US20140179900A1 - Treatment of atherosclerosis with cholesterol ester transport protein mimotopes - Google Patents

Treatment of atherosclerosis with cholesterol ester transport protein mimotopes Download PDF

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US20140179900A1
US20140179900A1 US14/086,159 US201314086159A US2014179900A1 US 20140179900 A1 US20140179900 A1 US 20140179900A1 US 201314086159 A US201314086159 A US 201314086159A US 2014179900 A1 US2014179900 A1 US 2014179900A1
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klh
cetp
alum
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Sylvia Brunner
Petra Luehrs
Frank Mattner
Walter Schmidt
Barbara Wittmann
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Affiris AG
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    • C07K7/04Linear peptides containing only normal peptide links
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    • A61K47/64Drug-peptide, drug-protein or drug-polyamino acid conjugates, i.e. the modifying agent being a peptide, protein or polyamino acid which is covalently bonded or complexed to a therapeutically active agent
    • A61K47/643Albumins, e.g. HSA, BSA, ovalbumin or a Keyhole Limpet Hemocyanin [KHL]
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    • A61K47/64Drug-peptide, drug-protein or drug-polyamino acid conjugates, i.e. the modifying agent being a peptide, protein or polyamino acid which is covalently bonded or complexed to a therapeutically active agent
    • A61K47/646Drug-peptide, drug-protein or drug-polyamino acid conjugates, i.e. the modifying agent being a peptide, protein or polyamino acid which is covalently bonded or complexed to a therapeutically active agent the entire peptide or protein drug conjugate elicits an immune response, e.g. conjugate vaccines
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    • CCHEMISTRY; METALLURGY
    • C07ORGANIC CHEMISTRY
    • C07KPEPTIDES
    • C07K7/00Peptides having 5 to 20 amino acids in a fully defined sequence; Derivatives thereof
    • C07K7/04Linear peptides containing only normal peptide links
    • C07K7/06Linear peptides containing only normal peptide links having 5 to 11 amino acids
    • AHUMAN NECESSITIES
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    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K39/00Medicinal preparations containing antigens or antibodies
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    • A61K2039/55511Organic adjuvants
    • A61K2039/55555Liposomes; Vesicles, e.g. nanoparticles; Spheres, e.g. nanospheres; Polymers
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    • A61K2039/55511Organic adjuvants
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    • A61K2039/60Medicinal preparations containing antigens or antibodies characteristics by the carrier linked to the antigen
    • A61K2039/6031Proteins
    • A61K2039/6081Albumin; Keyhole limpet haemocyanin [KLH]

Definitions

  • the invention relates to the prevention and treatment of atherosclerosis, atherosclerosis risk diseases and atherosclerosis sequelae.
  • Atherosclerotic sequelae such as the peripheral arterial occlusion disease, coronary heart disease as well as the apoplectic cerebral insultus, are still among the main causes of death in the United States, Europe, and in large parts of Asia.
  • the development of the atherosclerosis is considered to be a chronic progressive inflammation of the arterial vessel wall which is characterized by a complex interaction of growth factors, cytokines and cell interactions.
  • the “injury” of the endothelium constitutes the initial event of the disease, leading to an endothelial dysfunction which triggers a cascade of cellular interactions culminating in the formation of the atherosclerotic lesions.
  • exogenous and endogenous influences are mentioned which correlate statistically significantly with atherosclerosis.
  • Increased and modified LDL, Lp(a), arterial hypertension, Diabetes mellitus and hyperhomocysteinaemia are, for instance, counted among the most important ones of these endothelium-damaging factors.
  • the endothelium does not constitute a rigid, but much rather an extremely dynamic barrier, a plurality of molecular changes occur in the course of the endothelial dysfunction in addition to an increased permeability for lipoproteins, which molecular changes have a decisive influence on the interaction of monocytes, T-lymphocytes and endothelial cells.
  • endothelial adhesion molecules of the type of the E, L and P selectins, integrins, ICMA-1, VCAM-1 and platelet-endothelial-cell adhesion molecule-1 adhesion of monocytes and T-lymphocytes at the lumen side occurs.
  • the subsequent migration of the leukocytes over the endothelium is mediated by MCP-1, interleukin-8, PDGF, MCSF and osteopontin.
  • macrophages and monocytes resident in the intima are capable of taking up the penetrated LDL particles and to deposit them as vacuoles of cholesterol esters in the cytoplasma.
  • LDL are lipoproteins of low density and are formed by catabolic effects of lipolytic enzymes from VLDL particles rich in triglyceride. Besides their damaging properties on endothelial cells and smooth muscle cells of the media, LDL moreover has a chemotactic effect on monocytes and is capable of increasing the expression of MCSF and MCP-1 of the endothelial cells via gene amplification.
  • HDL is capable of taking up cholesterol esters from loaded macrophages mediated by apolipoprotein E, under formation of so-called HDLc complexes.
  • these cholesterol ester-loaded particles are capable of binding to hepatocytes or to cells of the adrenal cortex and delivering cholesterol for the production of bile acids and steroids, respectively.
  • This mechanism is called reverse cholesterol transport and elucidates the protective function of HDL.
  • Activated macrophages are capable of presenting antigens via HLA-DR and thereby activate CD4 and CD8 lymphocytes which, consequently, are stimulated to secrete cytokines, such as IFN-gamma and TNF-alpha, and moreover, contribute to increasing the inflammatory reaction.
  • smooth muscle cells of the media start to grow into the region of the intima which has been altered by inflammation.
  • the intermediary lesion forms at this stage.
  • the progressive and complicated lesion will develop over time, which is morphologically characterized by a necrotic core, cellular detritus and a fibrinous cap rich in collagen on the side of the lumen. If the cell number and the portion of the lipoids increase continuously, tears in the endothelium will occur, and surfaces with thrombotic properties will be exposed. Due to the adhesion and activation of thrombocytes at these tears, granules will be released which contain cytokines, growth factors and thrombin.
  • Proteolytic enzymes of the macrophages are responsible for the thinning of the fibrinous cap which, at last, will lead to a rupture of the plaques with consecutive thrombosis and stenosing of the vessels and an acute ischemia of the terminal vessels.
  • Hyperlipoproteinemia A disease which involves an excessive increase in the total and LDL cholesterol is the familial hypercholesterinemia (FH). It belongs to the most frequent monogenetically inherited metabolic diseases. The moderate heterozygous form occurs with a frequency of 1:500, the homozygous form with 1:1 million clearly more rarely.
  • FH familial hypercholesterinemia
  • causes of the familial hypercholesterinemia are mutations in the LDL receptor gene on the short arm of chromosome 19. These mutations may be deletions, insertions or point mutations.
  • the characteristic finding of the lipoproteins in familial hypercholesterinemia is an increase in the total and LDL cholesterol at mostly normal triglyceride and VLDL concentrations. Often the HDL is lowered. Phenotypically, there is a type IIAa-hyperlipoproteinemia. In the heterozygous form, the total cholesterol is increased by the two to three-fold, in the homozygous form it is increased by the five to six-fold as compared to the normal level. Clinically the familial hypercholesterinemia manifests itself by an early coronary sclerosis. As a rule, in heterozygous men the first symptoms of a coronary heart disease (CHD) occur between their 30 th and the 40 th year of age, in women on an average 10 years later.
  • CHD coronary heart disease
  • LDL lipoprotein
  • IDL intermediate-density lipoproteins
  • LDL low-density lipoproteins
  • HDL high-density lipoproteins
  • Lp(a) lipoprotein
  • the core is formed by esterified cholesterol molecules.
  • This highly hydrophobic core is surrounded by an envelope of phospholipids, non-esterified cholesterol and one single Apo B100 molecule.
  • Apoprotein E is found on the surface of the LDL particles.
  • the function of the LDL consists in transporting cholesterol to peripheral tissues where—mediated by the apoprotein B-100—it is taken up into the cells via the LDL receptor.
  • LDL cholesterol levels of higher than 160 mg/dl constitute a high cardiovascular risk.
  • the level of the vessel-protecting HDL cholesterol plays an important role when estimating the risk profile for cardiovascular diseases.
  • Lipoprotein(a) (Lp(a)) has a density of 1.05 to 1.12 g/ml and resembles LDL in its composition. Besides apoprotein B-100, its protein portion consists of the apoprotein(a) which is characteristic of Lp(a). To date, very little is known about the physiology and function of the Lp(a). Since the apoprotein(a) molecule has a high sequence homology to plasminogen, it is assumed that Lp(a) both promotes the formation of thrombi on atherosclerotic plaques and also has an atherogenic effect.
  • Lp(a) is found together with apoprotein B in atherosclerotic lesions. Retrospective studies have shown a correlation between increased Lp(a) and a CHD. Likewise, the metaanalysis of numerous prospective studies has shown that Lp(a) is an independent risk factor for the occurrence of a CHD. Levels of between 15 and 35 mg/dl are considered to be normal. So far, Lp(a) can be influenced neither by diet nor by medicaments. Therefore, therapy measures are restricted to reducing further risk factors. In particular, a lowering of the LDL cholesterol seems to lower the cardiovascular risk of Lp(a). In the pathogenesis of atherosclerosis, considerable pathophysiologic importance is, moreover, attributed to coagulation factors.
  • the cholesterol ester transfer protein (CETP) is a stable plasma glycoprotein which is responsible for the transfer of neutral lipids and phospholipids between lipoproteins and which down-regulates the plasma concentration of HDL.
  • the inhibition of the CETP lipid transfer activity has already been suggested as a therapeutic approach for increasing the HDL plasma level.
  • CETP lowers the HDL concentration by the transfer of cholesterol esters from HDL to LDL and VLDL.
  • the transient inhibition of CETP with anti-CETP monoclonal antibodies, antisense oligonucleotides or CETP inhibitors led to the increase in the HDL levels.
  • Lasting CETP inhibition with antisense oligonucleotides increased the HDL levels and, thus, led to a reduction of the atherosclerotic lesions in the rabbit animal model for atherosclerosis.
  • polypeptides and their analogues are described which are capable of inhibiting CETP that catalyses the transfer of cholesterol esters from HDL to VLDL and LDL, and, therefore, have anti-atherosclerotic activity if administered to a patient.
  • a CETP polypeptide inhibitor is derived from apolipoprotein C-I of various sources, wherein especially N-terminal fragments up to amino acid 36 have been identified as CETP inhibitors.
  • a CETP-binding peptide which is capable of inhibiting the activity of CETP in an individual.
  • the CETP-inhibitory protein comprises an N-terminal fragment of porcine apolipoprotein C-III.
  • peptides which are derived from CETP and comprise T-cell and/or B-cell epitopes. These peptides are able to induce in vivo the formation of CETP specific antibodies.
  • peptides are disclosed which, because of the induction of a CETP-specific immune response, can be used for the treatment and prevention of cardiovascular diseases, such as, e.g., atheroslerosis.
  • These peptides comprise a T helper cell epitope which is not derived from CETP, and at least one B-cell epitope that comes from CETP and can be derived directly from the latter.
  • the T helper cell epitope advantageously is derived from tetanus toxoid and is covalently bound to at least one B-cell epitope of CETP.
  • CETP mimotopes to be used for the manufacture of a medicament for the treatment or prevention of atherosclerosis is described.
  • the problem with the CETi-1 vaccine is that it uses endogenous antigen.
  • the human immune system is tolerant relative to endogenous structures, since with most of the endogenous molecules—other than with CETP—it is vital that no autoantibodies be formed. Thus, it was the object of the CETi-1 vaccine to break the endogenous tolerance which, apparently, it has not achieved to a sufficient extent.
  • antigens for an anti-CETP vaccine which are selected such that they are considered as foreign by the immune system and therefore need not break a self-tolerance.
  • These antigens may be used for preventing and/or treating atherosclerosis, atherosclerosis risk diseases and atherosclerosis sequelae.
  • FIG. 1 shows the result of a representative competition ELISA after screening phage display library Ph.D. 7 with monoclonal antibody “Paula”.
  • FIGS. 2 a and 2 b show the results of 2 typical competition ELISAs after screening phage display library Ph.D. 12 with monoclonal antibody “Paula”.
  • FIGS. 3 a and 3 b show the results of 2 representative competition ELISAs after screening phage display library Ph.D. 7 with mAb Frida.
  • FIG. 4 a shows the result of a representative competition ELISA after screening phage display library Ph.D. 12 with monoclonal antibody “Frida”.
  • FIG. 4 b shows binding of monoclonal antibody “Frida” to ELISA plates coated with mimotope-BSA.
  • FIGS. 5 a and 5 b show the results of a representative competition ELISA after screening phage display library Ph.D. 12 with monoclonal antibody “Frida”.
  • FIG. 6 shows the results of a competition ELISA of two mimotopes after screening phage display library Ph.D. 12 with monoclonal antibody “Frida”.
  • FIGS. 7 a , 7 b , 7 c and 7 d show the antibody titer (anti mouse IgG) of in vivo experiments, whereby the following mimotope-BSA conjugates were injected into mice.
  • FIGS. 8 a and 8 b show the results of two representative competition ELISA after screening phage display library Ph.D. 7C7 with monoclonal antibody “Frida”.
  • FIG. 9 shows an in vitro ELISA test for the detection of the binding between “Frida” and cyclic mimotopes.
  • FIGS. 10 a and 10 b show the results of an inhibition ELISA assay with FGFPSHLIIDWLQSLS (SEQ ID NO. 179), FGFPAHVFIDWLQSLS (SEQ ID NO. 222) and FGFPAHVYIDWLQSLS (SEQ ID NO. 223).
  • FIG. 11 shows the in vivo induction of antibodies directed to CETP by mimotopes of the invention that are administered to mice.
  • FIGS. 12 a and 12 b show the in vivo induction of CETP specific antibodies by the administration of the mimotopes of the invention.
  • FIG. 13 shows the in vivo induction of antibodies directed to CETP by mimotopes of the invention that are administered to mice.
  • FIG. 14 shows a CETP activity assay, wherein 0.6 ⁇ l human serum (with endogenous CETP activity) is mixed with serum from wild-type mice (not containing CETP activity) vaccinated with KLH/Alum (negative control group), p4703-KLH/Alum (original CETP epitope), or p4361 (or p4362 or p 4325) mimotope, respectively.
  • FIG. 15 shows that the addition of p4325-KLH/Alum to human serum inhibits significantly CETP activity.
  • FIG. 16 shows that the addition of p4361-KLH/Alum to human serum inhibits significantly CETP activity.
  • FIG. 17 shows that the addition of p4362-KLH/Alum to human serum inhibits significantly CETP activity.
  • FIG. 18 a shows an inhibition ELISA with mimotopes (Coat. 1 ⁇ M 4073 peptide, detection ⁇ IgG1).
  • FIG. 18 b shows an inhibition ELISA with mimotopes (Coat. 1 ⁇ M 4073 peptide, detection ⁇ IgG1).
  • FIG. 18 c shows a inhibition ELISA with mimotopes screen PhD12 Frida and Ala-exchange for mimotope characterisation/mAb Frida (Coat 1 ⁇ M 4073. Detection ⁇ IgG1.)
  • FIG. 19 a shows a peptide ELISA, immunisation with C-DFGFPAHVYIDWLQSLS (p4628-KLH/Alum) (SEQ ID NO. 236), titre to original epitope.
  • FIG. 19 b shows a peptide ELISA, immunisation with C-FGFPAHVFIDWLQSLN (p4474-KLH/Alum) (SEQ ID NO. 230), titre to original epitope.
  • FIG. 19 c shows a peptide ELISA, immunisation with C-FGFPAHVFIDWLQSLN (p4474-KLH/Alum) (SEQ ID NO. 230), titre to injected mimotope.
  • FIG. 19 d shows an anti-protein ELISA.
  • Mice were injected 3 times with 30 ⁇ g of the indicated mimotopes coupled to KLH with Alum as adjuvant.
  • Sera from each group (comprising 5 mice) were pooled, diluted 1:100 and tested on ELISA plates coated with purified rabbit CETP.
  • FIG. 19 e shows an anti-protein ELISA, wherein mice were injected 3 times with 30 ⁇ g of the indicated mimotopes coupled to KLH with Alum as adjuvant. Mouse sera (from single mice) were diluted 1:100 and tested on ELISA plates coated with purified rabbit CETP.
  • the present invention relates to the use of a compound comprising the amino acid sequence
  • Z 1 is an amino acid residue other than C
  • X 1 is an amino acid residue selected from the group consisting of D, A, R, E, S, N, T and G
  • X 2 is an amino acid residue selected from the group consisting of F, A, W, R, S, L, Q, V and M
  • X 3 is an amino acid residue selected from the group consisting of L, A, S, W, E, R, I and H
  • X 4 is an amino acid residue selected from the group consisting of Q, A, H, D, K, R, S and E
  • Z 2 is an amino acid residue other than C
  • n is an integer between 0 and 10, preferably between 0 and 9
  • m is an integer between 0 and 3
  • TMAFPLN SEQ ID NO. 3
  • HYHGAFL SEQ ID NO. 4
  • EHHDIFL SEQ ID NO. 5
  • TGLSVFL SEQ ID NO. 6
  • WMPSLFY SEQ ID NO. 7
  • SMPWWFF SEQ ID NO. 8
  • TMPLLFW SEQ ID NO. 9
  • DTWPGLE SEQ ID NO. 10
  • SMPPIFY SEQ ID NO. 11
  • MPLWWWD SEQ ID NO. 12
  • SMPNLFY SEQ ID NO. 13
  • RMPPIFY SEQ ID NO. 14
  • NPFEVFL SEQ ID NO. 15
  • TLPNWFW SEQ ID NO. 16
  • SMPLTFY SEQ ID NO.
  • SEQ ID NO. 17 SPHPHFL (SEQ ID NO. 18), NFMSIGL (SEQ ID NO. 19), SQFLASL (SEQ ID NO. 20), WSWPGLN (SEQ ID NO. 21), IAWPGLD (SEQ ID NO. 22), SKFMDTL (SEQ ID NO. 23), SMPMVFY (SEQ ID NO. 24), YEWVGLM (SEQ ID NO. 25), KGFLDHL (SEQ ID NO. 26), HQSDDKMPWWFF (SEQ ID NO. 27), YVWQDPSFTTFF (SEQ ID NO. 28), YVWQDPSFTTFF (SEQ ID NO. 29), LPQTHPLHLLED (SEQ ID NO.
