44 FKRPKA 49

402
36 RRKSRF 41

403
44 FKRPKA 49

Hyaluronan mediated
404
66 ARKVKS 71

motility receptor
405
66 ARKVKS 71

Short transient receptor
406
753 FKKTRY 758

potential channel 7
407
753 FKKTRY 758

Liprin-alpha2
408
825 PKKKGIKS 832

409
575 IRRPRR 580

410
748 LRKHRR 753

411
839 GKKEKA 844

412
875 DRRLKK 880

413
575 IRRPRR 580

414
748 LRKHRR 753

415
839 GKKEKA 844

416
875 DRRLKK 880

Transcription
417
904 DKRKCERL 911

intermediary factor 1-
418
1035 PRKKRLKS 1042

alpha
419
321 NKKGKA 326

420
1035 PRKKRL 1040

421
321 NKKGKA 326

422
1035 PRKKRL 1040

CARTILAGE INTERMEDIATE
423
719 QRRNKR 724

LAYER PROTEIN
424
719 QRRNKR 724

UBX domain-containing
425
194 YRKIKL 199

protien 1
426
194 YRKIKL 199

Arachidonate 12-
427
166 VRRHRN 171

lipoxygenase, 12R type
428
233 WKRLKD 238

429
166 VRRHRN 171

430
233 WKRLKD 238

Hematopoietic PBX-
431
159 LRRRRGRE 166

interacting protein
432
698 LKKRSGKK 705

433
159 LRRRRG 164

434
703 GKKDKH 708

435
159 LRRRRG 164

436
703 GKKDKH 708

NAG18
437
28 LKKKKK 33

438
28 LKKKKK 33

POU 5 domain protein
439
222 ARKRKR 227

440
222 ARKRKR 227

NRCAM PROTEIN
441
2 PKKKRL 7

442
887 SKRNRR 892

443
1185 IRRNKG 1190

444
1273 GKKEKE 1278

445
2 PKKKRL 7

446
887 SKRNRR 892

447
1185 IRRNKG 1190

448
1273 GKKEKE 1278

protocadherin gamma
449
11 TRRSRA 16

cluster
450
11 TRRSRA 16

SKD1 protein
451
288 IRRRFEKR 295

452
251 ARRIKT 256

453
362 FKKVRG 367

454
251 ARRIKT 256

455
362 FKKVRG 367

ANTI-DEATH PROTEIN
456
58 HRKRSRRV 65

457
59 RKRSRR 64

458
59 RKRSRR 64

Centrin 3
459
14 TKRKKRRE 21

460
14 TKRKKR 19

461
14 TKRKKR 19

Ectonucleoside
462
512 TRRKRH 517

triphosphate
463
512 TRRKRH 517

diphosphohydrolase 3

Homeobox protein prophet
464
12 PKKGRV 17

of PIT-1
465
69 RRRHRT 74

466
119 NRRAKQ 124

467
12 PKKGRV 17

468
69 RRRHRT 74

469
119 NRRAKQ 124

PROSTAGLANDIN EP3
470
77 YRRRESKR 84

RCEPTOR
471
389 MRKRRLRE 396

472
82 SKRKKS 87

473
389 MRKRRL394

474
82 SKRKKS 87

475
389 MRKRRL394

Pituitary homeobox 3
476
58 LKKKQRRQ 65

477
59 KKKQRR 64

478
112 NRRAXW 117

479
118 RKRERS 123

480
59 KKKQRR 64

481
112 NRRAKW 117

482
118 RKRERS 123

HPRL-3
483
136 KRRGRI 141

484
136 KRRGRI 141

Advillin
485
812 MKKEKG 817

486
812 MKKEKG 817

Nuclear LIM interactor-
487
32 GRRARP 37

interacting factor 1
488
109 LKKQRS 114

489
32 GRRARP 37

490
109 LKKQRS 114

Core histone macro-H2A.1
491
5 GKKKSTKT 12

492
114 AKKRGSKG 121

493
70 NKKGRV 75

494
132 ANKAKS 137

495
154 ARKSKK 159

496
302 DKKLKS 307

497
70 NKKGRV 75

498
132 AKKAKS 137

499
154 ARKSKK 159

500