  • the present invention provides CETP mimotopes for these purposes. These mimotopes are able to induce antibodies which are able to inhibit CETP enzyme activity.
  • the CETP mimotopes according to the present invention preferably are antigenic polypeptides which in their amino acid sequence vary from the amino acid sequence of CETP or of fragments of CETP.
  • the inventive mimotopes may comprise one or more non-natural amino acids (i.e. not from the 20 “classical” amino acids) or they may be completely assembled of such non-natural amino acids.
  • inventive antigens which induce anti-CETP antibodies may be assembled of D- or L-amino acids or of combinations of DL-amino acids and, optionally, they may have been changed by further modifications, ring closures or derivatizations.
  • Suitable anti-CETP-antibody-inducing antigens may be provided from commercially available peptide libraries.
  • these peptides are at least 4 amino acid residues in length, in particular at least 7 amino acids, and preferred lengths may be up to 16, preferably up to 14 or 20 amino acids (e.g. 5 to 16 amino acid residues).
  • the mimotopes of the present invention may also be part of a polypeptide and consequently comprising at their N- and/or C-terminus at least one further amino acid residue.
  • the mimotopes of the present invention are capable to bind to antibodies which may be obtained by administration of C-FGFPEHLLVDFLQSLS (SEQ ID NO. 146) (16 C-terminal amino acids of CETP protein) coupled to KLH or other carriers to mammals. Once administered to a mammal the mimotopes are able to induce a corresponding immune response, so that antibodies directed against CETP are produced in said mammal.
  • CETP-mimotopes i.e. anti-CETP-antibody-inducing antigens
  • the CETP-mimotopes (i.e. anti-CETP-antibody-inducing antigens) of the present invention can be identified and prepared by various methods, including phage libraries or peptide libraries. They can be produced and identified for instance by means of combinatorial chemistry or by means of high throughput screening techniques for the most varying structures (Display: A Laboratory Manual by Carlos F. Barbas (Editor), et al.; Willats W G Phage display: practicalities and prospects. Plant Mol. Biol. 2002; 50(6):837-54).
  • anti-CETP-antibody-inducing antigens based on nucleic acids may be employed, and these, too, may be found with the most varying (oligonucleotide) libraries (e.g. with 2-180 nucleic acid residues) (e.g. Burgstaller et al., Curr. Opin. Drug Discov. Dev. 5(5) (2002), 690-700; Famulok et al., Acc. Chem. Res. 33 (2000), 591-599; Mayer et al., PNAS 98 (2001), 4961-4965, etc.).
  • oligonucleotide libraries e.g. with 2-180 nucleic acid residues
  • the nucleic acid backbone can be provided e.g. by the natural phosphor-diester compounds, or also by phosphorotioates or combinations or chemical variations (e.g. as PNA), wherein as bases, according to the invention primarily U, T, A, C, G, H and mC can be employed.
  • the 2′-residues of the nucleotides which can be used according to the present invention preferably are H, OH, F, Cl, NH 2 , O-methyl, O-ethyl, O-propyl or O-butyl, wherein the nucleic acids may also be differently modified, i.e.
  • aptamer-based anti-CETP-antibody-inducing antigens are also preferred anti-CETP-antibody-inducing antigens within the scope of the present invention.
  • the term “mimotope” refers to a molecule which has a conformation that has a topology equivalent to the epitope of which it is a mimic.
  • the mimotope binds to the same antigen-binding region of an antibody which binds immunospecifically to a desired antigen.
  • the mimotope will elicit an immunological response in a host that is reactive to the antigen to which it is a mimic.
  • the mimotope may also act as a competitor for the epitope of which it is a mimic in in vitro inhibition assays (e.g. ELISA inhibition assays) which involve the epitope and an antibody binding to said epitope.
  • a mimotope of the present invention may not necessarily prevent or compete with the binding of the epitope of which it is a mimic in an in vitro inhibition assay although it is capable to induce a specific immune response when administered to a mammal.
  • epitope refers to an immunogenic region of an antigen which is recognized by a particular antibody molecule.
  • an antigen will possess one or more epitopes, each capable of binding an antibody that recognizes the particular epitope.
  • Amino Acid 3-Letter Code 1-Letter Code Alanine Ala A Arginine Arg R Asparagine Asn N Aspartic Asp D Cysteine Cys C Glutamic Glu E Glutamine Gln Q Glycine Gly G Histidine His H Isoleucine Ile I Leucine Leu L Lysine Lys K Methionine Met M Phenylalanine Phe F Proline Pro P Serine Ser S Threonine Thr T Tryptophan Trp W Tyrosine Tyr Y Valine Val V
  • the mimotopes of the present invention can be synthetically produced by chemical synthesis methods which are well known in the art, either as an isolated peptide or as a part of another peptide or polypeptide.
  • the peptide mimotope can be produced in a microorganism which produces the peptide mimotope which is then isolated and if desired, further purified.
  • the peptide mimotope can be produced in microorganisms such as bacteria, yeast or fungi, in eukaryote cells such as a mammalian or an insect cells, or in a recombinant virus vector such as adenovirus, poxvirus, herpesvirus, Simliki forest virus, baculovirus, bacteriophage, Sindbis virus or sendai virus.
  • Suitable bacteria for producing the peptide mimotope include E. coli, B. subtilis or any other bacterium that is capable of expressing peptides such as the peptide mimotope.
  • Suitable yeast types for expressing the peptide mimotope include Saccharomyces cerevisiae, Schizosaccharomyces pombe, Candida, Pichia pastoris or any other yeast capable of expressing peptides. Corresponding methods are well known in the art. Also methods for isolating and purifying recombinantly produced peptides are well known in the art and include e.g. as gel filtration, affinity chromatography, ion exchange chromatography etc.
  • a fusion polypeptide may be made wherein the peptide mimotope is translationally fused (covalently linked) to a heterologous polypeptide which enables isolation by affinity chromatography.
  • Typical heterologous polypeptides are His-Tag (e.g. His 6 ; 6 histidine residues), GST-Tag (Glutathione-S-transferase) etc.
  • His-Tag e.g. His 6 ; 6 histidine residues
  • GST-Tag Glutathione-S-transferase
  • the fusion polypeptide may comprise a cleavage site at the junction between the peptide mimotope and the heterologous polypeptide.
  • the cleavage site consists of an amino acid sequence that is cleaved with an enzyme specific for the amino acid sequence at the site (e.g. proteases).
  • the mimotopes of the present invention may also modified at or nearby their N- and/or C-termini so that at said positions a cysteine residue is bound thereto.
  • terminally positioned (located at the N- and C-termini of the peptide) cysteine residues are used to cyclize the peptides through a disulfide bond.
  • the mimotopes of the present invention may also be used in various assays and kits, in particular in immunological assays and kits. Therefore, it is particularly preferred that the mimotope may be part of another peptide or polypeptide, particularly an enzyme which is used as a reporter in immunological assays.
  • reporter enzymes include e.g. alkaline phosphatase or horseradish peroxidase.
  • amysclerosis sequelae or “sequelae of atherosclerosis” refers to the diseases which are a consequence of atherosclerose. These diseases include among others peripheral arterial occlusive disease, coronary heart disease and apoplectic cerebral insultus (see e.g. Steinberg D. J. Lipid Res. (2005) 46: 179-190; Steinberg D et al. J. Lipid Res (2006) 47: 1339-1351).
  • X 1 is D and X 4 is Q or H, preferably Q.
  • Such a molecule preferably comprises at its N-terminus further amino acid residues having the sequence X a X b X c X d X e X f (SEQ ID NO. 41), wherein X a is P, Y, T or K, X b is an amino acid residue other than C, X c is H, X d is Y, L, H, V, T, I or F, X e is Y, I, P, L, Q, S, R, T, F or A and X f is A, W, V, Q, L, S, I, R or T.
  • n is 7, 8 or 9
  • Z 1 is an amino acid residue other than C or selected from the group consisting of F, G, F, A, P, W, Y, S, G, D, L, E, K, T, P, I and M, preferably from the group consisting of F, G, F, A, P, Y, T, S, G, K and D
  • Z 2 is selected from the group consisting of S, L, A, W, L, N, T, I, Y and H.
  • X 1 is selected from the group consisting of D, A, R, E and L
  • X 2 is selected from the group consisting of F
  • X 3 is selected from the group consisting of L
  • a and S is selected from the group consisting of Q, A and H.
  • X 1 is D
  • X 2 is selected from the group consisting of F, Q and W
  • X 3 is L or S
  • X 4 is Q or H.
  • the compound comprises the amino acid sequence FX 8 (F) o PX 9 HX 10 X 11 X 12 DX 2 X 3 X 4 X 5 X 6 X 7 (SEQ ID NO. 42), wherein
  • X 8 is selected from the group consisting of G, A, F, Y and K
  • X 9 is selected from the group consisting of E, Y, A, Q, K and S
  • X 10 is selected from the group consisting of H, V, L, F and I
  • X 11 is selected from the group consisting of L, W, S, I, F and Y
  • X 12 is V, T, F or I
  • X 5 is S or Y
  • X 6 is L, A or I
  • X 7 is S, N or T
  • o 0 or 1.
  • the compound of the present invention comprises preferably the amino acid sequence X 1 X 2 X 3 X 4 X 5 X 6 X 7 (SEQ ID NO. 43), wherein X 1 is selected from the group consisting of D, S, N, T and G, X 2 is F, X 3 is L, X 4 is selected from the group consisting of Q, D, K, R, S and E, X 5 is S or T, X 6 is L and X 7 is an amino acid residue other than C, preferably selected from the group consisting of S, T, A, M, F and W.
  • the amino acid sequence is selected from the group consisting of SSLELFL (SEQ ID NO. 44), SFLDTLT (SEQ ID NO. 45), NFLKTLS (SEQ ID NO. 46), DFLRTLT (SEQ ID NO. 47), AFLDTLV (SEQ ID NO. 48), TFLSSLA (SEQ ID NO. 49), GFLDSLM (SEQ ID NO. 50), SPHPHFL (SEQ ID NO. 51), SNFLKTL (SEQ ID NO. 52), TGFLATL (SEQ ID NO. 53), SDFLRAL (SEQ ID NO. 54), SANPRDFLETLF (SEQ ID NO. 55), RMFPESFLDTLW (SEQ ID NO.
  • TIYDSFLDSLAS SEQ ID NO. 57
  • KPYLLKDFLEAL SEQ ID NO. 58
  • AMGPYDALDLFL SEQ ID NO. 59
  • TWNPIESFLESL SEQ ID NO. 60
  • QYQTPLTFLEAL SEQ ID NO. 61
  • RHISPATFLEAL SEQ ID NO. 62
  • HTDSFLSTFYGD SEQ ID NO. 63
  • ADSTFTSFLQTL SEQ ID NO. 64
  • GPVSIYADTDFL SEQ ID NO. 65
  • DSNDTLTLAAFL SEQ ID NO. 66
  • TPTHYYADFSQL SEQ ID NO. 67
  • LPGHLIWDSLHY SEQ ID NO.
  • LPGHLIWDSLHSL SEQ ID NO. 91
  • LPGHLIWDSLHSLS SEQ ID NO. 92
  • GLPGHLIWDSLHYL SEQ ID NO. 93
  • GLPGHLIWDSLHSL SEQ ID NO. 94
  • FGLPGHLIWDSLHSLS SEQ ID NO. 95
  • FGFPGHLIWDSLHSLS SEQ ID NO. 96
  • LPQTHPLHLLED SEQ ID NO. 97
  • IPYHHLVDQLHH SEQ ID NO. 98
  • IPYHHLVDQLHLS SEQ ID NO. 99
  • IPYHHLVDQLHSLS SEQ ID NO. 100
  • FGIPYHHLVDQLHHLS SEQ ID NO.
  • GIPSHHLQDSLQLL SEQ ID NO. 111
  • FGIPSHHLQDSLQLLS SEQ ID NO. 112
  • FGFPSHHLQDSLQSLS SEQ ID NO. 113
  • EYAHHTSLDLRQ SEQ ID NO. 114
  • EPLHFRSDRIQA SEQ ID NO. 115
  • EPLHFRSDRIQALS SEQ ID NO. 116
  • EPLHFRSDRIQSLS SEQ ID NO. 117
  • GEPLHFRSDRIQAL SEQ ID NO. 118
  • FGEPLHFRSDRIQALS SEQ ID NO. 119
  • FGFPLHFRSDRIQSLS SEQ ID NO. 120
  • APKHLYADMSQA SEQ ID NO.
  • APKHLYADMSQALS SEQ ID NO. 122
  • APKHLYADMSQSLS SEQ ID NO. 123
  • GAPKHLYADMSQAL SEQ ID NO. 124
  • FGFPKHLYADMSQSLS SEQ ID NO. 125
  • MPAHLSRDLRQS SEQ ID NO. 126
  • MPAHLSRDLRQSL SEQ ID NO. 127
  • MPAHLSRDLRQSLS SEQ ID NO. 128)
  • GMPAHLSRDLRQSL SEQ ID NO. 129
  • FGFPAHLSRDLRQSLS SEQ ID NO. 130
  • NPKHYSIDRHQA SEQ ID NO. 131
  • TPFHFAQDSWQW SEQ ID NO.
  • TPFHFAQDSWQWLS SEQ ID NO. 133
  • TPFHFAQDSWQSLS SEQ ID NO. 134
  • GTPFHFAQDSWQWL SEQ ID NO. 135)
  • FGFPFHFAQDSWQSLS SEQ ID NO. 136
  • ACSFAYLYRC SEQ ID NO. 137
  • ACFMGDKWVC SEQ ID NO. 138
  • ACVLYPKAIC SEQ ID NO. 139
  • ACYMGQQFVC SEQ ID NO. 140
  • ACLTAYLHWC SEQ ID NO. 141
  • ACTLFPVAYC SEQ ID NO. 142
  • ACWLFPYAHC SEQ ID NO. 143
  • ACKSINMWLC SEQ ID NO.
  • FGFPEHALVDFLQSLS (SEQ ID NO. 155), FGFPEHLAVDFLQSLS (SEQ ID NO. 156), FGFPEHLLADFLQSLS (SEQ ID NO. 157), FGFPEHLLVAFLQSLS (SEQ ID NO. 158), FGFPEHLLVDALQSLS (SEQ ID NO. 159), FGFPEHLLVDFAQSLS (SEQ ID NO. 160), FGFPEHLLVDFLASLS (SEQ ID NO. 161), FGFPEHLLVDFLQALS (SEQ ID NO. 162), FGFPEHLLVDFLQSAS (SEQ ID NO. 163), FGFPEHLLVDFLQSLA (SEQ ID NO.
  • FAFPAHLLVDFLQALA SEQ ID NO. 165
  • AAFPAHLLADFLQALA SEQ ID NO. 166
  • SPQHLTTDRAQA SEQ ID NO. 167
  • SPQHLTTDRAQALS SEQ ID NO. 168
  • SPQHLTTDRAQSLS SEQ ID NO. 169
  • GSPQHLTTDRAQAL SEQ ID NO. 170
  • FGFPQHLTTDRAQSLS SEQ ID NO. 171
  • FGFPQHLTTDWAQSLS SEQ ID NO. 172
  • FGFPQHLTTDRLQSLS SEQ ID NO. 173
  • FGFPQHLTTDWLQSLS SEQ ID NO.
  • ATPSHLIIDRAQ SEQ ID NO. 175)
  • ATPSHLIIDRAQSLS SEQ ID NO. 176
  • FGFPSHLIIDRAQSLS SEQ ID NO. 177
  • FGFPSHLIIDWAQSLS SEQ ID NO. 178
  • FGFPSHLIIDWLQSLS SEQ ID NO. 179
  • FGFPSHLIIDWSQSLS SEQ ID NO. 180
  • FATPSHLIIDWLQSLS SEQ ID NO. 181), FKPAHVSIDWLQ (SEQ ID NO. 182)
  • FKPAHVSIDWLQSLS SEQ ID NO. 183
  • FGFPAHVSIDWLQSLS SEQ ID NO.
  • FGFPAHVSIRWLQSLS (SEQ ID NO. 195), FGFPAHVSIEWLQSLS (SEQ ID NO. 196), FGFPAHVSIDWLNSLS (SEQ ID NO. 197), FGFPAHVSIDWLHSLS (SEQ ID NO. 198), AGFPAHVSIDWLQSLS (SEQ ID NO. 199), PGFPAHVSIDWLQSLS (SEQ ID NO. 200), WGFPAHVSIDWLQSLS (SEQ ID NO. 201), FAFPAHVSIDWLQSLS (SEQ ID NO. 202), FSFPAHVSIDWLQSLS (SEQ ID NO. 203), FYFPAHVSIDWLQSLS (SEQ ID NO.
  • FAFPAHVFIDWLQALA SEQ ID NO. 215)
  • FGFPAHVSIDRAQSLS SEQ ID NO. 216
  • FGFPTHVSIDWLQSLS SEQ ID NO. 217)
  • FGFPFHVSIDWLQSLS SEQ ID NO. 2148
  • FGFPAHISIDWLQSLS SEQ ID NO. 219
  • FGFPAHIIIDWLQSLS SEQ ID NO. 220
  • FGFPAHLTTDWLQSLS SEQ ID NO. 221
  • FGFPAHVFIDWLQSLS SEQ ID NO. 222
  • FGFPAHVYIDWLQSLS SEQ ID NO. 223
  • FGFPAHVSLDWLQSLS SEQ ID NO.
  • FGFPAHVSADWLQSLS (SEQ ID NO. 225), TPTHYYADFSQSLS (SEQ ID NO. 226), FGFPAHVSIDWSQSLS (SEQ ID NO. 227), FGFPAHVSIDFSQSLS (SEQ ID NO. 228), FGFPSHIIIDWLQSLS (SEQ ID NO. 239), FGFPSHLIIEWLQSLS (SEQ ID NO. 240), AAFPAHLLADAAQALA (SEQ ID NO. 241), AAFPAHAAADFLQALA (SEQ ID NO. 242), AAFAAHLLADFLQAAA (SEQ ID NO. 243), AAAPAHLLVDAAQAAA (SEQ ID NO.