302 DKKLKS 307

Villin-like protein
501
180 KRRRNQKL 187

502
179 EKRRRN 184

503
179 EKRRRN 184

BETA-FILAMIN
504
254 PKKARA 259

505
2002 ARRAKV 2007

506
254 FKKARA 259

507
2002 ARRAKV 2007

Tripartite motif protein
508
290 LKKFKD 295

TRIM31 alpha
509
290 LKKFKD 295

Nuclear receptor co-
510
106 SKRPRL 111

repressor 1
511
299 ARKQRE 304

512
330 RRKAKE 335

513
349 IRKQRE 354

514
412 QRRVKF 417

515
497 KRRGRN 502

516
580 RRKGRI 585

517
687 SRKPRE 692

518
2332 SRKSKS 2337

519
106 SKRPRL 111

520
299 ARKQRE 304

521
330 RRKAKE 335

522
349 IRKQRE 354

523
412 QRRVKF 417

524
497 KRRGRN 502

525
580 RRKGRI 585

526
687 SRKPRE 692

527
2332 SRKSKS 2337

BRAIN EXPRESSED RING
528
432 KRRVKS 437

FINGER PROTEIN
529
432 KRRVKS 437

PB39
530
231 TKKIKL 236

531
231 TKKIKL 236

Sperm acrosomal protein
532
48 FRKRMEKE 55

533
24 RRKARE 29

534
135 KRKLKE 140

535
213 KKRLRQ 218

536
24 RRKARE 29

537
135 KRKLKE 140

538
213 KKRLRQ 218

VESICLE TRAFFICKING
539
177 SKKYRQ 182

PROTEIN SEC22B
540
177 SKKYRQ 182

Nucleolar transcription
541
79 VRKFRT 84

factor 1
542
102 GKKLKK 107

543
125 EKRAKY 130

544
147 SKKYKE 152

545
156 KKKNKY 161

546
240 KKRLKW 245

547
451 KKKAKY 456

548
523 EKKEKL 528

549
558 SKKMKF 563

550
79 VRKFRT 84

551
102 GKKLKK 107

552
125 EKRAKY 130

553
147 SKKYKE 152

554
156 KKKMKY 161

555
240 KKRLKW 245

556
451 KKKAKY 456

557
523 EKKEKL 528

558
558 SKKMKF 563

Plexin-B3
559
248 FRRRGARA 255

Junctophilin type 3
560
626 QKRRYSKG 633

Plaucible mixed-lineage
561
773 YRKKPHRP 780

kinase protein
562
312 ERRLKM 317

563
312 ERRLKM 317

fatty acid binding
564
78 DRKVKS 83

protein 4, adipocyte
565
105 IKRKRE 110

566
78 DRKVKS 83

567
105 IKRKRE 110

exostoses (multiple) 1
568
78 SKKGRK 83

569
78 SKKGRK 83

DHHC-domain-containing
570
64 HRRPRG 69

cysteine-rich protein
571
64 HRRPRG 69

Myb proto-oncogene
572
2 ARRPRH 7

protein
573
292 EKRIKE 297

574
523 LKKIKQ 528

575
2 ARRPRH 7

576
292 EKRIKE 297

577
523 LKKIKQ 528

Longchain-fatty-acid--
578
259 RRKPKP 264

COA ligase 2
579
259 RRKPKP 264

syntaxin1B2
580
260 ARRKKI 265

581
260 ARRKKI 265

Dachshund 2
582
162 ARRKRQ 167

583
516 QKRLKK 521

584
522 EKKTKR 527

585
162 APRKRQ 167

586
516 QKRLKK 521

587
522 EKKTKR 527

DEAD/DEXH helicase DDX31
588
344 EKRKSEKA 351

589
760 TRKKRK 765

590
760 TRKKRK 765

Androgen receptor
591
628 ARKLKK 633

592
628 ARKLKK 633

Retinoic acid receptor
593
364 RKRRPSRP 371

alpha
594
163 NKKKKE 168

595
363 VRKRRP 368

596
163 NKKKKE 168

597
363 VRKRRP 368

Kinesin heavy chain
598
340 WKKKYEKE 347

599
605 VKRCKQ 610