  • FAFPAHVFIDWLQSLS (SEQ ID NO. 245); FGFPAHVFIDWLQALS (SEQ ID NO. 246), FGFPAHVFIDWLQSLA (SEQ ID NO. 247), GFPAHVFIDWLQSLS (SEQ ID NO. 248), FPAHVFIDWLQSLS (SEQ ID NO. 249), PAHVFIDWLQSLS (SEQ ID NO. 250), FAFPAHVFIDWLQALA (SEQ ID NO. 251), FGFPEHLFVDFLQSLS (SEQ ID NO. 252), FGFPAHVHIDWLQSLS (SEQ ID NO. 253), FGFPAHVPIDWLQSLS (SEQ ID NO.
  • FGFPSHLFIDWAQSLS (SEQ ID NO. 255), PGFPAHVFIDWLQLIT (SEQ ID NO. 256), PAHVYIDWLQSLS (SEQ ID NO. 257), FGFPAHVYIDWLQ (SEQ ID NO. 258), FGFPAHVFIDWLQ (SEQ ID NO. 259), DFGFPSHLIIDWLQSLS (SEQ ID NO. 235), DFGFPAHVFIDWLQSLN (SEQ ID NO. 260), PSHLIIDWLQ (SEQ ID NO. 261), PAHVFIDWLQ (SEQ ID NO. 262), DFGFPAHVTIDWLQSLN (SEQ ID NO. 263), DFGFPAHVLIDWLQSLN (SEQ ID NO. 264), FGFPAHVFIDWLQSLN (SEQ ID NO. 230) and FGFPAHVFIDWLQSLA (SEQ ID NO. 265).
  • Particularly preferred mimotopes to be used according to the present invention are SANPRDFLETLF (SEQ ID NO. 55), RMFPESFLDTLW (SEQ ID NO. 56), SFLDTLT (SEQ ID NO. 45), NFLKTLS (SEQ ID NO. 46), DFLRTLT (SEQ ID NO. 47), TFLSSLA (SEQ ID NO. 49), GFLDSLM (SEQ ID NO. 50), FGFPYHVQVDVLQSLS (SEQ ID NO. 107), FGFPSHLIIDRAQSLS (SEQ ID NO. 177), FKPAHVSIDWLQSLS (SEQ ID NO. 183), FGFPAHVSIDWLQSLS (SEQ ID NO.
  • FGFPQHLTTDRAQSLS (SEQ ID NO. 171), FGFPTHYYADFSQSLS (SEQ IN NO. 87), FGFPGHLIWDSLHSLS (SEQ ID NO. 96), FGFPYHHLVDQLHSLS (SEQ ID NO. 102), FGFPSHHLQDSLQSLS (SEQ ID NO. 113), FGFPLHFRSDRIQSLS (SEQ ID NO. 120), FGFPKHLYADMSQSLS (SEQ ID NO. 125), FGFPAHLSRDLRQSLS (SEQ ID NO. 130) and FGFPFHFAQDSWQSLS (SEQ ID NO. 136).
  • Especially preferred mimotopes of the present invention are FGFPSHLIIDWLQSLS (SEQ ID NO. 179), FGFPAHVFIDWLQSLS (SEQ ID NO. 222) and FGFPAHVYIDWLQSLS(SEQ ID NO. 223).
  • mimotopes are FGFPAHVWIDWLQSLS (SEQ ID NO. 229), FGFPAHVFIDWLQSLN (SEQ ID NO. 230), FGFPAHFSIDWLQSLS (SEQ ID NO. 231), FGFPAHVSFDWLQSLS (SEQ ID NO. 232), FGFPEHVFIDWLQSLS (SEQ ID NO. 233), DFGFPAHVFIDWLQSLS (SEQ ID NO. 234), DFGFPSHLIIDWLQSLS (SEQ ID NO. 235), DFGFPAHVYIDWLQSLS (SEQ ID NO. 236), FGFPQHLFTDWLQSLS (SEQ ID NO. 237) and FGFPKHLLVDFLQSLS (SEQ ID NO. 238).
  • the compound is coupled to a pharmaceutically acceptable carrier, preferably KLH (Keyhole Limpet Hemocyanin), tetanus toxoid, albumin-binding protein, bovine serum albumin, a dendrimer (MAP; Biol. Chem. 358: 581), peptide linkers (or flanking regions) as well as the adjuvant substances described in Singh et al., Nat. Biotech. 17 (1999), 1075-1081 (in particular those in Table 1 of that document), and O'Hagan et al., Nature Reviews, Drug Discovery 2 (9) (2003), 727-735 (in particular the endogenous immuno-potentiating compounds and delivery systems described therein), or mixtures thereof.
  • KLH Keyhole Limpet Hemocyanin
  • tetanus toxoid albumin-binding protein
  • bovine serum albumin bovine serum albumin
  • MAP dendrimer
  • peptide linkers or flanking regions
  • the conjugation chemistry e.g. via heterobifunctional compounds such as GMBS and of course also others as described in “Bioconjugate Techniques”, Greg T. Hermanson
  • the vaccine composition may be formulated with an adjuvant, preferably a low soluble aluminium composition, in particular aluminium hydroxide.
  • adjuvants like MF59 aluminium phosphate, calcium phosphate, cytokines (e.g., IL-2, IL-12, GM-CSF), saponins (e.g., QS21), MDP derivatives, CpG oligos, LPS, MPL, polyphosphazenes, emulsions (e.g., Freund's, SAF), liposomes, virosomes, iscoms, cochleates, PLG microparticles, poloxamer particles, virus-like particles, heat-labile enterotoxin (LT), cholera toxin (CT), mutant toxins (e.g., LTK63 and LTR72), microparticles and/or polymerized liposomes may be used.
  • cytokines e.g., IL-2, IL-12, GM-CSF
  • saponins e.g., QS21
  • MDP derivatives e.g., CpG oligo
  • the compound of the present invention is preferably bound to the carrier or adjuvant via a linker, which is selected from the group consisting of NHS-poly (ethylene oxide) (PEO) (e.g. NHS-PEO 4 -maleimide).
  • a linker which is selected from the group consisting of NHS-poly (ethylene oxide) (PEO) (e.g. NHS-PEO 4 -maleimide).
  • a vaccine which comprises the present compound (mimotope) and the pharmaceutically acceptable carrier may be administered by any suitable mode of application, e.g. i.d., i.v., i.p., i.m., intranasally, orally, subcutaneously, etc. and in any suitable delivery device (O'Hagan et al., Nature Reviews, Drug Discovery 2 (9), (2003), 727-735).
  • the compound of the present invention is preferably formulated for intravenous, subcutaneous, intradermal or intramuscular administration (see e.g. “Handbook of Pharmaceutical Manufacturing Formulations”, Sarfaraz Niazi, CRC Press Inc, 2004).
  • the vaccine contains the compound according to the invention in an amount of from 0.1 ng to 10 mg, preferably 10 ng to 1 mg, in particular 100 ng to 100 ⁇ g, or, alternatively, e.g. 100 fmol to 10 ⁇ mol, preferably 10 pmol to 1 ⁇ mol, in particular 100 pmol to 100 nmol.
  • the vaccine may also contain auxiliary substances, e.g. buffers, stabilizers etc.
  • Another aspect of the present invention relates to a peptide consisting of at least one amino acid sequence selected from the group consisting of SYHATFL (SEQ ID NO. 2), TMAFPLN (SEQ ID NO. 3), HYHGAFL (SEQ ID NO. 4), EHHDIFL (SEQ ID NO. 5), SSLELFL (SEQ ID NO. 44), TGLSVFL (SEQ ID NO. 6), WMPSLFY (SEQ ID NO. 7), SMPWWFF (SEQ ID NO. 8), TMPLLFW (SEQ ID NO. 9), DTWPGLE (SEQ ID NO. 10), SMPPIFY (SEQ ID NO. 11), MPLWWWD (SEQ ID NO.
  • SEQ ID NO. 12 SMPNLFY (SEQ ID NO. 13), RMPPIFY (SEQ ID NO. 14), NPFEVFL (SEQ ID NO. 15), TLPNWFW (SEQ ID NO. 16), SMPLTFY (SEQ ID NO. 17), SFLDTLT (SEQ ID NO. 45), NFLKTLS (SEQ ID NO. 46), DFLRTLT (SEQ ID NO. 47), AFLDTLV (SEQ ID NO. 48), TFLSSLA (SEQ ID NO. 49), GFLDSLM (SEQ ID NO. 50), SPHPHFL (SEQ ID NO. 51), NFMSIGL (SEQ ID NO. 19), SQFLASL (SEQ ID NO. 20), SNFLKTL (SEQ ID NO.
  • TGFLATL SEQ ID NO. 53
  • WSWPGLN SEQ ID NO. 21
  • IAWPGLD SEQ ID NO. 22
  • SKFMDTL SEQ ID NO. 23
  • SDFLRAL SEQ ID NO. 54
  • SMPMVFY SEQ ID NO. 24
  • YEWVGLM SEQ ID NO. 25
  • KGFLDHL SEQ ID NO. 26
  • SANPRDFLETLF SEQ ID NO. 55
  • RMFPESFLDTLW SEQ ID NO. 56
  • TIYDSFLDSLAS SEQ ID NO. 57
  • HQSDDKMPWWFF SEQ ID NO. 27
  • KPYLLKDFLEAL SEQ ID NO.
  • AMGPYDALDLFL SEQ ID NO. 59
  • TWNPIESFLESL SEQ ID NO. 60
  • YVWQDPSFTTFF SEQ ID NO. 28
  • QYQTPLTFLEAL SEQ ID NO. 61
  • RHISPATFLEAL SEQ ID NO. 62
  • HTDSFLSTFYGD SEQ ID NO. 63
  • YVWQDPSFTTFF SEQ ID NO. 29
  • ADSTFTSFLQTL SEQ ID NO. 64
  • GPVSIYADTDFL SEQ ID NO. 65
  • DSNDTLTLAAFL SEQ ID NO. 66
  • NGSPALSHMLFL SEQ ID NO. 33
  • TDYDPMWVFFGY SEQ ID NO.
  • EPLHFRSDRIQA SEQ ID NO. 74
  • ATPSHLIIDRAQ SEQ ID NO. 75
  • APKHLYADMSQA SEQ ID NO. 76
  • FKPAHVSIDWLQ SEQ ID NO. 77
  • MPAHLSRDLRQS SEQ ID NO. 78
  • NPKHYSIDRHQA SEQ ID NO. 79
  • SPQHLTTDRAQA SEQ ID NO. 80
  • TPFHFAQDSWQW SEQ ID NO. 81
  • TPTHYYADFSQLLS SEQ ID NO. 82
  • TPTHYYADFSQSLS SEQ ID NO. 83
  • GTPTHYYADFSQLL SEQ ID NO.
  • GTPTHYYADFSQSL (SEQ ID NO. 85), FGTPTHYYADFSQSLS (SEQ ID NO. 86), FGFPTHYYADFSQSLS (SEQ ID NO. 87), LPGHLIWDSLHY (SEQ ID NO. 88), LPGHLIWDSLHYL (SEQ ID NO. 89), LPGHLIWDSLHYLS (SEQ ID NO. 90), LPGHLIWDSLHSL (SEQ ID NO. 91), LPGHLIWDSLHSLS (SEQ ID NO. 92), GLPGHLIWDSLHYL (SEQ ID NO. 93), GLPGHLIWDSLHSL (SEQ ID NO. 94), FGLPGHLIWDSLHSLS (SEQ ID NO.
  • EPLHFRSDRIQALS SEQ ID NO. 116
  • EPLHFRSDRIQSLS EPLHFRSDRIQSLS
  • SEQ ID NO. 117 EPLHFRSDRIQSLS
  • GEPLHFRSDRIQAL SEQ ID NO. 118
  • FGEPLHFRSDRIQALS SEQ ID NO. 119
  • FGFPLHFRSDRIQSLS SEQ ID NO. 120
  • APKHLYADMSQA SEQ ID NO. 121
  • APKHLYADMSQALS SEQ ID NO. 122
  • APKHLYADMSQSLS SEQ ID NO. 123
  • GAPKHLYADMSQAL SEQ ID NO. 124
  • FGFPKHLYADMSQSLS SEQ ID NO. 125
  • MPAHLSRDLRQS SEQ ID NO.
  • AGFPEHLLVDFLQSLS (SEQ ID NO. 149), FAFPEHLLVDFLQSLS (SEQ ID NO. 150), FGAPEHLLVDFLQSLS (SEQ ID NO. 151), FGFAEHLLVDFLQSLS (SEQ ID NO. 152), FGFPAHLLVDFLQSLS (SEQ ID NO. 153), FGFPEALLVDFLQSLS (SEQ ID NO. 154), FGFPEHALVDFLQSLS (SEQ ID NO. 155), FGFPEHLAVDFLQSLS (SEQ ID NO. 156), FGFPEHLLADFLQSLS (SEQ ID NO. 157), FGFPEHLLVAFLQSLS (SEQ ID NO.
  • FGFPEHLLVDALQSLS (SEQ ID NO. 159), FGFPEHLLVDFAQSLS (SEQ ID NO. 160), FGFPEHLLVDFLASLS (SEQ ID NO. 161), FGFPEHLLVDFLQALS (SEQ ID NO. 162), FGFPEHLLVDFLQSAS (SEQ ID NO. 163), FGFPEHLLVDFLQSLA (SEQ ID NO. 164), FAFPAHLLVDFLQALA (SEQ ID NO. 165), AAFPAHLLADFLQALA (SEQ ID NO. 166), SPQHLTTDRAQA (SEQ ID NO. 167), SPQHLTTDRAQALS (SEQ ID NO.
  • FGFPAHVSADWLQSLS (SEQ ID NO. 189), FGFPAHVSIDWLQALS (SEQ ID NO. 190), FGFPAHVSIDWLQSLA (SEQ ID NO. 191), FAFPAHVSIDWLQALA (SEQ ID NO. 192), FGFAAHVSIDWLQSLS (SEQ ID NO. 193), FGFFAHVSIDWLQSLS (SEQ ID NO. 194), FGFPAHVSIRWLQSLS (SEQ ID NO. 195), FGFPAHVSIEWLQSLS (SEQ ID NO. 196), FGFPAHVSIDWLNSLS (SEQ ID NO. 197), FGFPAHVSIDWLHSLS (SEQ ID NO.
  • FGFPAHISIDWLQSLS (SEQ ID NO. 219), FGFPAHIIIDWLQSLS (SEQ ID NO. 220), FGFPAHLTTDWLQSLS (SEQ ID NO. 221), FGFPAHVFIDWLQSLS (SEQ ID NO. 222), FGFPAHVYIDWLQSLS (SEQ ID NO. 223), FGFPAHVSLDWLQSLS (SEQ ID NO. 224), FGFPAHVSADWLQSLS (SEQ ID NO. 225), TPTHYYADFSQSLS (SEQ ID NO. 226), FGFPAHVWIDWLQSLS (SEQ ID NO. 229), FGFPAHVFIDWLQSLN (SEQ ID NO.
  • FGFPAHFSIDWLQSLS (SEQ ID NO. 231), FGFPAHVSFDWLQSLS (SEQ ID NO. 232), FGFPEHVFIDWLQSLS (SEQ ID NO. 233), DFGFPAHVFIDWLQSLS (SEQ ID NO. 234), DFGFPSHLIIDWLQSLS (SEQ ID NO. 235), DFGFPAHVYIDWLQSLS (SEQ ID NO. 236), FGFPQHLFTDWLQSLS (SEQ ID NO. 237), FGFPKHLLVDFLQSLS (SEQ ID NO. 238), FGFPAHVSIDFSQSLS (SEQ ID NO. 227), FGFPAHVSIDFSQSLS (SEQ ID NO.
  • FGFPSHIIIDWLQSLS (SEQ ID NO. 239), FGFPSHLIIEWLQSLS (SEQ ID NO. 240), AAFPAHLLADAAQALA (SEQ ID NO. 241), AAFPAHAAADFLQALA (SEQ ID NO. 242), AAFAAHLLADFLQAAA (SEQ ID NO. 243), AAAPAHLLVDAAQAAA (SEQ ID NO. 244), FAFPAHVFIDWLQSLS (SEQ ID NO. 245); FGFPAHVFIDWLQALS (SEQ ID NO. 246), FGFPAHVFIDWLQSLA (SEQ ID NO. 247), GFPAHVFIDWLQSLS (SEQ ID NO.
  • FPAHVFIDWLQSLS (SEQ ID NO. 249), PAHVFIDWLQSLS (SEQ ID NO. 250), FAFPAHVFIDWLQALA (SEQ ID NO. 251), FGFPEHLFVDFLQSLS (SEQ ID NO. 252), FGFPAHVHIDWLQSLS (SEQ ID NO. 253), FGFPAHVPIDWLQSLS (SEQ ID NO. 254), FGFPSHLFIDWAQSLS (SEQ ID NO. 255), PGFPAHVFIDWLQLIT (SEQ ID NO. 256), PAHVYIDWLQSLS (SEQ ID NO. 257), FGFPAHVYIDWLQ (SEQ ID NO.
  • FGFPAHVFIDWLQ (SEQ ID NO. 259), DFGFPAHVFIDWLQSLN (SEQ ID NO. 260), PSHLIIDWLQ (SEQ ID NO. 261), PAHVFIDWLQ (SEQ ID NO. 262), DFGFPAHVTIDWLQSLN (SEQ ID NO. 263), DFGFPAHVLIDWLQSLN (SEQ ID NO. 264), and FGFPAHVFIDWLQSLA (SEQ ID NO. 265).
  • the peptides of the present invention turned out to be mimotopes for CETP and, hence, the mimotopes were able to bind to antibodies binding to the CETP fragment C-FGFPEHLLVDFLQSLS (SEQ ID NO. 146) (16 C-terminal amino acids of CETP protein).
  • Another aspect of the present invention relates to a pharmaceutical formulation comprising at least one peptide according to the present invention.
  • the peptides of the present invention may be formulated in a pharmaceutical formulation which may be administered to an individual. These formulations may be used, e.g., for preventing and/or treating atherosclerosis, atherosclerosis risk diseases and atherosclerosis sequelae.