600
864 EKRLRA 869

601
605 VKRCKQ 610

602
864 EKRLRA 869

DIUBIQUITIN
603
30 VKKIKE 35

604
30 VKKIKE 35

BING1 PROTEIN
605
519 NKKFKM 524

606
564 ERRHRL 569

607
519 NKKFKM 524

608
564 ERRHRL 569

Focal adhesion kinase 1
609
664 SRRPRF 669

610
664 SRRPRF 669

EBN2 PROTEIN
611
20 TKRKKPRR 27

612
13 PKKDKL 18

613
20 TKRKKP 25

614
47 NKKNRE 52

615
64 LKKSRI 69

616
76 PKKPRE 81

617
493 SRKQRQ 498

618
566 VKRKRK 571

619
13 PKKDKL 18

620
20 TKRKKP 25

621
47 NKKNRE 52

622
64 LKKSRI 69

623
76 PKKPRE 81

624
493 SRKQRQ 498

625
566 VKRKRK 571

CO16 PROTEIN
626
33 ARRLRR 38

627
115 PRRCKW 120

628
33 ARRLRR 38

629
115 PRRCKW 120

KYNURENINE 3-
630
178 MKKPRF 183

MONOOXYGENASE
631
178 MKKPRF 183

MLN 51 protein
632
4 RRRQRA 9

633
255 PRRIRK 260

634
407 ARRTRT 412

635
4 RRRQRA 9

636
255 PRRIRK 260

637
407 ARRTRT 412

MHC class II antigen
638
99 QKRGRV 104

MHC class II antigen
639
99 QKRGRV 104

Transforming acidic
640
225 SRRSKL 230

colied-coli-containing
641
455 PKKAKS 460

protein 1
642
225 SRRSKL 230

643
455 PKKAKS 460

Neuro-endocrine specific
644
479 EKRNRK 484

protein VGF
645
479 EKRNRK 484

Organic cation
646
230 GRRYRR 235

transporter
647
535 PRKNKE 540

648
230 GRRYRR 235

649
535 PRKNKE 540

DNA polymerase theta
650
215 KRRKHLKR 222

651
214 WKRRKH 219

652
220 LKRSRD 225

653
1340 GRKLRIA 1345

654
1689 SRKRKL 1694

655
214 WKRRKH 219

656
220 LKRSRD 225

657
1340 GRKLRL 1345

658
1689 SRKRKL 1694

CDC45-related protein
659
169 MRRRQRRE 176

660
155 EKRTRL 160

661
170 RRRQRR 175

662
483 NRRCKL 488

663
155 EKRTRL 160

664
170 RRRQRR 175

665
483 NRRCKL 488

Chloride intracellular
666
197 AKKYRD 202

channel protein 2
667
197 AKKYRD 202

Methyl-CpG binding
668
85 KRKKPSRP 92

protein
669
83 SKKRKK 88

670
318 QKRQKC 323

671
354 YRRRKR 359

672
83 SKKRKK 88

673
318 QKRQKC 323

674
354 YRRRKR 359

Protein kinase C, eta
675
155 RKRQRA 160

type
676
155 RKRQRA 160

Heterogeneous nuclear
677
71 LKKDRE 76

ribonucleoprotein H
678
169 LKKHKE 174

679
71 LKKDRE 76

680
169 LKKHKE 174

ORF2
681
11 SRRTRW 16

682
155 ERRRKF 160

683
185 LRRCRA 190

684
530 SRRSRS 535

685
537 GRRRKS 542

686
742 ERRAKQ 747

687
11 SRRTRW 16

688
155 ERRRKF 160

689
185 LRRCRA 190

690
530 SRRSRS 535

691
537 GRRRKS 542

692
742 ERRAKQ 747

F-box only protein 24
693
9 LRRRRVKR 16

694
9 LRRRRV 14

695
29 EKRGKG 34

696
9 LRRRRV 14

697
29 EKRGKG 34

Leucin rich neuronal
698
51 NRRLKH 56

protein
699
51 NRRLKH 56

RER1 protein
700
181 KRRYRG 186

701
181 KRRYRG 186

Nephrocystin
702
3 ARRQRD 8

703
430 PKKPKT 435

704