  • the peptides in the formulation can be combined from the pool of peptides disclosed herein. Furthermore is also possible to provide pharmaceutical formulations, which comprise one or more of the peptides of the present invention, and which can be administered separately or together to an individual in need thereof.
  • the peptides of the present invention can be mixed into one single pharmaceutical formulation or in a combination of two or three.
  • the resulting formulation can be administered at the same or the different moments in time.
  • the peptide present in the formulation is coupled to a pharmaceutically acceptable carrier, preferably KLH (Keyhole Limpet Hemocyanin).
  • FIG. 1 shows the result of a representative competition ELISA after screening phage display library Ph.D. 7 with monoclonal antibody “Paula”.
  • FIGS. 2 a and 2 b show the results of 2 typical competition ELISAs after screening phage display library Ph.D. 12 with monoclonal antibody “Paula”.
  • FIGS. 3 a and 3 b show the results of 2 representative competition ELISAs after screening phage display library Ph.D. 7 with mAb Frida.
  • FGFPEHLLVDFLQSLS SEQ ID NO. 146 FGFPEHLLVDFLQSLS SEQ ID NO. 147 WPLHLWQ SEQ ID NO. 39 VSAYNNV SEQ ID NO. 38
  • FIG. 4 a shows the result of a representative competition ELISA after screening phage display library Ph.D. 12 with monoclonal antibody “Frida”.
  • FGFPEHLLVDFLQSLS SEQ ID NO. 146 FGFPEHLLVDFLQSLS SEQ ID NO. 147 TPTHYYADFSQL SEQ ID NO. 67 LPGHLIWDSLHY SEQ ID NO. 68 LPQTHPLHLLED SEQ ID NO. 69
  • FIG. 4 b shows binding of monoclonal antibody “Frida” to ELISA plates coated with mimotope-BSA
  • FIGS. 5 a and 5 b show the results of a representative competition ELISA after screening phage display library Ph.D. 12 with monoclonal antibody “Frida”.
  • FGFPEHLLVDFLQSLS SEQ ID NO. 146 FGFPEHLLVDFLQSLS SEQ ID NO. 147 GTPTHYYADFSQLL SEQ ID NO. 84 GTPTHYYADFSQSL SEQ ID NO. 85
  • FGTPTHYYADFSQSLS SEQ ID NO. 86 FGFPTHYYADFSQSLS SEQ ID NO. 87 GLPGHLIWDSLHYL SEQ ID NO. 93 GLPGHLIWDSLHSL SEQ ID NO. 94 FGLPGHLIWDSLHSLS SEQ ID NO. 95 FGFPGHLIWDSLHSLS SEQ ID NO. 96 FGIPYHHLVDQLHHLS SEQ ID NO. 101 FGFPYHHLVDQLHSLS SEQ ID NO.
  • FGFPKHLYADMSQSLS SEQ ID NO. 125 FKPAHVSIDWLQSLS SEQ ID NO. 183 FGFPAHVSIDWLQSLS SEQ ID NO. 184 GMPAHLSRDLRQSL SEQ ID NO. 129 FGFPAHLSRDLRQSLS SEQ ID NO. 130 GSPQHLTTDRAQAL SEQ ID NO. 170 FGFPQHLTTDRAQSLS SEQ ID NO. 171 GTPFHFAQDSWQWL SEQ ID NO. 135 FGFPFHFAQDSWQSLS SEQ ID NO. 136
  • FIG. 6 shows the results of a competition ELISA of two mimotopes after screening phage display library Ph.D. 12 with monoclonal antibody “Frida”.
  • FGFPEHLLVDFLQSLS SEQ ID NO. 146 FGFPEHLLVDFLQSLS SEQ ID NO. 147 FGFPSHLIIDWAQSLS SEQ ID NO. 178 FGFPSHLIIDWLQSLS SEQ ID NO. 179
  • FIGS. 7 a to 7 d show the antibody titer (anti mouse IgG) of in vivo experiments, whereby the following mimotope-BSA conjugates were injected into mice:
  • FIGS. 8 a and 8 b show the results of two representative competition ELISA after screening phage display library Ph.D. 7C7 with monoclonal antibody “Frida”.
  • FIG. 9 shows an in vitro ELISA test for the detection of the binding between “Frida” and cyclic mimotopes.
  • FGFPEHLLVDFLQSLS SEQ ID NO. 147 ACSFAYLYRC SEQ ID NO. 137 ACYMGQQFVC SEQ ID NO. 140 ACLTAYLHWC SEQ ID NO. 141 ACTLFPVAYC SEQ ID NO. 142 ACWLFPYAHC SEQ ID NO. 143 ACQTINRWLC SEQ ID NO. 145
  • FIGS. 10 a and 10 b show the results of an inhibition ELISA assay with FGFPSHLIIDWLQSLS (SEQ ID NO. 179), FGFPAHVFIDWLQSLS (SEQ ID NO. 222) and FGFPAHVYIDWLQSLS (SEQ ID NO. 223).
  • FIG. 10 a Coat 1 ⁇ M peptide. Detection ⁇ IgG1
  • FIG. 10 b Coat 1 ⁇ M peptide. Detection ⁇ IgG1
  • FIG. 11 shows the in vivo induction of antibodies directed to CETP by mimotopes of the invention that are administered to mice.
  • Balb/c mice/30 ⁇ g Peptide, 2 injections in 2 week intervals. S3 2 weeks after 3rd injection.
  • Alum as adjuvant. Titers against original epitope (p4073) induced by injection of mimotopes.
  • FIGS. 12 a and 12 b show the in vivo induction of CETP specific antibodies by the administration of the mimotopes of the invention.
  • Titers to p4073 and its correlation to titers to CETP of selected groups (which show high titers against p4073): gr.4, gr.9, gr.10, gr.14, gr.16-20/gr.1 (KLH), gr.2 (original epitope) as controls.
  • KLH/ Alum group 11 C-FSFPAHVSIDWLQSLS p4342- 0.38 0.41 (SEQ ID NO. 203) KLH/ Alum group 12 C-FYFPAHVSIDWLQSLS p4343- 0.61 1.05 (SEQ ID NO. 204) KLH/ Alum group 13 C-FDFPAHVSIDWLQSLS p4344- 0.35 0.43 (SEQ ID NO. 205) KLH/ Alum group 15 C-FGFPAHVSIDWLQYLS p4351- 0.54 0.59 (SEQ ID NO. 211) KLH/ Alum group 11 C-FSFPAHVSIDWLQSLS p4342- 0.38 0.41 (SEQ ID NO. 203) KLH/ Alum group 12 C-FYFPAHVSIDWLQSLS p4343- 0.61 1.05 (SEQ ID NO. 204) KLH/ Alum group 13 C-FDFPAHVSIDWLQSLS p4344- 0.35 0.43 (SEQ ID NO. 205)
  • FIG. 13 shows the in vivo induction of antibodies directed to CETP by mimotopes of the invention that are administered to mice.
  • Sera of each group (5 Balb/c mice each) were combined, diluted 1:100 and tested on ELISA plates coated with recombinant GST-CETP or rabbit CETP, respectively. Detection of bound antibodies was with algG.
  • KLH/ Alum group 7 C-FGFPAHVSIDWLQSLY P4354- 0.29 0.23 (SEQ ID NO. 214) KLH/ Alum group 8 C-FGFPAHVSIRWLQSLS p4337- 0.24 0.14 (SEQ ID NO. 195) KLH/ Alum
  • FIG. 14 shows a CETP activity assay, wherein 0.6 ⁇ l human serum (with endogenous CETP activity) is mixed with serum from wild-type mice (not containing CETP activity) vaccinated with KLH/Alum (negative control group), p4703-KLH/Alum (original CETP epitope), or p4361 (or p4362 or p 4325) mimotope, respectively.
  • FIG. 15 shows that the addition of p4325-KLH/Alum to human serum inhibits significantly CETP activity.
  • FIG. 16 shows that the addition of p4361-KLH/Alum to human serum inhibits significantly CETP activity.
  • FIG. 17 shows that the addition of p4362-KLH/Alum to human serum inhibits significantly CETP activity.
  • FIG. 18 a shows an inhibition ELISA with mimotopes (Coat. 1 ⁇ M 4073 peptide, detection ⁇ IgG1).
  • FIG. 18 b shows an inhibition ELISA with mimotopes (Coat. 1 ⁇ M 4073 peptide, detection ⁇ IgG1).
  • VLI; p4361 F replaced by L, plus D on N-term and N instead of S on C-term p5067 FGFPAHVYIDWLQSLS-C p4362 C on C-terminus 0.563 0.217 (SEQ ID NO. 223) p5068 FGFPAHVFIDWLQSLN-C p4474 C on C-terminus 0.757 0.271 (SEQ ID NO. 230)
  • FIG. 18 c shows a inhibition ELISA with mimotopes screen PhD12 Frida and Ala-exchange for mimotope characterisation/mAb Frida (Coat 1 ⁇ M 4073. Detection ⁇ IgG1.)
  • FIG. 19 a shows a peptide ELISA, immunisation with C-DFGFPAHVYIDWLQSLS (p4628-KLH/Alum) (SEQ ID NO. 236), titre to original epitope.
  • FIG. 19 b shows a peptide ELISA, immunisation with C-FGFPAHVFIDWLQSLN (p4474-KLH/Alum) (SEQ ID NO. 230), titre to original epitope.
  • FIG. 19 c shows a peptide ELISA, immunisation with C-FGFPAHVFIDWLQSLN (p4474-KLH/Alum) (SEQ ID NO. 230), titre to injected mimotope.
  • FIG. 19 d shows an anti-protein ELISA.
  • Mice were injected 3 times with 30 ⁇ g of the indicated mimotopes coupled to KLH with Alum as adjuvant.
  • Sera from each group (comprising 5 mice) were pooled, diluted 1:100 and tested on ELISA plates coated with purified rabbit CETP.
  • FIG. 19 e shows an anti-protein ELISA, wherein mice were injected 3 times with 30 ⁇ g of the indicated mimotopes coupled to KLH with Alum as adjuvant. Mouse sera (from single mice) were diluted 1:100 and tested on ELISA plates coated with purified rabbit CETP.
  • HDLs high density lipoproteins
  • CHD coronary heart disease
  • CETP is a plasma glycoprotein that facilitates transfer of neutral lipids and phospholipids between lipoproteins and regulates the concentration of plasma HDL.
  • the inhibition of CETP activity is expected to increase plasma HDL concentrations for several reasons.
  • CETP lowers HDL concentrations by moving cholesteryl esters from HDLs to VLDLs and LDLs.
  • Transient inhibition of CETP in rabbits and hamsters by monoclonal antibodies, small molecules (Sikorski, J. A., J. Med. Chem. 49 (1) (2006): 1-22), or antisense oligonucleotides causes HDL increase.
  • the problem of the anti-CETP vaccine approach discussed above is that the vaccine formulation comprises a self peptide and therefore must break natural tolerance against self antigens.
  • the invention describes a CETP mimotope that can be used for vaccination: The mimotope shall induce the production of antibodies against CETP.
  • the CETP mimotope does not have a self sequence and therefore does not need to break tolerance. Thus, the induction of an anti-CETP antibody response is greatly facilitated.
  • the mimotope is identified with a monoclonal antibody (mAb) and (commercially available) peptide libraries.
  • An anti-CETP monoclonal antibody is used that neutralizes CETP activity. This mAb detects a sequence within the C-terminal 26 amino acids of CETP necessary for neutral lipid transfer activity.
  • Phage Display was done according to manufacturer's protocol (www.neb.com).
  • mice wildtype or CETP-transgenic mice; subcutaneously into the flank or intra-dermaly into the ears
  • rabbits subcutaneously into the flank
  • an appropriate adjuvant aluminium hydroxide and Gerbu 100 for mice and aluminium hydroxide or CFA/IFA for rabbits.
  • FIG. 1 The result of a representative competition ELISA is shown in FIG. 1 .
  • Subcutaneous injections in the flank were performed in week 1, week 3 and week 7 with 30 ⁇ g peptide-KLH per mouse.
  • Intradermal injections in the ear were performed in week 1, week 3 and week 6 with 10 ⁇ g peptide-KLH per mouse.
  • Sera were taken 2 weeks after the 3rd injection.
  • Vaccine formulation with Alum up to 250 ⁇ l, injected into one flank.
  • the Alum formulation with 1 ml per mouse (500 ⁇ l into each flank) was in 1 ⁇ PBS as buffer.
  • Vaccine formulation with Gerbu Adjuvant 100 (Gerbu Cat. Nr. #3100; always 50 ⁇ l adjuvant per mouse): 200 ⁇ l, 100 ⁇ l injected into each flank comprising 1 ⁇ HEPES as buffer.
  • Results of 2 typical competition ELISAs are shown in FIGS. 2A and 2 b.
  • mimotope P12-37 C-TIYDSFLDSLAS did not induce an antibody response to the original epitope.
  • FIGS. 3A and 3 b The results of 2 representative competition ELISAs with mAb “Frida” are shown in FIGS. 3A and 3 b . The same pattern was seen with mAb “James”.
  • FIGS. 5A and 5 b Representative examples of inhibition ELISA are shown in FIGS. 5A and 5 b .
  • the elongated peptides Fr12/3/84 ext2 and Fr12/3/55 ext3 showed a significant inhibition:
  • C-FGFPAHVSIDWLQSLS (SEQ ID NO. 184)
  • C-FGFPSHLIIDRAQSLS (SEQ ID NO. 177)
  • C-FGFPSHLIIDWAQSLS (SEQ ID NO. 178)
  • R C-FGFPSHLIIDWLQSLS
  • Fr12/3/55 ext2 WL instead of RA
  • Further preferred mimotopes have been characterised by the following example-set-up:
  • mice Female Balb/c mice, five mice per group, were subcutaneously immunized with 30 ⁇ g peptide coupled to KLH. Control groups were administered KLH or C-FGFPEHLLVDFLQSLS (SEQ ID NO. 147). As adjuvant alum was used. The peptides administered were all able to bind to “Frida” and to induce an immune response for CETP, although some of these peptides did not inhibit the binding of CETP to “Frida” in vitro (in an in vitro inhibition assay). The in vitro ELISA assay to determine the antibody titer was performed with pooled sera after two vaccinations in a two week interval (S2; see FIGS. 7 a to 7 d ).
  • the wells of the ELISA plate were coated with KLH (positive control), mimotope-BSA conjugate, C-FGFPEHLLVDFLQSLS (SEQ ID NO. 147) and a irrelevant peptide-BSA conjugate (negative control).
  • the detection was performed with anti-mouse IgG.
  • the CETP activity assay was performed with assays commercially available (e.g. ROAR CETP Activity Assay) and described, for instance, in the U.S. Pat. No. 5,585,235, U.S. Pat. No. 5,618,683 and U.S. Pat. No. 5,770,355. The assay is performed according to the manufacturers' recommendations.
  • assays commercially available e.g. ROAR CETP Activity Assay

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Abstract

The present invention relates to the use of compounds for producing a medicament for preventing and/or treating atherosclerosis, atherosclerosis risk diseases and atherosclerosis sequelae.

Description

  • This application is a divisional of U.S. Ser. No. 12/673,081 filed Feb. 11, 2010, incorporated herein by reference, which was a National Stage of PCT/AT08/000,281 filed Aug. 8, 2008 and claims the benefit of Austrian application A1 258/2007 filed Aug. 10, 2007.
  • The invention relates to the prevention and treatment of atherosclerosis, atherosclerosis risk diseases and atherosclerosis sequelae.
  • Atherosclerotic sequelae, such as the peripheral arterial occlusion disease, coronary heart disease as well as the apoplectic cerebral insultus, are still among the main causes of death in the United States, Europe, and in large parts of Asia. The development of the atherosclerosis is considered to be a chronic progressive inflammation of the arterial vessel wall which is characterized by a complex interaction of growth factors, cytokines and cell interactions. According to the “response-to-injury” hypothesis, the “injury” of the endothelium constitutes the initial event of the disease, leading to an endothelial dysfunction which triggers a cascade of cellular interactions culminating in the formation of the atherosclerotic lesions. As risk factors promoting such an “injury”, exogenous and endogenous influences are mentioned which correlate statistically significantly with atherosclerosis. Increased and modified LDL, Lp(a), arterial hypertension, Diabetes mellitus and hyperhomocysteinaemia are, for instance, counted among the most important ones of these endothelium-damaging factors. Since the endothelium does not constitute a rigid, but much rather an extremely dynamic barrier, a plurality of molecular changes occur in the course of the endothelial dysfunction in addition to an increased permeability for lipoproteins, which molecular changes have a decisive influence on the interaction of monocytes, T-lymphocytes and endothelial cells. By the expression of endothelial adhesion molecules of the type of the E, L and P selectins, integrins, ICMA-1, VCAM-1 and platelet-endothelial-cell adhesion molecule-1, adhesion of monocytes and T-lymphocytes at the lumen side occurs. The subsequent migration of the leukocytes over the endothelium is mediated by MCP-1, interleukin-8, PDGF, MCSF and osteopontin. Via the so-called scavenger receptor, macrophages and monocytes resident in the intima are capable of taking up the penetrated LDL particles and to deposit them as vacuoles of cholesterol esters in the cytoplasma. The foam cells formed in this manner accumulate mainly in groups in the region of the vessel intima and form the “fatty streak” lesions occurring already in childhood. LDL are lipoproteins of low density and are formed by catabolic effects of lipolytic enzymes from VLDL particles rich in triglyceride. Besides their damaging properties on endothelial cells and smooth muscle cells of the media, LDL moreover has a chemotactic effect on monocytes and is capable of increasing the expression of MCSF and MCP-1 of the endothelial cells via gene amplification. In contrast to LDL, HDL is capable of taking up cholesterol esters from loaded macrophages mediated by apolipoprotein E, under formation of so-called HDLc complexes. By the interaction of SR-B1 receptors, these cholesterol ester-loaded particles are capable of binding to hepatocytes or to cells of the adrenal cortex and delivering cholesterol for the production of bile acids and steroids, respectively. This mechanism is called reverse cholesterol transport and elucidates the protective function of HDL. Activated macrophages are capable of presenting antigens via HLA-DR and thereby activate CD4 and CD8 lymphocytes which, consequently, are stimulated to secrete cytokines, such as IFN-gamma and TNF-alpha, and moreover, contribute to increasing the inflammatory reaction. In the further course of the disease, smooth muscle cells of the media start to grow into the region of the intima which has been altered by inflammation. By this, the intermediary lesion forms at this stage. Starting from the intermediary lesion, the progressive and complicated lesion will develop over time, which is morphologically characterized by a necrotic core, cellular detritus and a fibrinous cap rich in collagen on the side of the lumen. If the cell number and the portion of the lipoids increase continuously, tears in the endothelium will occur, and surfaces with thrombotic properties will be exposed. Due to the adhesion and activation of thrombocytes at these tears, granules will be released which contain cytokines, growth factors and thrombin. Proteolytic enzymes of the macrophages are responsible for the thinning of the fibrinous cap which, at last, will lead to a rupture of the plaques with consecutive thrombosis and stenosing of the vessels and an acute ischemia of the terminal vessels.
  • Various risk factors are held responsible for the forming of atherosclerotic lesions. Hyperlipoproteinemia, arterial hypertension and abuse of nicotine are of particular significance in this respect. A disease which involves an excessive increase in the total and LDL cholesterol is the familial hypercholesterinemia (FH). It belongs to the most frequent monogenetically inherited metabolic diseases. The moderate heterozygous form occurs with a frequency of 1:500, the homozygous form with 1:1 million clearly more rarely. Causes of the familial hypercholesterinemia are mutations in the LDL receptor gene on the short arm of chromosome 19. These mutations may be deletions, insertions or point mutations. The characteristic finding of the lipoproteins in familial hypercholesterinemia is an increase in the total and LDL cholesterol at mostly normal triglyceride and VLDL concentrations. Often the HDL is lowered. Phenotypically, there is a type IIAa-hyperlipoproteinemia. In the heterozygous form, the total cholesterol is increased by the two to three-fold, in the homozygous form it is increased by the five to six-fold as compared to the normal level. Clinically the familial hypercholesterinemia manifests itself by an early coronary sclerosis. As a rule, in heterozygous men the first symptoms of a coronary heart disease (CHD) occur between their 30th and the 40th year of age, in women on an average 10 years later. 50% of the afflicted men die of the consequences of their coronary sclerosis before they are 50 years old. Besides the massively increased LDL levels, also lowered HDL concentrations are responsible for the rapid progress of atherosclerosis. Atherosclerotic changes may become manifest also on extra-cardiac vessels, such as the aorta, the carotid arteries and peripheral arteries. With the homozygous form of the disease, the coronary sclerosis develops already in early childhood. The first myocardial infarction often occurs before the 10th year of age, and in most cases the afflicted persons die before they are 20 years old. The development of xanthomas is a function of the level of the serum cholesterol and the duration of the disease. Approximately 75% of the heterozygous individuals afflicted who are more than 20 years old exhibit tendinous xanthomas. The homozygous individuals have skin and tendon xanthomas in nearly 100%. Lipid deposits may also occur on the eye lid and in the cornea (xanthelasmas; Arcus lipoides). These are, however, not a specific sign of a hypercholesterinemia, since they are also found with normal cholesterol levels. Furthermore, with the FH, acute arthritides and tendosynovitides occur frequently. The individual lipoproteins differ with respect to size and density, since they contain differently large portions of lipids and proteins, so-called apoproteins. The density increases with increasing protein and decreasing lipid portion. Due to their different densities, they can be separated into different fractions by ultracentrifugation. This is the basis for the classification of the lipoproteins into their main groups: chylomicrones, very-low-density lipoproteins (VLDL), intermediate-density lipoproteins (IDL), low-density lipoproteins (LDL), high-density lipoproteins (HDL), lipoprotein (a) (Lp(a)). Among the lipoproteins with a high atherogenic potential there are primarily the LDL, the Lp(a) and the VLDL. LDL has a density of approximately d=1.006-1.063 g/ml. The core is formed by esterified cholesterol molecules. This highly hydrophobic core is surrounded by an envelope of phospholipids, non-esterified cholesterol and one single Apo B100 molecule. Besides, Apoprotein E is found on the surface of the LDL particles. The function of the LDL consists in transporting cholesterol to peripheral tissues where—mediated by the apoprotein B-100—it is taken up into the cells via the LDL receptor. In comprehensive epidemiologic studies, a positive correlation between the level of the serum cholesterol and the occurrence of a coronary heart disease could be demonstrated. LDL cholesterol levels of higher than 160 mg/dl constitute a high cardiovascular risk. Besides the level of the LDL cholesterol, also the level of the vessel-protecting HDL cholesterol plays an important role when estimating the risk profile for cardiovascular diseases. Levels of below 35 mg/dl are associated with an increased risk. VLDL are lipoproteins with a low density (d=0.94-1.006 g/ml) and a high triglyceride portion. Substantially, VLDL contain apoprotein C, and small portions of apoproteins B-100 and E. Different from chylomicrons, VLDL do not consist of food lipids, but are synthesized in the liver from endogenously formed triglycerides and secreted into circulation. As with the chylomicrons, the triglycerides are hydrolyzed by the aproprotein C-II-activated lipoprotein-lipase, and the free fatty acids are supplied to the muscle and fat tissue. The remaining cholesterol-rich VLDL remnants are called intermediate density lipoproteins because of their higher density. Lipoprotein(a) (Lp(a)) has a density of 1.05 to 1.12 g/ml and resembles LDL in its composition. Besides apoprotein B-100, its protein portion consists of the apoprotein(a) which is characteristic of Lp(a). To date, very little is known about the physiology and function of the Lp(a). Since the apoprotein(a) molecule has a high sequence homology to plasminogen, it is assumed that Lp(a) both promotes the formation of thrombi on atherosclerotic plaques and also has an atherogenic effect. Lp(a) is found together with apoprotein B in atherosclerotic lesions. Retrospective studies have shown a correlation between increased Lp(a) and a CHD. Likewise, the metaanalysis of numerous prospective studies has shown that Lp(a) is an independent risk factor for the occurrence of a CHD. Levels of between 15 and 35 mg/dl are considered to be normal. So far, Lp(a) can be influenced neither by diet nor by medicaments. Therefore, therapy measures are restricted to reducing further risk factors. In particular, a lowering of the LDL cholesterol seems to lower the cardiovascular risk of Lp(a). In the pathogenesis of atherosclerosis, considerable pathophysiologic importance is, moreover, attributed to coagulation factors. Epidemiologic findings suggest a correlation between the fibrinogen concentration in plasma and the development of a coronary heart disease, and, primarily, a myocardial infarction. In this context, increased fibrinogen levels (>300 mg/dl) proved to be an independent indicator and risk factor for cardiovascular diseases. Yet also high concentrations of the tissue plasminogen activator inhibitor tPA-I are associated with the occurrence of CHD. The relationship between hypertriglyceridemia and coronary risk is a different one in each case, depending on the cause of the elevation of the blood lipids. Despite the discussion whether or not triglycerides are to be considered as an independent risk factor it is undisputed that they play an important role in the pathogenesis of coronary heart diseases. Incidence of the disease is the highest in patients who exhibit high LDL cholesterol and a high triglyceride level.
  • The cholesterol ester transfer protein (CETP) is a stable plasma glycoprotein which is responsible for the transfer of neutral lipids and phospholipids between lipoproteins and which down-regulates the plasma concentration of HDL. The inhibition of the CETP lipid transfer activity has already been suggested as a therapeutic approach for increasing the HDL plasma level. There are numerous reasons which suggest that the reduction of CETP activity in plasma should lead to an increase in the HDL levels. Thus, CETP lowers the HDL concentration by the transfer of cholesterol esters from HDL to LDL and VLDL. In animal experiments with rabbits and hamsters, the transient inhibition of CETP with anti-CETP monoclonal antibodies, antisense oligonucleotides or CETP inhibitors led to the increase in the HDL levels. Lasting CETP inhibition with antisense oligonucleotides increased the HDL levels and, thus, led to a reduction of the atherosclerotic lesions in the rabbit animal model for atherosclerosis.
  • In the literature several CETP inhibitors are described, some of which are in clinical trials (e.g. Anacetrapib (Krishna R., Lancet 370 (9603) (2007): 1907-14) and Torcetrapib (Sikorski, J. A., J. Med. Chem. 49 (1) (2006): 1-22)).
  • In U.S. Pat. No. 5,512,548 and in WO 93/011782, polypeptides and their analogues are described which are capable of inhibiting CETP that catalyses the transfer of cholesterol esters from HDL to VLDL and LDL, and, therefore, have anti-atherosclerotic activity if administered to a patient. According to these documents, such a CETP polypeptide inhibitor is derived from apolipoprotein C-I of various sources, wherein especially N-terminal fragments up to amino acid 36 have been identified as CETP inhibitors.
  • Also in U.S. Pat. No. 5,880,095 A, a CETP-binding peptide is disclosed which is capable of inhibiting the activity of CETP in an individual. The CETP-inhibitory protein comprises an N-terminal fragment of porcine apolipoprotein C-III.
  • In the US 2006/0276400 and the WO 96/034888 peptides are disclosed, which are derived from CETP and comprise T-cell and/or B-cell epitopes. These peptides are able to induce in vivo the formation of CETP specific antibodies.
  • In US 2004/0087481 and U.S. Pat. No. 6,410,022 B1, peptides are disclosed which, because of the induction of a CETP-specific immune response, can be used for the treatment and prevention of cardiovascular diseases, such as, e.g., atheroslerosis. These peptides comprise a T helper cell epitope which is not derived from CETP, and at least one B-cell epitope that comes from CETP and can be derived directly from the latter. The T helper cell epitope advantageously is derived from tetanus toxoid and is covalently bound to at least one B-cell epitope of CETP. By using a T helper cell epitope that is alien to the organism, it becomes possible to induce antibodies in the body of an individual, which antibodies are directed against that peptide portion that consists of at least one CETP-B-cell epitope.
  • In Mao D et al (Vaccine 24 (2006): 4942-4950) the use of a plasmid comprising a nucleic acid molecule encoding for a B cell epitope of CETP as vaccine is described.
  • In the WO 2006/029982 CETP mimotopes to be used for the manufacture of a medicament for the treatment or prevention of atherosclerosis is described.
  • Most recently, there have already been suggestions for a vaccine approach with regard to CETP. Thus, e.g., rabbits have been treated with a vaccine which contained that peptide of CETP responsible for the cholesterol-ester transfer as an antigen. The immunized rabbits had a reduced CETP activity and altered lipoprotein levels with increased HDL and reduced LDL values. Moreover, the treated test animals of the atherosclerosis model also showed reduced atherosclerotic lesions in comparison with control animals.
  • The results of a phase II-clinical study were published, which study had been carried out by the American biotechnology company Avant with the vaccine CETi-1 (BioCentury Extra For Wednesday, Oct. 22, 2003). In this phase II-study, just as in the preceding phase I-study, a very good safety profile without any questionable side effects was proven, allowing the conclusion to be drawn that basically no side effects are to be expected from an anti-CETP vaccination approach. With regard to efficacy, however, the Avant vaccine was disappointing since it did not lead to increased HDL levels significantly better than those attained by a placebo treatment.
  • The problem with the CETi-1 vaccine is that it uses endogenous antigen. The human immune system is tolerant relative to endogenous structures, since with most of the endogenous molecules—other than with CETP—it is vital that no autoantibodies be formed. Thus, it was the object of the CETi-1 vaccine to break the endogenous tolerance which, apparently, it has not achieved to a sufficient extent.
  • Thus, it is the object of the present invention to provide antigens for an anti-CETP vaccine which are selected such that they are considered as foreign by the immune system and therefore need not break a self-tolerance. These antigens may be used for preventing and/or treating atherosclerosis, atherosclerosis risk diseases and atherosclerosis sequelae.
    • BRIEF DESCRIPTION OF THE DRAWINGS
  • FIG. 1 shows the result of a representative competition ELISA after screening phage display library Ph.D. 7 with monoclonal antibody “Paula”.
  • FIGS. 2 a and 2 b show the results of 2 typical competition ELISAs after screening phage display library Ph.D. 12 with monoclonal antibody “Paula”.
  • FIGS. 3 a and 3 b show the results of 2 representative competition ELISAs after screening phage display library Ph.D. 7 with mAb Frida.
  • FIG. 4 a shows the result of a representative competition ELISA after screening phage display library Ph.D. 12 with monoclonal antibody “Frida”.
  • FIG. 4 b shows binding of monoclonal antibody “Frida” to ELISA plates coated with mimotope-BSA.
  • FIGS. 5 a and 5 b show the results of a representative competition ELISA after screening phage display library Ph.D. 12 with monoclonal antibody “Frida”.
  • FIG. 6 shows the results of a competition ELISA of two mimotopes after screening phage display library Ph.D. 12 with monoclonal antibody “Frida”.
  • FIGS. 7 a, 7 b, 7 c and 7 d show the antibody titer (anti mouse IgG) of in vivo experiments, whereby the following mimotope-BSA conjugates were injected into mice.
  • FIGS. 8 a and 8 b show the results of two representative competition ELISA after screening phage display library Ph.D. 7C7 with monoclonal antibody “Frida”.
  • FIG. 9 shows an in vitro ELISA test for the detection of the binding between “Frida” and cyclic mimotopes.
  • FIGS. 10 a and 10 b show the results of an inhibition ELISA assay with FGFPSHLIIDWLQSLS (SEQ ID NO. 179), FGFPAHVFIDWLQSLS (SEQ ID NO. 222) and FGFPAHVYIDWLQSLS (SEQ ID NO. 223).
  • FIG. 11 shows the in vivo induction of antibodies directed to CETP by mimotopes of the invention that are administered to mice.
  • FIGS. 12 a and 12 b show the in vivo induction of CETP specific antibodies by the administration of the mimotopes of the invention.
  • FIG. 13 shows the in vivo induction of antibodies directed to CETP by mimotopes of the invention that are administered to mice.
  • FIG. 14 shows a CETP activity assay, wherein 0.6 μl human serum (with endogenous CETP activity) is mixed with serum from wild-type mice (not containing CETP activity) vaccinated with KLH/Alum (negative control group), p4703-KLH/Alum (original CETP epitope), or p4361 (or p4362 or p 4325) mimotope, respectively.
  • FIG. 15 shows that the addition of p4325-KLH/Alum to human serum inhibits significantly CETP activity.
  • FIG. 16 shows that the addition of p4361-KLH/Alum to human serum inhibits significantly CETP activity.
  • FIG. 17 shows that the addition of p4362-KLH/Alum to human serum inhibits significantly CETP activity.
  • FIG. 18 a shows an inhibition ELISA with mimotopes (Coat. 1 μM 4073 peptide, detection α IgG1).
  • FIG. 18 b shows an inhibition ELISA with mimotopes (Coat. 1 μM 4073 peptide, detection α IgG1).
  • FIG. 18 c shows a inhibition ELISA with mimotopes screen PhD12 Frida and Ala-exchange for mimotope characterisation/mAb Frida (Coat 1 μM 4073. Detection αIgG1.)
  • FIG. 19 a shows a peptide ELISA, immunisation with C-DFGFPAHVYIDWLQSLS (p4628-KLH/Alum) (SEQ ID NO. 236), titre to original epitope.
  • FIG. 19 b shows a peptide ELISA, immunisation with C-FGFPAHVFIDWLQSLN (p4474-KLH/Alum) (SEQ ID NO. 230), titre to original epitope.
  • FIG. 19 c shows a peptide ELISA, immunisation with C-FGFPAHVFIDWLQSLN (p4474-KLH/Alum) (SEQ ID NO. 230), titre to injected mimotope.
  • FIG. 19 d shows an anti-protein ELISA. Mice were injected 3 times with 30 μg of the indicated mimotopes coupled to KLH with Alum as adjuvant. Sera from each group (comprising 5 mice) were pooled, diluted 1:100 and tested on ELISA plates coated with purified rabbit CETP.
  • FIG. 19 e shows an anti-protein ELISA, wherein mice were injected 3 times with 30 μg of the indicated mimotopes coupled to KLH with Alum as adjuvant. Mouse sera (from single mice) were diluted 1:100 and tested on ELISA plates coated with purified rabbit CETP.
    •
  • Therefore the present invention relates to the use of a compound comprising the amino acid sequence
  • (Z1)nX1X2X3X4(Z2)m, (SEQ ID NO. 1)
  • wherein
    Z1 is an amino acid residue other than C,
    X1 is an amino acid residue selected from the group consisting of D, A, R, E, S, N, T and G,
    X2 is an amino acid residue selected from the group consisting of F, A, W, R, S, L, Q, V and M,
    X3 is an amino acid residue selected from the group consisting of L, A, S, W, E, R, I and H,
    X4 is an amino acid residue selected from the group consisting of Q, A, H, D, K, R, S and E,
    Z2 is an amino acid residue other than C,
    n is an integer between 0 and 10, preferably between 0 and 9,
    m is an integer between 0 and 3,
    is not, or does not comprise, a 4- to 16-mer polypeptide fragment of the cholesterol ester transport protein (CETP) or a CETP-epitope, said compound having a binding capacity to an antibody which is specific for the natural CETP glycoprotein,
    or
    comprising an amino acid sequence selected from the group consisting of SYHATFL (SEQ ID NO. 2), TMAFPLN (SEQ ID NO. 3), HYHGAFL (SEQ ID NO. 4), EHHDIFL (SEQ ID NO. 5), TGLSVFL (SEQ ID NO. 6), WMPSLFY (SEQ ID NO. 7), SMPWWFF (SEQ ID NO. 8), TMPLLFW (SEQ ID NO. 9), DTWPGLE (SEQ ID NO. 10), SMPPIFY (SEQ ID NO. 11), MPLWWWD (SEQ ID NO. 12), SMPNLFY (SEQ ID NO. 13), RMPPIFY (SEQ ID NO. 14), NPFEVFL (SEQ ID NO. 15), TLPNWFW (SEQ ID NO. 16), SMPLTFY (SEQ ID NO. 17), SPHPHFL (SEQ ID NO. 18), NFMSIGL (SEQ ID NO. 19), SQFLASL (SEQ ID NO. 20), WSWPGLN (SEQ ID NO. 21), IAWPGLD (SEQ ID NO. 22), SKFMDTL (SEQ ID NO. 23), SMPMVFY (SEQ ID NO. 24), YEWVGLM (SEQ ID NO. 25), KGFLDHL (SEQ ID NO. 26), HQSDDKMPWWFF (SEQ ID NO. 27), YVWQDPSFTTFF (SEQ ID NO. 28), YVWQDPSFTTFF (SEQ ID NO. 29), LPQTHPLHLLED (SEQ ID NO. 30), GPVSIYADTDFL (SEQ ID NO. 31), DSNDTLTLAAFL (SEQ ID NO. 32), NGSPALSHMLFL (SEQ ID NO. 33), TDYDPMWVFFGY (SEQ ID NO. 34), IFPLDSQWQTFW (SEQ ID NO. 35), NESMPDLFYQPS (SEQ ID NO. 36), DWGDKYFSSFWN (SEQ ID NO. 37), VSAYNNV (SEQ ID NO. 38) and WPLHLWQ (SEQ ID NO. 39)
    for producing a medicament for preventing and/or treating atherosclerosis, atherosclerosis risk diseases and atherosclerosis sequelae.