557 NRRSRN 562

705
641 EKRDKE 646

706
3 ARRQRD 8

707
430 PKKPKT 435

708
557 NRRSRN 562

709
641 EKRDKE 646

Adenylate kinase
710
60 GKKLKA 65

isoenzyme 2,
711
116 KRKEKL 121

mitochondrial
712
60 GKKLKA 65

713
116 KRKEKL 121

Chiordecone reductase
714
245 AKKHKR 250

715
245 AKKHKR 250

Metaxin 2
716
166 KRKNKA 171

717
166 KRKMKA 171

Paired mesoderm
718
89 KKKRKQRR 96

homebox protein 1
719
88 EKKKRK 93

720
94 QRRNRT 99

721
144 NRRAKF 149

722
88 EKKKRK 93

723
94 QRRNRT 99

724
144 NRRAKF 149

Ring finger protein
725
174 LKRKWZLRC 181

726
8 TRKIKL 13

727
95 MRKQRE 100

728
8 TRKIKL 13

729
95 MRKQRE 100

Ataxin 7
730
55 PRRTRP 60

731
377 GRRKRF 382

732
704 GKKRKN 709

733
834 GKKRKC 839

734
55 PRRTRP 60

735
377 GRRKRF 382

736
704 GKKRKN 709

737
834 GKKRKC 839

Growth-arrest-specific
738
169 ARRRCDRD 176

protein 1

SKAP55 protein
739
115 EKKSKD 120

740
115 EKKSKD 120

Serine palmitoyl-
741
232 PRKARV 237

transferase 1
742
232 PRKARV 237

Serine palmitoyl-
743
334 KKKYKA 339

transferase 2
744
450 RRRLKE 455

745
334 KKKYKA 339

746
450 RRRLKE 455

Synaptopodin
747
405 KRRQRD 410

748
405 KRRQRD 410

Alpha-tectorin
749
1446 TRRCRC 1451

750
2080 IRRKRL 2085

751
1446 TRRCRC 1451

752
2080 IRRKRL 2085

LONG FORM TRANSCRIPTION
753
291 QKRRTLKN 298

FACTOR C-MAF

Usher syndrome type
754
1285 MRRLRS 1290

IIa protein
755
1285 MRRLRS 1290

MSin3A associated
756
95 QKKVKI 100

polypeptied p30
757
124 NRRKRK 129

758
158 LRRYKR 163

759
95 QKKVKI 100

760
124 NRRKRK 129

761
158 LRRYKR 163

Ig delta chain C region
762
142 KKKEKE 147

763
142 KKKEKE 147

THYROID HORMONE
764
383 AKRKADRE 390

RECEPTOR-ASSOCIATED
765
833 KKRHRE 838

PROTEIN COMPLEX
766
833 KKRHRE 838

COMPONENT TRAP100

P60 katanin
767
369 LRRRLEKR 376

768
326 SRRVKA 331

769
326 SRRVKA 331

Transcription factor
770
286 RKRKLERI 293

jun-D
771
273 RKRLRN 278

772
285 CRKRKL 290

773
273 RKRLRN 278

774
285 CRKRKL 290

Sterol/retinol
775
152 VRKARG 157

dehydrogenase
776
152 VRKARG 157

Glycogen [starch]
777
554 DRRFRS 559

synthase liver
778
578 SRRQRI 583

779
554 DRRFRS 559

780
578 SRRQRI 583

Estrogen-related
781
173 TKRRRK 178

receptor gamma
782
353 VKKYKS 358

783
173 TKRRRK 178

784
353 VKKYKS 358

Neural retina-specific
785
162 QRRRTLKN 169

leucine zipper protein

Cytosolic phospholipase
786
514 NKKKILRE 521

A2-gamma
787
31 LKKLRI 36

788
218 FKKGRL 223

789
428 CRRHKI 433

790
31 LKKLRI 36

Cytosolic phospholipase
791
218 FKKGRL 223

A2-gamma
792
428 CRRHKI 433

GLE1
793
415 AKKIKM 420

794
415 AKKIKM 420

Multiple exostoses type
795