  • The present invention provides CETP mimotopes for these purposes. These mimotopes are able to induce antibodies which are able to inhibit CETP enzyme activity. The CETP mimotopes according to the present invention preferably are antigenic polypeptides which in their amino acid sequence vary from the amino acid sequence of CETP or of fragments of CETP. In this respect, the inventive mimotopes may comprise one or more non-natural amino acids (i.e. not from the 20 “classical” amino acids) or they may be completely assembled of such non-natural amino acids. Moreover, the inventive antigens which induce anti-CETP antibodies may be assembled of D- or L-amino acids or of combinations of DL-amino acids and, optionally, they may have been changed by further modifications, ring closures or derivatizations. Suitable anti-CETP-antibody-inducing antigens may be provided from commercially available peptide libraries. Preferably, these peptides are at least 4 amino acid residues in length, in particular at least 7 amino acids, and preferred lengths may be up to 16, preferably up to 14 or 20 amino acids (e.g. 5 to 16 amino acid residues). According to the invention, however, also longer peptides may very well be employed as anti-CETP-antibody-inducing antigens. Furthermore the mimotopes of the present invention may also be part of a polypeptide and consequently comprising at their N- and/or C-terminus at least one further amino acid residue.
  • The mimotopes of the present invention are capable to bind to antibodies which may be obtained by administration of C-FGFPEHLLVDFLQSLS (SEQ ID NO. 146) (16 C-terminal amino acids of CETP protein) coupled to KLH or other carriers to mammals. Once administered to a mammal the mimotopes are able to induce a corresponding immune response, so that antibodies directed against CETP are produced in said mammal.
  • The CETP-mimotopes (i.e. anti-CETP-antibody-inducing antigens) of the present invention can be identified and prepared by various methods, including phage libraries or peptide libraries. They can be produced and identified for instance by means of combinatorial chemistry or by means of high throughput screening techniques for the most varying structures (Display: A Laboratory Manual by Carlos F. Barbas (Editor), et al.; Willats W G Phage display: practicalities and prospects. Plant Mol. Biol. 2002; 50(6):837-54).
  • Furthermore, according to the invention also anti-CETP-antibody-inducing antigens based on nucleic acids (“aptamers”) may be employed, and these, too, may be found with the most varying (oligonucleotide) libraries (e.g. with 2-180 nucleic acid residues) (e.g. Burgstaller et al., Curr. Opin. Drug Discov. Dev. 5(5) (2002), 690-700; Famulok et al., Acc. Chem. Res. 33 (2000), 591-599; Mayer et al., PNAS 98 (2001), 4961-4965, etc.). In anti-CETP-antibody-inducing antigens based on nucleic acids, the nucleic acid backbone can be provided e.g. by the natural phosphor-diester compounds, or also by phosphorotioates or combinations or chemical variations (e.g. as PNA), wherein as bases, according to the invention primarily U, T, A, C, G, H and mC can be employed. The 2′-residues of the nucleotides which can be used according to the present invention preferably are H, OH, F, Cl, NH2, O-methyl, O-ethyl, O-propyl or O-butyl, wherein the nucleic acids may also be differently modified, i.e. for instance with protective groups, as they are commonly employed in oligonucleotide synthesis. Thus, aptamer-based anti-CETP-antibody-inducing antigens are also preferred anti-CETP-antibody-inducing antigens within the scope of the present invention.
  • According to the present invention the term “mimotope” refers to a molecule which has a conformation that has a topology equivalent to the epitope of which it is a mimic. The mimotope binds to the same antigen-binding region of an antibody which binds immunospecifically to a desired antigen. The mimotope will elicit an immunological response in a host that is reactive to the antigen to which it is a mimic. The mimotope may also act as a competitor for the epitope of which it is a mimic in in vitro inhibition assays (e.g. ELISA inhibition assays) which involve the epitope and an antibody binding to said epitope. However, a mimotope of the present invention may not necessarily prevent or compete with the binding of the epitope of which it is a mimic in an in vitro inhibition assay although it is capable to induce a specific immune response when administered to a mammal.
  • As used herein, the term “epitope” refers to an immunogenic region of an antigen which is recognized by a particular antibody molecule. In general, an antigen will possess one or more epitopes, each capable of binding an antibody that recognizes the particular epitope.
  • The abbreviations for the amino acid residues disclosed in the present invention follow the IUPAC recommendations:
  • Amino Acid 3-Letter Code 1-Letter Code
    Alanine Ala A
    Arginine Arg R
    Asparagine Asn N
    Aspartic Asp D
    Cysteine Cys C
    Glutamic Glu E
    Glutamine Gln Q
    Glycine Gly G
    Histidine His H
    Isoleucine Ile I
    Leucine Leu L
    Lysine Lys K
    Methionine Met M
    Phenylalanine Phe F
    Proline Pro P
    Serine Ser S
    Threonine Thr T
    Tryptophan Trp W
    Tyrosine Tyr Y
    Valine Val V
  • The mimotopes of the present invention can be synthetically produced by chemical synthesis methods which are well known in the art, either as an isolated peptide or as a part of another peptide or polypeptide. Alternatively, the peptide mimotope can be produced in a microorganism which produces the peptide mimotope which is then isolated and if desired, further purified. The peptide mimotope can be produced in microorganisms such as bacteria, yeast or fungi, in eukaryote cells such as a mammalian or an insect cells, or in a recombinant virus vector such as adenovirus, poxvirus, herpesvirus, Simliki forest virus, baculovirus, bacteriophage, sindbis virus or sendai virus. Suitable bacteria for producing the peptide mimotope include E. coli, B. subtilis or any other bacterium that is capable of expressing peptides such as the peptide mimotope. Suitable yeast types for expressing the peptide mimotope include Saccharomyces cerevisiae, Schizosaccharomyces pombe, Candida, Pichia pastoris or any other yeast capable of expressing peptides. Corresponding methods are well known in the art. Also methods for isolating and purifying recombinantly produced peptides are well known in the art and include e.g. as gel filtration, affinity chromatography, ion exchange chromatography etc.
  • To facilitate isolation of the peptide mimotope, a fusion polypeptide may be made wherein the peptide mimotope is translationally fused (covalently linked) to a heterologous polypeptide which enables isolation by affinity chromatography. Typical heterologous polypeptides are His-Tag (e.g. His6; 6 histidine residues), GST-Tag (Glutathione-S-transferase) etc. The fusion polypeptide facilitates not only the purification of the mimotopes but can also prevent the mimotope polypeptide from being degraded during purification. If it is desired to remove the heterologous polypeptide after purification the fusion polypeptide may comprise a cleavage site at the junction between the peptide mimotope and the heterologous polypeptide. The cleavage site consists of an amino acid sequence that is cleaved with an enzyme specific for the amino acid sequence at the site (e.g. proteases).
  • The mimotopes of the present invention may also modified at or nearby their N- and/or C-termini so that at said positions a cysteine residue is bound thereto. In a preferred embodiment terminally positioned (located at the N- and C-termini of the peptide) cysteine residues are used to cyclize the peptides through a disulfide bond.
  • The mimotopes of the present invention may also be used in various assays and kits, in particular in immunological assays and kits. Therefore, it is particularly preferred that the mimotope may be part of another peptide or polypeptide, particularly an enzyme which is used as a reporter in immunological assays. Such reporter enzymes include e.g. alkaline phosphatase or horseradish peroxidase.
  • The term “atherosclerosis sequelae” or “sequelae of atherosclerosis” refers to the diseases which are a consequence of atherosclerose. These diseases include among others peripheral arterial occlusive disease, coronary heart disease and apoplectic cerebral insultus (see e.g. Steinberg D. J. Lipid Res. (2005) 46: 179-190; Steinberg D et al. J. Lipid Res (2006) 47: 1339-1351).
  • According to another preferred embodiment of the present invention X1 is D and X4 is Q or H, preferably Q. Such a molecule preferably comprises at its N-terminus further amino acid residues having the sequence Xa Xb Xc Xd Xe Xf (SEQ ID NO. 41), wherein Xa is P, Y, T or K, Xb is an amino acid residue other than C, Xc is H, Xd is Y, L, H, V, T, I or F, Xe is Y, I, P, L, Q, S, R, T, F or A and Xf is A, W, V, Q, L, S, I, R or T.
  • According to a preferred embodiment of the present invention n is 7, 8 or 9, Z1 is an amino acid residue other than C or selected from the group consisting of F, G, F, A, P, W, Y, S, G, D, L, E, K, T, P, I and M, preferably from the group consisting of F, G, F, A, P, Y, T, S, G, K and D, and Z2 is selected from the group consisting of S, L, A, W, L, N, T, I, Y and H.
  • According to a further preferred embodiment of the present invention X1 is selected from the group consisting of D, A, R, E and L, X2 is selected from the group consisting of F, A, W, Q and R, X3 is selected from the group consisting of L, A and S, and X4 is selected from the group consisting of Q, A and H.
  • According to a preferred embodiment of the present invention X1 is D, X2 is selected from the group consisting of F, Q and W, X3 is L or S and X4 is Q or H.
  • According to a preferred embodiment of the present invention the compound comprises the amino acid sequence FX8 (F)oPX9HX10X11X12DX2X3X4X5X6X7 (SEQ ID NO. 42), wherein
  • X8 is selected from the group consisting of G, A, F, Y and K,
    X9 is selected from the group consisting of E, Y, A, Q, K and S,
    X10 is selected from the group consisting of H, V, L, F and I,
    X11 is selected from the group consisting of L, W, S, I, F and Y,
    • X12 is V, T, F or I, X5 is S or Y, X6 is L, A or I, X7 is S, N or T, and
  • o is 0 or 1.
  • The compound of the present invention comprises preferably the amino acid sequence X1X2X3X4X5X6X7 (SEQ ID NO. 43), wherein X1 is selected from the group consisting of D, S, N, T and G, X2 is F, X3 is L, X4 is selected from the group consisting of Q, D, K, R, S and E, X5 is S or T, X6 is L and X7 is an amino acid residue other than C, preferably selected from the group consisting of S, T, A, M, F and W.