296 VRKRCHKH 303

II protein EAXT.2
796
659 RKKFKC 664

797
659 RKKFKC 664

Cyclic-AMP-dependent
798
86 EKKARS 91

transcription factor
799
332 GRRRRT 337

ATF-7
800
344 ERRQRF 349

801
86 EKKARS 91

802
332 GRRRRT 337

803
344 ERRQRF 349

Protein kinase/
804
886 LRKFRT 891

endoribonulcease
805
886 LRKFRT 891

Transcription factor
806
23 RRRCRD 28

E2F6
807
59 VKRPRF 64

808
98 VRKRRV 103

809
117 EKKSKN 122

810
23 RRRCRD 28

811
59 VKRPRF 64

812
98 VRKRRV 103

813
117 EKKSKN 122

MAP kinase-activating
814
1333 IRKKVRRL 1340

death domain protein
815
160 KRRAKA 165

816
943 MKKVRR 948

817
1034 DKRKRS 1039

818
1334 RKKVRR 1339

819
1453 TKKCRE 1458

820
160 KRRAKA 165

821
943 MKKVRR 948

822
1034 DKRKRS 1039

823
1334 RKKVRR 1339

824
1453 TKKCRE 1458

Orphan nuclear receptor
825
126 KRKKSERT 133

PXR
826
87 TRKTRR 92

827
125 IKRKKS 130

828
87 TRKTRR 92

829
125 IKRKKS 130

LENS EPITHELIUM-DERIVED
830
149 RKRKAEKQ 156

GROWTH FACTOR
831
286 KKRKGGRN 293

832
145 ARRGRK 150

833
178 PKRGRP 183

834
285 EKKRKG 290

835
313 DRKRKQ 318

836
400 LKKIRR 405

837
337 VKKVEKKRE 345

838
145 ARRGRK 150

839
178 PKRGRP 183

840
285 EKKRKG 290

841
313 DRKRKQ 318

842
400 LKKIRR 405

LIM homeobox protein
843
255 TKRRKRKN 262

cofactor
844
255 TKRRKR 260

845
255 TKRRKR 260

MULTIPLE MEMBRANE
846
229 WKRIRF 234

SPANNING RECEPTOR TRC8
847
229 WKRIRF 234

Transcription factor
848
172 DKKKLRRL 179

SUPT3H
849
169 MRKDKK 174

850
213 NKRQKI 218

851
169 MRKDKK 174

852
213 NKRQKI 218

GEMININ
853
50 KRKHFN 55

854
104 EKRRKA 109

855
50 KRKHRN 55

856
104 EKRRKA 109

Cell cycle-regulated
857
165 EKKKVSKA 172

factor p78
858
124 IKRKKF 129

859
188 TKRVKK 193

860
381 DRRQKR 386

861
124 IKRKKF 129

862
188 TKRVKK 193

863
381 DRRQKR 386

lymphocyte antigen 6
864
61 QRKGRK 66

complex, locus D
865
85 ARRLRA 90

866
61 QRKGRK 66

867
85 ARRLRA 90

Delta 1-pyrroline-5-
868
455 LRRTRI 460

carboxylate synthetase
869
455 LRRTRI 460

B CELL LINKER PROTEIN
870
36 IKKLKV 41

BLINK
871
36 IKKLKV 41

B CELL LINKER PROTEIN
872
36 IKKLKV 41

BLINK-S
873
36 IKKLKV 41

fetal Alzheimer antigen
874
5 ARRRRKRR 12

875
16 PRRRRRRT 23

876
93 WKKKTSRP 100

877
5 ARRRRK 10

878
16 PRRRRR 21

879
26 PRRPRI 31

880
35 TRRMRW 40

881
5 ARRRRK 10

882
16 PRRRRR 21

883
26 PRRPRI 31

884
35 TRRMRW 40

Transient receptor
885
505 CKKKMRRK 512

potential channel zeta
886
506 KKKMRR 511

splice variant
887
676 HRRSKQ 681

888
506 KKKNRR 511

889
676 HRRSKQ 681

Myofibrillogenesis
890
65 RKRGKN 70

regulator MR-2
891
65 RKRGKN 70

SH2 domain-containing
892
269 IKKRSLRS 276

phosphatase anchor

protein 2c

immunoglobulin super-
893
394 SKRPKN 399

family, member 3
894
394 SKRPKN 399

Meis (mouse) homolog 3
895
112 PRRSRR 117

896
120 WRRTRG 125

897
112 PRRSRR 117

898
120 WRRTRG 125

Deleted in azoospermia 2
899
105 GKKLKL 110

900
114 IRKQKL 119

901
105 GKKLKL 110

902
114 IRKQKL 119

Centaurin gamma3
903
543 NRKKHRRK 550

904
544 RKKHRR 549

905
544 RKKHRR 549

Pre-B-cell leukemia
906
233 ARRKRR 238

transcription factor-1
907
286 NKRIRY 291

908
233 ARRKRR 238

909
286 NKRIRY 291

60S ribosomal protein
910
112 DKKKRM 117

L13a
911
158 KRKEKA 163

912
167 YRKKKQ 172

913
112 DKKKRM 117

914
158 KRKEKA 163

915
167 YRKKKQ 172

WD40-and FYVE-domain
916
388 IKRLKI 393

containing protein 3
917
388 IKRLKI 393

LENG1 protein
918
34 RKRRGLRS 41

919
84 SRKKTRRM 91

920
1 MRRSRA 6

921
33 ERKRRG 38

922
85 RKKTRR 90

923
1 MRRSRA 6

924
33 ERKRRG 38

925
85 RKKTRR 90

MRIP2
926
375 NKKKHLKK 382

G protein-coupled
927
430 EKKKLKRH 437

receptor
928
290 WKKKRA 295

929
395 RKKAKF 400

930
431 KKKLKR 436

931
290 WKKKRA 295

932
395 RKKAKF 400

933
431 KKKLKR 436

934
143 LKKFRQ 148

935
228 LRKIRT 233

936
143 LKKFRQ 148

937
228 LRKIRT 233

938
232 QKRRRHRA 239

939
232 QKRRRH 237

940
232 QKRRRH 237

Sperm ion channel
941
402 QKRKTGRL 409

A-kinase anchoring
942
2232 KRKKLVRD 2239

protein
943
2601 EKRRRERE 2608

944
2788 EKKKKNKT 2795

945
370 RKKNKG 375

946
1763 SKKSKE 1768

947
2200 EKKVRL 2205

948
2231 LKRKKL 2236

949
2601 EKRRRE 2606

950
2785 EKKEKK 2790

951
1992 QKKDVVKRQ 2000

952
370 RKKNKG 375

953
1763 SKKSKE 1768

954
2200 EKKVRL 2205

955
2231 LKRKKL 2236

956
2601 EKRRRE 2606

957
2785 EKKEKK 2790

Lymphocyte-specific
958
315 GKRYKF 320

protein LSP1
959
315 GKRYKF 320

similar to signaling
960
261 RRRGKT 266

lymphocytic activation
961
261 RRRGKT 266

molecule (H. sapiens)

Dermatan-4-
962
242 VRRYRA 247

sulfotransferase-1
963
242 VRRYRA 247

Moesin
964
291 MRRRKP 296

965
325 EKKKRE 330

966
291 MRRRKP 296

967
325 EKKKRE 330

A-Raf proto-oncogene
968
288 KKKVKN 293

serine/threonine-protein
969
358 LRKTRH 363

kinase
970
288 KKKVKN 293

971
358 LRKTRH 363

Cytochrome P450 2C18
972
117 GKRWKE 122

973
117 GKRWKE 122

974
117 GKRWKE 122

975
156 LRKTKA 161

976
117 GKRWKE 122

977
156 LRKTKA 161

Protein tyrosine
978
594 IRRRAVRS 601

phosphatase non-receptor
979
263 FKRKKF 268

type 3
980
388 IRKPRH 393

981
874 VRKMRD 879

982
263 FKRKKF 268

983
388 IRKPRH 393

984
874 VRKMRD 879

similar to kallikrein 7
985
15 VKKVRL 20

(chymotryptic, stratum
986
15 VKKVRL 20

corneum)

Hormone sensitive lipase
987
703 ARRLRN 708

988
703 ARRLRN 708

40S ribosomal protein
989
25 KKKKTGRA 32

S30
990
23 EKKKKK 28

991
23 EKKKKK 28

Zinc finger protein 91
992
617 LRRHKR 622

993
617 LRRHKR 622

NNP-1 protein
994
320 NRKRLYKV 327

995
387 ERKRSRRR 394

996
432 QRRRTPRP 439

997
454 EKKKKRRE 461

998
29 VRKLRK 34

999
355 GRRQKK 360

1000
361 TKKQKR 366

1001
388 RKRSRR 393

1002
454 EKKKKR 459

1003
29 VRKLRK 34

1004
355 GRRQKK 360

1005
361 TKKQKR 366

1006
388 RKRSRR 393

1007
454 EKKKKR 459

Methionyl-tRNA
1008
725 WKRIKG 730

synthetase
1009
725 WKRIKG 730

ELMO2
1010
560 NRRRQERF 567

Meningioma-expressed
1011
432 RKEAKD 437

antigen 6/11
1012
432 RKRAKD 437

Inositol polyphosphate
1013
375 LRKKLHKF 382

4-phosphatase type
1014
829 ARKNKN 834

I-beta
1015
829 ARKNKN 834

1016
815 SKKRKN 820

1017
815 SKKRKN 820

C7ORF12
1018
40 SRRYRG 45

1019
338 HRKNKP 343

1020
40 SRRYRG 45

1021
338 HRKNKP 343

Rap guanine nucleotide
1022
138 SRRRFRKI 145

exchange factor
1023
1071 QRKKRWRS 1078

1024
1099 HKKRARRS 1106

1025
139 RRRFRK 144

1026
661 SKKVKA 666

1027
930 LKRMKI 935

1028
1071 QRKKRW 1076

1029
1100 KKRARR 1105

1030
1121 ARKVKQ 1126

1031
139 RRRFRK 144

1032
661 SKKVKA 666

1033
930 LKRMKI 935

1034
1071 QRKKRW 1076

1035
1100 KKRARR 1105

1036
1121 ARKVKQ 1126

Sigma 1C adaptin
1037
27 ERKKITRE 34

Alsin
1038
883 GRKRKE 888

1039
883 GRKRKE 888

NOPAR2
1040
14 LKRPRL 19

1041
720 VKREKP 725

1042
14 LKRPRL 19

1043
720 VKREKP 725

AT-binding transcription
1044
294 SKRPKT 299

factor 1
1045
961 EKKNKL 966

1046
1231 NKRPRT 1236

1047
1727 DKRLRT 1732

1048
2032 QKRFRT 2037

1049
2087 EKKSKL 2092

1050
2317 QRKDKD 2322

1051
2343 PKKEKG 2348

1052
294 SKRPKT 299

1053
961 EKKNKL 966

1054
1231 NKRPRT 1236

1055
1727 DKRLRT 1732

1056
2032 QKRFRT 2037

1057
2087 EKKSKL 2092

1058
2317 QRKDKD 2322

1059
2343 PKKEKG 2348

Suppressin
1060
232 YKRRKK 237

1061
232 YKRRKK 237

Midline 1 protein
1062
100 TRRERA 105

1063
494 HRKLKV 499

1064
100 TRRERA 105

1065
494 HRKLKV 499

High mobility group
1066
6 PKKPKG 11

protein 2a
1067
84 GKKKKD 89

1068
6 PKKPKG 11

1069
84 GKKKKD 89

This application claims priority to A 1952/2003 filed on Dec. 4, 2003, the entirety of which is hereby incorporated by reference.

Number	Date	Country
WO 9207935	May 1992	WO
WO 9634965	Nov 1996	WO
WO 0220715	Mar 2002	WO

	Number	Date	Country
Parent	11422169	Jun 2006	US
Child	12131311		US

	Number	Date	Country
Parent	PCT/EP2004/013670	Dec 2004	US
Child	11422169		US

GAG binding protein

Information

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Date Filed

Date Issued

Inventors

Original Assignees

Examiners

Agents

CPC

US Classifications

Field of Search

US

International Classifications

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Abstract

Description

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Priority Claims (1)

Parent Case Info

Foreign Referenced Citations (3)

Related Publications (1)

Divisions (1)

Continuations (1)