  • According to a preferred embodiment of the present invention the amino acid sequence is selected from the group consisting of SSLELFL (SEQ ID NO. 44), SFLDTLT (SEQ ID NO. 45), NFLKTLS (SEQ ID NO. 46), DFLRTLT (SEQ ID NO. 47), AFLDTLV (SEQ ID NO. 48), TFLSSLA (SEQ ID NO. 49), GFLDSLM (SEQ ID NO. 50), SPHPHFL (SEQ ID NO. 51), SNFLKTL (SEQ ID NO. 52), TGFLATL (SEQ ID NO. 53), SDFLRAL (SEQ ID NO. 54), SANPRDFLETLF (SEQ ID NO. 55), RMFPESFLDTLW (SEQ ID NO. 56), TIYDSFLDSLAS (SEQ ID NO. 57), KPYLLKDFLEAL (SEQ ID NO. 58), AMGPYDALDLFL (SEQ ID NO. 59), TWNPIESFLESL (SEQ ID NO. 60), QYQTPLTFLEAL (SEQ ID NO. 61), RHISPATFLEAL (SEQ ID NO. 62), HTDSFLSTFYGD (SEQ ID NO. 63), ADSTFTSFLQTL (SEQ ID NO. 64), GPVSIYADTDFL (SEQ ID NO. 65), DSNDTLTLAAFL (SEQ ID NO. 66), TPTHYYADFSQL (SEQ ID NO. 67), LPGHLIWDSLHY (SEQ ID NO. 68), LPQTHPLHLLED (SEQ ID NO. 69), IPYHHLVDQLHH (SEQ ID NO. 70), YPYHVQVDVLQN (SEQ ID NO. 71), IPSHHLQDSLQL (SEQ ID NO. 72), EYAHHTSLDLRQ (SEQ ID NO. 73), EPLHFRSDRIQA (SEQ ID NO. 74), ATPSHLIIDRAQ (SEQ ID NO. 75), APKHLYADMSQA (SEQ ID NO. 76), FKPAHVSIDWLQ (SEQ ID NO. 77), MPAHLSRDLRQS (SEQ ID NO. 78), NPKHYSIDRHQA (SEQ ID NO. 79), SPQHLTTDRAQA (SEQ ID NO. 80), TPFHFAQDSWQW (SEQ ID NO. 81), TPTHYYADFSQLLS (SEQ ID NO. 82), TPTHYYADFSQSLS (SEQ ID NO. 83), GTPTHYYADFSQLL (SEQ ID NO. 84), GTPTHYYADFSQSL (SEQ ID NO. 85), FGTPTHYYADFSQSLS (SEQ ID NO. 86), FGFPTHYYADFSQSLS (SEQ ID NO. 87), LPGHLIWDSLHY (SEQ ID NO. 88), LPGHLIWDSLHYL (SEQ ID NO. 89), LPGHLIWDSLHYLS (SEQ ID NO. 90), LPGHLIWDSLHSL (SEQ ID NO. 91), LPGHLIWDSLHSLS (SEQ ID NO. 92), GLPGHLIWDSLHYL (SEQ ID NO. 93), GLPGHLIWDSLHSL (SEQ ID NO. 94), FGLPGHLIWDSLHSLS (SEQ ID NO. 95), FGFPGHLIWDSLHSLS (SEQ ID NO. 96), LPQTHPLHLLED (SEQ ID NO. 97), IPYHHLVDQLHH (SEQ ID NO. 98), IPYHHLVDQLHLS (SEQ ID NO. 99), IPYHHLVDQLHSLS (SEQ ID NO. 100), FGIPYHHLVDQLHHLS (SEQ ID NO. 101), FGFPYHHLVDQLHSLS (SEQ ID NO. 102), YPYHVQVDVLQN (SEQ ID NO. 103), YPYHVQVDVLQNLS (SEQ ID NO. 104), YPYHVQVDVLQSLS (SEQ ID NO. 105), FGYPYHVQVDVLQNLS (SEQ ID NO. 106), FGFPYHVQVDVLQSLS (SEQ ID NO. 107), IPSHHLQDSLQL (SEQ ID NO. 108), IPSHHLQDSLQLLS (SEQ ID NO. 109), IPSHHLQDSLQSLS (SEQ ID NO. 110), GIPSHHLQDSLQLL (SEQ ID NO. 111), FGIPSHHLQDSLQLLS (SEQ ID NO. 112), FGFPSHHLQDSLQSLS (SEQ ID NO. 113), EYAHHTSLDLRQ (SEQ ID NO. 114), EPLHFRSDRIQA (SEQ ID NO. 115), EPLHFRSDRIQALS (SEQ ID NO. 116), EPLHFRSDRIQSLS (SEQ ID NO. 117), GEPLHFRSDRIQAL (SEQ ID NO. 118), FGEPLHFRSDRIQALS (SEQ ID NO. 119), FGFPLHFRSDRIQSLS (SEQ ID NO. 120), APKHLYADMSQA (SEQ ID NO. 121), APKHLYADMSQALS (SEQ ID NO. 122), APKHLYADMSQSLS (SEQ ID NO. 123), GAPKHLYADMSQAL (SEQ ID NO. 124), FGFPKHLYADMSQSLS (SEQ ID NO. 125), MPAHLSRDLRQS (SEQ ID NO. 126), MPAHLSRDLRQSL (SEQ ID NO. 127), MPAHLSRDLRQSLS (SEQ ID NO. 128), GMPAHLSRDLRQSL (SEQ ID NO. 129), FGFPAHLSRDLRQSLS (SEQ ID NO. 130), NPKHYSIDRHQA (SEQ ID NO. 131), TPFHFAQDSWQW (SEQ ID NO. 132), TPFHFAQDSWQWLS (SEQ ID NO. 133), TPFHFAQDSWQSLS (SEQ ID NO. 134), GTPFHFAQDSWQWL (SEQ ID NO. 135), FGFPFHFAQDSWQSLS (SEQ ID NO. 136), ACSFAYLYRC (SEQ ID NO. 137), ACFMGDKWVC (SEQ ID NO. 138), ACVLYPKAIC (SEQ ID NO. 139), ACYMGQQFVC (SEQ ID NO. 140), ACLTAYLHWC (SEQ ID NO. 141), ACTLFPVAYC (SEQ ID NO. 142), ACWLFPYAHC (SEQ ID NO. 143), ACKSINMWLC (SEQ ID NO. 144), ACQTINRWLC (SEQ ID NO. 145), FGFPEHLLVDFLQSLS (SEQ ID NO. 146), FGFPEHLLVDFLQSLS (SEQ ID NO. 147), FPEHLLVDFLQSL (SEQ ID NO. 148), AGFPEHLLVDFLQSLS (SEQ ID NO. 149), FAFPEHLLVDFLQSLS (SEQ ID NO. 150), FGAPEHLLVDFLQSLS (SEQ ID NO. 151), FGFAEHLLVDFLQSLS (SEQ ID NO. 152), FGFPAHLLVDFLQSLS (SEQ ID NO. 153), FGFPEALLVDFLQSLS (SEQ ID NO. 154), FGFPEHALVDFLQSLS (SEQ ID NO. 155), FGFPEHLAVDFLQSLS (SEQ ID NO. 156), FGFPEHLLADFLQSLS (SEQ ID NO. 157), FGFPEHLLVAFLQSLS (SEQ ID NO. 158), FGFPEHLLVDALQSLS (SEQ ID NO. 159), FGFPEHLLVDFAQSLS (SEQ ID NO. 160), FGFPEHLLVDFLASLS (SEQ ID NO. 161), FGFPEHLLVDFLQALS (SEQ ID NO. 162), FGFPEHLLVDFLQSAS (SEQ ID NO. 163), FGFPEHLLVDFLQSLA (SEQ ID NO. 164), FAFPAHLLVDFLQALA (SEQ ID NO. 165), AAFPAHLLADFLQALA (SEQ ID NO. 166), SPQHLTTDRAQA (SEQ ID NO. 167), SPQHLTTDRAQALS (SEQ ID NO. 168), SPQHLTTDRAQSLS (SEQ ID NO. 169), GSPQHLTTDRAQAL (SEQ ID NO. 170), FGFPQHLTTDRAQSLS (SEQ ID NO. 171), FGFPQHLTTDWAQSLS (SEQ ID NO. 172), FGFPQHLTTDRLQSLS (SEQ ID NO. 173), FGFPQHLTTDWLQSLS (SEQ ID NO. 174), ATPSHLIIDRAQ (SEQ ID NO. 175), ATPSHLIIDRAQSLS (SEQ ID NO. 176), FGFPSHLIIDRAQSLS (SEQ ID NO. 177), FGFPSHLIIDWAQSLS (SEQ ID NO. 178), FGFPSHLIIDWLQSLS (SEQ ID NO. 179), FGFPSHLIIDWSQSLS (SEQ ID NO. 180), FATPSHLIIDWLQSLS (SEQ ID NO. 181), FKPAHVSIDWLQ (SEQ ID NO. 182), FKPAHVSIDWLQSLS (SEQ ID NO. 183), FGFPAHVSIDWLQSLS (SEQ ID NO. 184), AGFPAHVSIDWLQSLS (SEQ ID NO. 185), FAFPAHVSIDWLQSLS (SEQ ID NO. 186), FGAPAHVSIDWLQSLS (SEQ ID NO. 187), FGFAAHVSIDWLQSLS (SEQ ID NO. 188), FGFPAHVSADWLQSLS (SEQ ID NO. 189), FGFPAHVSIDWLQALS (SEQ ID NO. 190), FGFPAHVSIDWLQSLA (SEQ ID NO. 191), FAFPAHVSIDWLQALA (SEQ ID NO. 192), FGFAAHVSIDWLQSLS (SEQ ID NO. 193), FGFFAHVSIDWLQSLS (SEQ ID NO. 194), FGFPAHVSIRWLQSLS (SEQ ID NO. 195), FGFPAHVSIEWLQSLS (SEQ ID NO. 196), FGFPAHVSIDWLNSLS (SEQ ID NO. 197), FGFPAHVSIDWLHSLS (SEQ ID NO. 198), AGFPAHVSIDWLQSLS (SEQ ID NO. 199), PGFPAHVSIDWLQSLS (SEQ ID NO. 200), WGFPAHVSIDWLQSLS (SEQ ID NO. 201), FAFPAHVSIDWLQSLS (SEQ ID NO. 202), FSFPAHVSIDWLQSLS (SEQ ID NO. 203), FYFPAHVSIDWLQSLS (SEQ ID NO. 204), FDFPAHVSIDWLQSLS (SEQ ID NO. 205), FGAPAHVSIDWLQSLS (SEQ ID NO. 206), FGFPAHVSIDWLQLLS (SEQ ID NO. 207), FGFPAHVSIDWLQWLS (SEQ ID NO. 208), FGFPAHVSIDWLQNLS (SEQ ID NO. 209), FGFPAHVSIDWLQTLS (SEQ ID NO. 210), FGFPAHVSIDWLQYLS (SEQ ID NO. 211), FGFPAHVSIDWLQSIS (SEQ ID NO. 212), FGFPAHVSIDWLQSLT (SEQ ID NO. 213), FGFPAHVSIDWLQSLY (SEQ ID NO. 214), FAFPAHVFIDWLQALA (SEQ ID NO. 215), FGFPAHVSIDRAQSLS (SEQ ID NO. 216), FGFPTHVSIDWLQSLS (SEQ ID NO. 217), FGFPFHVSIDWLQSLS (SEQ ID NO. 218), FGFPAHISIDWLQSLS (SEQ ID NO. 219), FGFPAHIIIDWLQSLS (SEQ ID NO. 220), FGFPAHLTTDWLQSLS (SEQ ID NO. 221), FGFPAHVFIDWLQSLS (SEQ ID NO. 222), FGFPAHVYIDWLQSLS (SEQ ID NO. 223), FGFPAHVSLDWLQSLS (SEQ ID NO. 224), FGFPAHVSADWLQSLS (SEQ ID NO. 225), TPTHYYADFSQSLS (SEQ ID NO. 226), FGFPAHVSIDWSQSLS (SEQ ID NO. 227), FGFPAHVSIDFSQSLS (SEQ ID NO. 228), FGFPSHIIIDWLQSLS (SEQ ID NO. 239), FGFPSHLIIEWLQSLS (SEQ ID NO. 240), AAFPAHLLADAAQALA (SEQ ID NO. 241), AAFPAHAAADFLQALA (SEQ ID NO. 242), AAFAAHLLADFLQAAA (SEQ ID NO. 243), AAAPAHLLVDAAQAAA (SEQ ID NO. 244), FAFPAHVFIDWLQSLS (SEQ ID NO. 245); FGFPAHVFIDWLQALS (SEQ ID NO. 246), FGFPAHVFIDWLQSLA (SEQ ID NO. 247), GFPAHVFIDWLQSLS (SEQ ID NO. 248), FPAHVFIDWLQSLS (SEQ ID NO. 249), PAHVFIDWLQSLS (SEQ ID NO. 250), FAFPAHVFIDWLQALA (SEQ ID NO. 251), FGFPEHLFVDFLQSLS (SEQ ID NO. 252), FGFPAHVHIDWLQSLS (SEQ ID NO. 253), FGFPAHVPIDWLQSLS (SEQ ID NO. 254), FGFPSHLFIDWAQSLS (SEQ ID NO. 255), PGFPAHVFIDWLQLIT (SEQ ID NO. 256), PAHVYIDWLQSLS (SEQ ID NO. 257), FGFPAHVYIDWLQ (SEQ ID NO. 258), FGFPAHVFIDWLQ (SEQ ID NO. 259), DFGFPSHLIIDWLQSLS (SEQ ID NO. 235), DFGFPAHVFIDWLQSLN (SEQ ID NO. 260), PSHLIIDWLQ (SEQ ID NO. 261), PAHVFIDWLQ (SEQ ID NO. 262), DFGFPAHVTIDWLQSLN (SEQ ID NO. 263), DFGFPAHVLIDWLQSLN (SEQ ID NO. 264), FGFPAHVFIDWLQSLN (SEQ ID NO. 230) and FGFPAHVFIDWLQSLA (SEQ ID NO. 265).
  • Particularly preferred mimotopes to be used according to the present invention are SANPRDFLETLF (SEQ ID NO. 55), RMFPESFLDTLW (SEQ ID NO. 56), SFLDTLT (SEQ ID NO. 45), NFLKTLS (SEQ ID NO. 46), DFLRTLT (SEQ ID NO. 47), TFLSSLA (SEQ ID NO. 49), GFLDSLM (SEQ ID NO. 50), FGFPYHVQVDVLQSLS (SEQ ID NO. 107), FGFPSHLIIDRAQSLS (SEQ ID NO. 177), FKPAHVSIDWLQSLS (SEQ ID NO. 183), FGFPAHVSIDWLQSLS (SEQ ID NO. 184), FGFPQHLTTDRAQSLS (SEQ ID NO. 171), FGFPTHYYADFSQSLS (SEQ IN NO. 87), FGFPGHLIWDSLHSLS (SEQ ID NO. 96), FGFPYHHLVDQLHSLS (SEQ ID NO. 102), FGFPSHHLQDSLQSLS (SEQ ID NO. 113), FGFPLHFRSDRIQSLS (SEQ ID NO. 120), FGFPKHLYADMSQSLS (SEQ ID NO. 125), FGFPAHLSRDLRQSLS (SEQ ID NO. 130) and FGFPFHFAQDSWQSLS (SEQ ID NO. 136).
  • Especially preferred mimotopes of the present invention are FGFPSHLIIDWLQSLS (SEQ ID NO. 179), FGFPAHVFIDWLQSLS (SEQ ID NO. 222) and FGFPAHVYIDWLQSLS(SEQ ID NO. 223).
  • Further preferred mimotopes are FGFPAHVWIDWLQSLS (SEQ ID NO. 229), FGFPAHVFIDWLQSLN (SEQ ID NO. 230), FGFPAHFSIDWLQSLS (SEQ ID NO. 231), FGFPAHVSFDWLQSLS (SEQ ID NO. 232), FGFPEHVFIDWLQSLS (SEQ ID NO. 233), DFGFPAHVFIDWLQSLS (SEQ ID NO. 234), DFGFPSHLIIDWLQSLS (SEQ ID NO. 235), DFGFPAHVYIDWLQSLS (SEQ ID NO. 236), FGFPQHLFTDWLQSLS (SEQ ID NO. 237) and FGFPKHLLVDFLQSLS (SEQ ID NO. 238).
  • According to a preferred embodiment of the present invention the compound is coupled to a pharmaceutically acceptable carrier, preferably KLH (Keyhole Limpet Hemocyanin), tetanus toxoid, albumin-binding protein, bovine serum albumin, a dendrimer (MAP; Biol. Chem. 358: 581), peptide linkers (or flanking regions) as well as the adjuvant substances described in Singh et al., Nat. Biotech. 17 (1999), 1075-1081 (in particular those in Table 1 of that document), and O'Hagan et al., Nature Reviews, Drug Discovery 2 (9) (2003), 727-735 (in particular the endogenous immuno-potentiating compounds and delivery systems described therein), or mixtures thereof. The conjugation chemistry (e.g. via heterobifunctional compounds such as GMBS and of course also others as described in “Bioconjugate Techniques”, Greg T. Hermanson) in this context can be selected from reactions known to the skilled man in the art. Moreover, the vaccine composition may be formulated with an adjuvant, preferably a low soluble aluminium composition, in particular aluminium hydroxide. Of course, also adjuvants like MF59 aluminium phosphate, calcium phosphate, cytokines (e.g., IL-2, IL-12, GM-CSF), saponins (e.g., QS21), MDP derivatives, CpG oligos, LPS, MPL, polyphosphazenes, emulsions (e.g., Freund's, SAF), liposomes, virosomes, iscoms, cochleates, PLG microparticles, poloxamer particles, virus-like particles, heat-labile enterotoxin (LT), cholera toxin (CT), mutant toxins (e.g., LTK63 and LTR72), microparticles and/or polymerized liposomes may be used.
  • The compound of the present invention is preferably bound to the carrier or adjuvant via a linker, which is selected from the group consisting of NHS-poly (ethylene oxide) (PEO) (e.g. NHS-PEO4-maleimide).
  • A vaccine which comprises the present compound (mimotope) and the pharmaceutically acceptable carrier may be administered by any suitable mode of application, e.g. i.d., i.v., i.p., i.m., intranasally, orally, subcutaneously, etc. and in any suitable delivery device (O'Hagan et al., Nature Reviews, Drug Discovery 2 (9), (2003), 727-735). The compound of the present invention is preferably formulated for intravenous, subcutaneous, intradermal or intramuscular administration (see e.g. “Handbook of Pharmaceutical Manufacturing Formulations”, Sarfaraz Niazi, CRC Press Inc, 2004).
  • Typically, the vaccine contains the compound according to the invention in an amount of from 0.1 ng to 10 mg, preferably 10 ng to 1 mg, in particular 100 ng to 100 μg, or, alternatively, e.g. 100 fmol to 10 μmol, preferably 10 pmol to 1 μmol, in particular 100 pmol to 100 nmol. Typically, the vaccine may also contain auxiliary substances, e.g. buffers, stabilizers etc.
  • Another aspect of the present invention relates to a peptide consisting of at least one amino acid sequence selected from the group consisting of SYHATFL (SEQ ID NO. 2), TMAFPLN (SEQ ID NO. 3), HYHGAFL (SEQ ID NO. 4), EHHDIFL (SEQ ID NO. 5), SSLELFL (SEQ ID NO. 44), TGLSVFL (SEQ ID NO. 6), WMPSLFY (SEQ ID NO. 7), SMPWWFF (SEQ ID NO. 8), TMPLLFW (SEQ ID NO. 9), DTWPGLE (SEQ ID NO. 10), SMPPIFY (SEQ ID NO. 11), MPLWWWD (SEQ ID NO. 12), SMPNLFY (SEQ ID NO. 13), RMPPIFY (SEQ ID NO. 14), NPFEVFL (SEQ ID NO. 15), TLPNWFW (SEQ ID NO. 16), SMPLTFY (SEQ ID NO. 17), SFLDTLT (SEQ ID NO. 45), NFLKTLS (SEQ ID NO. 46), DFLRTLT (SEQ ID NO. 47), AFLDTLV (SEQ ID NO. 48), TFLSSLA (SEQ ID NO. 49), GFLDSLM (SEQ ID NO. 50), SPHPHFL (SEQ ID NO. 51), NFMSIGL (SEQ ID NO. 19), SQFLASL (SEQ ID NO. 20), SNFLKTL (SEQ ID NO. 52), TGFLATL (SEQ ID NO. 53), WSWPGLN (SEQ ID NO. 21), IAWPGLD (SEQ ID NO. 22), SKFMDTL (SEQ ID NO. 23), SDFLRAL (SEQ ID NO. 54), SMPMVFY (SEQ ID NO. 24), YEWVGLM (SEQ ID NO. 25), KGFLDHL (SEQ ID NO. 26), SANPRDFLETLF (SEQ ID NO. 55), RMFPESFLDTLW (SEQ ID NO. 56), TIYDSFLDSLAS (SEQ ID NO. 57), HQSDDKMPWWFF (SEQ ID NO. 27), KPYLLKDFLEAL (SEQ ID NO. 58), AMGPYDALDLFL (SEQ ID NO. 59), TWNPIESFLESL (SEQ ID NO. 60), YVWQDPSFTTFF (SEQ ID NO. 28), QYQTPLTFLEAL (SEQ ID NO. 61), RHISPATFLEAL (SEQ ID NO. 62), HTDSFLSTFYGD (SEQ ID NO. 63), YVWQDPSFTTFF (SEQ ID NO. 29), ADSTFTSFLQTL (SEQ ID NO. 64), GPVSIYADTDFL (SEQ ID NO. 65), DSNDTLTLAAFL (SEQ ID NO. 66), NGSPALSHMLFL (SEQ ID NO. 33), TDYDPMWVFFGY (SEQ ID NO. 34), IFPLDSQWQTFW (SEQ ID NO. 35), NESMPDLFYQPS (SEQ ID NO. 36), DWGDKYFSSFWN (SEQ ID NO. 37), VSAYNNV (SEQ ID NO. 38), WPLHLWQ (SEQ ID NO. 39), TPTHYYADFSQL (SEQ ID NO. 67), LPGHLIWDSLHY (SEQ ID NO. 68), LPQTHPLHLLED (SEQ ID NO. 69), IPYHHLVDQLHH (SEQ ID NO. 70), YPYHVQVDVLQN (SEQ ID NO. 71), IPSHHLQDSLQL (SEQ ID NO. 72), EYAHHTSLDLRQ (SEQ ID NO. 73), EPLHFRSDRIQA (SEQ ID NO. 74), ATPSHLIIDRAQ (SEQ ID NO. 75), APKHLYADMSQA (SEQ ID NO. 76), FKPAHVSIDWLQ (SEQ ID NO. 77), MPAHLSRDLRQS (SEQ ID NO. 78), NPKHYSIDRHQA (SEQ ID NO. 79), SPQHLTTDRAQA (SEQ ID NO. 80), TPFHFAQDSWQW (SEQ ID NO. 81), TPTHYYADFSQLLS (SEQ ID NO. 82), TPTHYYADFSQSLS (SEQ ID NO. 83), GTPTHYYADFSQLL (SEQ ID NO. 84), GTPTHYYADFSQSL (SEQ ID NO. 85), FGTPTHYYADFSQSLS (SEQ ID NO. 86), FGFPTHYYADFSQSLS (SEQ ID NO. 87), LPGHLIWDSLHY (SEQ ID NO. 88), LPGHLIWDSLHYL (SEQ ID NO. 89), LPGHLIWDSLHYLS (SEQ ID NO. 90), LPGHLIWDSLHSL (SEQ ID NO. 91), LPGHLIWDSLHSLS (SEQ ID NO. 92), GLPGHLIWDSLHYL (SEQ ID NO. 93), GLPGHLIWDSLHSL (SEQ ID NO. 94), FGLPGHLIWDSLHSLS (SEQ ID NO. 95), FGFPGHLIWDSLHSLS (SEQ ID NO. 96), LPQTHPLHLLED (SEQ ID NO. 97), IPYHHLVDQLHH (SEQ ID NO. 98), IPYHHLVDQLHLS (SEQ ID NO. 99), IPYHHLVDQLHSLS (SEQ ID NO. 100), FGIPYHHLVDQLHHLS (SEQ ID NO. 101), FGFPYHHLVDQLHSLS (SEQ ID NO. 102), YPYHVQVDVLQN (SEQ ID NO. 103), YPYHVQVDVLQNLS (SEQ ID NO. 104), YPYHVQVDVLQSLS (SEQ ID NO. 105), FGYPYHVQVDVLQNLS (SEQ ID NO. 106), FGFPYHVQVDVLQSLS (SEQ ID NO. 107), IPSHHLQDSLQL (SEQ ID NO. 108), IPSHHLQDSLQLLS (SEQ ID NO. 109), IPSHHLQDSLQSLS (SEQ ID NO. 110), GIPSHHLQDSLQLL (SEQ ID NO. 111), FGIPSHHLQDSLQLLS (SEQ ID NO. 112), FGFPSHHLQDSLQSLS (SEQ ID NO. 113), EYAHHTSLDLRQ (SEQ ID NO. 114), EPLHFRSDRIQA (SEQ ID NO. 115), EPLHFRSDRIQALS (SEQ ID NO. 116), EPLHFRSDRIQSLS (SEQ ID NO. 117), GEPLHFRSDRIQAL (SEQ ID NO. 118), FGEPLHFRSDRIQALS (SEQ ID NO. 119), FGFPLHFRSDRIQSLS (SEQ ID NO. 120), APKHLYADMSQA (SEQ ID NO. 121), APKHLYADMSQALS (SEQ ID NO. 122), APKHLYADMSQSLS (SEQ ID NO. 123), GAPKHLYADMSQAL (SEQ ID NO. 124), FGFPKHLYADMSQSLS (SEQ ID NO. 125), MPAHLSRDLRQS (SEQ ID NO. 126), MPAHLSRDLRQSL (SEQ ID NO. 127), MPAHLSRDLRQSLS (SEQ ID NO. 128), GMPAHLSRDLRQSL (SEQ ID NO. 129), FGFPAHLSRDLRQSLS (SEQ ID NO. 130), NPKHYSIDRHQA (SEQ ID NO. 131), TPFHFAQDSWQW (SEQ ID NO. 132), TPFHFAQDSWQWLS (SEQ ID NO. 133), TPFHFAQDSWQSLS (SEQ ID NO. 134), GTPFHFAQDSWQWL (SEQ ID NO. 135), FGFPFHFAQDSWQSLS (SEQ ID NO. 136), ACSFAYLYRC (SEQ ID NO. 137), ACFMGDKWVC (SEQ ID NO. 138), ACVLYPKAIC (SEQ ID NO. 139), ACYMGQQFVC (SEQ ID NO. 140), ACLTAYLHWC (SEQ ID NO. 141), ACTLFPVAYC (SEQ ID NO. 142), ACWLFPYAHC (SEQ ID NO. 143), ACKSINMWLC (SEQ ID NO. 144), ACQTINRWLC (SEQ ID NO. 145), FGFPEHLLVDFLQSLS (SEQ ID NO. 146), FGFPEHLLVDFLQSLS (SEQ ID NO. 147), FPEHLLVDFLQSL (SEQ ID NO. 148), AGFPEHLLVDFLQSLS (SEQ ID NO. 149), FAFPEHLLVDFLQSLS (SEQ ID NO. 150), FGAPEHLLVDFLQSLS (SEQ ID NO. 151), FGFAEHLLVDFLQSLS (SEQ ID NO. 152), FGFPAHLLVDFLQSLS (SEQ ID NO. 153), FGFPEALLVDFLQSLS (SEQ ID NO. 154), FGFPEHALVDFLQSLS (SEQ ID NO. 155), FGFPEHLAVDFLQSLS (SEQ ID NO. 156), FGFPEHLLADFLQSLS (SEQ ID NO. 157), FGFPEHLLVAFLQSLS (SEQ ID NO. 158), FGFPEHLLVDALQSLS (SEQ ID NO. 159), FGFPEHLLVDFAQSLS (SEQ ID NO. 160), FGFPEHLLVDFLASLS (SEQ ID NO. 161), FGFPEHLLVDFLQALS (SEQ ID NO. 162), FGFPEHLLVDFLQSAS (SEQ ID NO. 163), FGFPEHLLVDFLQSLA (SEQ ID NO. 164), FAFPAHLLVDFLQALA (SEQ ID NO. 165), AAFPAHLLADFLQALA (SEQ ID NO. 166), SPQHLTTDRAQA (SEQ ID NO. 167), SPQHLTTDRAQALS (SEQ ID NO. 168), SPQHLTTDRAQSLS (SEQ ID NO. 169), GSPQHLTTDRAQAL (SEQ ID NO. 170), FGFPQHLTTDRAQSLS (SEQ ID NO. 171), FGFPQHLTTDWAQSLS (SEQ ID NO. 172), FGFPQHLTTDRLQSLS (SEQ ID NO. 173), FGFPQHLTTDWLQSLS (SEQ ID NO. 174), ATPSHLIIDRAQ (SEQ ID NO. 175), ATPSHLIIDRAQSLS (SEQ ID NO. 176), FGFPSHLIIDRAQSLS (SEQ ID NO. 177), FGFPSHLIIDWAQSLS (SEQ ID NO. 178), FGFPSHLIIDWLQSLS (SEQ ID NO. 179), FGFPSHLIIDWSQSLS (SEQ ID NO. 180), FATPSHLIIDWLQSLS (SEQ ID NO. 181), FKPAHVSIDWLQ (SEQ ID NO. 182), FKPAHVSIDWLQSLS (SEQ ID NO. 183), FGFPAHVSIDWLQSLS (SEQ ID NO. 184), AGFPAHVSIDWLQSLS (SEQ ID NO. 185), FAFPAHVSIDWLQSLS (SEQ ID NO. 186), FGAPAHVSIDWLQSLS (SEQ ID NO. 187), FGFAAHVSIDWLQSLS (SEQ ID NO. 188), FGFPAHVSADWLQSLS (SEQ ID NO. 189), FGFPAHVSIDWLQALS (SEQ ID NO. 190), FGFPAHVSIDWLQSLA (SEQ ID NO. 191), FAFPAHVSIDWLQALA (SEQ ID NO. 192), FGFAAHVSIDWLQSLS (SEQ ID NO. 193), FGFFAHVSIDWLQSLS (SEQ ID NO. 194), FGFPAHVSIRWLQSLS (SEQ ID NO. 195), FGFPAHVSIEWLQSLS (SEQ ID NO. 196), FGFPAHVSIDWLNSLS (SEQ ID NO. 197), FGFPAHVSIDWLHSLS (SEQ ID NO. 198), AGFPAHVSIDWLQSLS (SEQ ID NO. 199), PGFPAHVSIDWLQSLS (SEQ ID NO. 200), WGFPAHVSIDWLQSLS (SEQ ID NO. 201), FAFPAHVSIDWLQSLS (SEQ ID NO. 202), FSFPAHVSIDWLQSLS (SEQ ID NO. 203), FYFPAHVSIDWLQSLS (SEQ ID NO. 204), FDFPAHVSIDWLQSLS (SEQ ID NO. 205), FGAPAHVSIDWLQSLS (SEQ ID NO. 206), FGFPAHVSIDWLQLLS (SEQ ID NO. 207), FGFPAHVSIDWLQWLS (SEQ ID NO. 208), FGFPAHVSIDWLQNLS (SEQ ID NO. 209), FGFPAHVSIDWLQTLS (SEQ ID NO. 210), FGFPAHVSIDWLQYLS (SEQ ID NO. 211), FGFPAHVSIDWLQSIS (SEQ ID NO. 212), FGFPAHVSIDWLQSLT (SEQ ID NO. 213), FGFPAHVSIDWLQSLY (SEQ ID NO. 214), FAFPAHVSIDWLQALA (SEQ ID NO. 215), FGFPAHVSIDRAQSLS (SEQ ID NO. 216), FGFPTHVSIDWLQSLS (SEQ ID NO. 217), FGFPFHVSIDWLQSLS (SEQ ID NO. 218), FGFPAHISIDWLQSLS (SEQ ID NO. 219), FGFPAHIIIDWLQSLS (SEQ ID NO. 220), FGFPAHLTTDWLQSLS (SEQ ID NO. 221), FGFPAHVFIDWLQSLS (SEQ ID NO. 222), FGFPAHVYIDWLQSLS (SEQ ID NO. 223), FGFPAHVSLDWLQSLS (SEQ ID NO. 224), FGFPAHVSADWLQSLS (SEQ ID NO. 225), TPTHYYADFSQSLS (SEQ ID NO. 226), FGFPAHVWIDWLQSLS (SEQ ID NO. 229), FGFPAHVFIDWLQSLN (SEQ ID NO. 230), FGFPAHFSIDWLQSLS (SEQ ID NO. 231), FGFPAHVSFDWLQSLS (SEQ ID NO. 232), FGFPEHVFIDWLQSLS (SEQ ID NO. 233), DFGFPAHVFIDWLQSLS (SEQ ID NO. 234), DFGFPSHLIIDWLQSLS (SEQ ID NO. 235), DFGFPAHVYIDWLQSLS (SEQ ID NO. 236), FGFPQHLFTDWLQSLS (SEQ ID NO. 237), FGFPKHLLVDFLQSLS (SEQ ID NO. 238), FGFPAHVSIDFSQSLS (SEQ ID NO. 227), FGFPAHVSIDFSQSLS (SEQ ID NO. 228), FGFPSHIIIDWLQSLS (SEQ ID NO. 239), FGFPSHLIIEWLQSLS (SEQ ID NO. 240), AAFPAHLLADAAQALA (SEQ ID NO. 241), AAFPAHAAADFLQALA (SEQ ID NO. 242), AAFAAHLLADFLQAAA (SEQ ID NO. 243), AAAPAHLLVDAAQAAA (SEQ ID NO. 244), FAFPAHVFIDWLQSLS (SEQ ID NO. 245); FGFPAHVFIDWLQALS (SEQ ID NO. 246), FGFPAHVFIDWLQSLA (SEQ ID NO. 247), GFPAHVFIDWLQSLS (SEQ ID NO. 248), FPAHVFIDWLQSLS (SEQ ID NO. 249), PAHVFIDWLQSLS (SEQ ID NO. 250), FAFPAHVFIDWLQALA (SEQ ID NO. 251), FGFPEHLFVDFLQSLS (SEQ ID NO. 252), FGFPAHVHIDWLQSLS (SEQ ID NO. 253), FGFPAHVPIDWLQSLS (SEQ ID NO. 254), FGFPSHLFIDWAQSLS (SEQ ID NO. 255), PGFPAHVFIDWLQLIT (SEQ ID NO. 256), PAHVYIDWLQSLS (SEQ ID NO. 257), FGFPAHVYIDWLQ (SEQ ID NO. 258), FGFPAHVFIDWLQ (SEQ ID NO. 259), DFGFPAHVFIDWLQSLN (SEQ ID NO. 260), PSHLIIDWLQ (SEQ ID NO. 261), PAHVFIDWLQ (SEQ ID NO. 262), DFGFPAHVTIDWLQSLN (SEQ ID NO. 263), DFGFPAHVLIDWLQSLN (SEQ ID NO. 264), and FGFPAHVFIDWLQSLA (SEQ ID NO. 265).
  • The peptides of the present invention turned out to be mimotopes for CETP and, hence, the mimotopes were able to bind to antibodies binding to the CETP fragment C-FGFPEHLLVDFLQSLS (SEQ ID NO. 146) (16 C-terminal amino acids of CETP protein).
  • Yet, another aspect of the present invention relates to a pharmaceutical formulation comprising at least one peptide according to the present invention.
  • The peptides of the present invention may be formulated in a pharmaceutical formulation which may be administered to an individual. These formulations may be used, e.g., for preventing and/or treating atherosclerosis, atherosclerosis risk diseases and atherosclerosis sequelae.
  • The peptides in the formulation can be combined from the pool of peptides disclosed herein. Furthermore is also possible to provide pharmaceutical formulations, which comprise one or more of the peptides of the present invention, and which can be administered separately or together to an individual in need thereof.
  • The peptides of the present invention can be mixed into one single pharmaceutical formulation or in a combination of two or three. The resulting formulation can be administered at the same or the different moments in time. According to a preferred embodiment of the present invention the peptide present in the formulation is coupled to a pharmaceutically acceptable carrier, preferably KLH (Keyhole Limpet Hemocyanin).
  • The present invention is further illustrated by the following figures and examples, however, without being restricted thereto.
  • FIG. 1 shows the result of a representative competition ELISA after screening phage display library Ph.D. 7 with monoclonal antibody “Paula”.
  •
    FGFPEHLLVDFLQSLS SEQ ID NO. 146
    FGFPEHLLVDFLQSLS SEQ ID NO. 147
    SYHATFL SEQ ID NO. 2
    TMAFPLN SEQ ID NO. 3
    HYHGAFL SEQ ID NO. 4
    EHHDIFL SEQ ID NO. 5
    SSLELFL SEQ ID NO. 44
    TGLSVFL SEQ ID NO. 6
    WMPSLFY SEQ ID NO. 7
    SMPWWFF SEQ ID NO. 8
    TMPLLFW SEQ ID NO. 9
    DTWPGLE SEQ ID NO. 10
    SMPPIFY SEQ ID NO. 11
    MPLWWWD SEQ ID NO. 12
    SMPNLFY SEQ ID NO. 13
    RMPPIFY SEQ ID NO. 14
    NPFEVFL SEQ ID NO. 15
    TLPNWFW SEQ ID NO. 16
  • FIGS. 2 a and 2 b show the results of 2 typical competition ELISAs after screening phage display library Ph.D. 12 with monoclonal antibody “Paula”.
  •
    FGFPEHLLVDFLQSLS SEQ ID NO. 146
    FGFPEHLLVDFLQSLS SEQ ID NO. 147
    RHISPATFLEAL SEQ ID NO. 62
    TIYDSFLDSLAS SEQ ID NO. 57
    HTDSFLSTFYGD SEQ ID NO. 63
    ADSTFTSFLQTL SEQ ID NO. 64
    GPVSIYADTDFL SEQ ID NO. 65
    DSNDTLTLAAFL SEQ ID NO. 66
    NGSPALSHMLFL SEQ ID NO. 33
    TDYDPMWVFFGY SEQ ID NO. 34
    IFPLDSQWQTFW SEQ ID NO. 35
    NESMPDLFYQPS SEQ ID NO. 36
    DWGDKYFSSFWN SEQ ID NO. 37
    HQSDDKMPWWFF SEQ ID NO. 27
    KPYLLKDFLEAL SEQ ID NO. 58
    SANPRDFLETLF SEQ ID NO. 55
    RMFPESFLDTLW SEQ ID NO. 56
    AMGPYDALDLFL SEQ ID NO. 59
    TWNPIESFLESL SEQ ID NO. 60
    YVWQDPSFTTFF SEQ ID NO. 29
    QYQTPLTFLEAL SEQ ID NO. 61
  • FIGS. 3 a and 3 b show the results of 2 representative competition ELISAs after screening phage display library Ph.D. 7 with mAb Frida.
  •
    FGFPEHLLVDFLQSLS SEQ ID NO. 146
    FGFPEHLLVDFLQSLS SEQ ID NO. 147
    WPLHLWQ SEQ ID NO. 39
    VSAYNNV SEQ ID NO. 38
  • FIG. 4 a shows the result of a representative competition ELISA after screening phage display library Ph.D. 12 with monoclonal antibody “Frida”.
  •
    FGFPEHLLVDFLQSLS SEQ ID NO. 146
    FGFPEHLLVDFLQSLS SEQ ID NO. 147
    TPTHYYADFSQL SEQ ID NO. 67
    LPGHLIWDSLHY SEQ ID NO. 68
    LPQTHPLHLLED SEQ ID NO. 69
  • FIG. 4 b shows binding of monoclonal antibody “Frida” to ELISA plates coated with mimotope-BSA
  • FIGS. 5 a and 5 b show the results of a representative competition ELISA after screening phage display library Ph.D. 12 with monoclonal antibody “Frida”.
  •
    FGFPEHLLVDFLQSLS SEQ ID NO. 146
    FGFPEHLLVDFLQSLS SEQ ID NO. 147
    GTPTHYYADFSQLL SEQ ID NO. 84
    GTPTHYYADFSQSL SEQ ID NO. 85
    FGTPTHYYADFSQSLS SEQ ID NO. 86
    FGFPTHYYADFSQSLS SEQ ID NO. 87
    GLPGHLIWDSLHYL SEQ ID NO. 93
    GLPGHLIWDSLHSL SEQ ID NO. 94
    FGLPGHLIWDSLHSLS SEQ ID NO. 95
    FGFPGHLIWDSLHSLS SEQ ID NO. 96
    FGIPYHHLVDQLHHLS SEQ ID NO. 101
    FGFPYHHLVDQLHSLS SEQ ID NO. 102
    FGYPYHVQVDVLQNLS SEQ ID NO. 106
    FGFPYHVQVDVLQSLS SEQ ID NO. 107
    GIPSHHLQDSLQLL SEQ ID NO. 111
    FGIPSHHLQDSLQLLS SEQ ID NO. 112
    FGFPSHHLQDSLQSLS SEQ ID NO. 113
    GEPLHFRSDRIQAL SEQ ID NO. 118
    FGEPLHFRSDRIQALS SEQ ID NO. 119
    FGFPLHFRSDRIQSLS SEQ ID NO. 120
    ATPSHLIIDRAQSLS SEQ ID NO. 176
    FGFPSHLIIDRAQSLS SEQ ID NO. 177
    GAPKHLYADMSQAL SEQ ID NO. 124
    FGFPKHLYADMSQSLS SEQ ID NO. 125
    FKPAHVSIDWLQSLS SEQ ID NO. 183
    FGFPAHVSIDWLQSLS SEQ ID NO. 184
    GMPAHLSRDLRQSL SEQ ID NO. 129
    FGFPAHLSRDLRQSLS SEQ ID NO. 130
    GSPQHLTTDRAQAL SEQ ID NO. 170
    FGFPQHLTTDRAQSLS SEQ ID NO. 171
    GTPFHFAQDSWQWL SEQ ID NO. 135
    FGFPFHFAQDSWQSLS SEQ ID NO. 136
  • FIG. 6 shows the results of a competition ELISA of two mimotopes after screening phage display library Ph.D. 12 with monoclonal antibody “Frida”.
  •
    FGFPEHLLVDFLQSLS SEQ ID NO. 146
    FGFPEHLLVDFLQSLS SEQ ID NO. 147
    FGFPSHLIIDWAQSLS SEQ ID NO. 178
    FGFPSHLIIDWLQSLS SEQ ID NO. 179
  • FIGS. 7 a to 7 d show the antibody titer (anti mouse IgG) of in vivo experiments, whereby the following mimotope-BSA conjugates were injected into mice:
  •
    Fr12/3/26/65 ext4 C-FGFPYHVQ  (SEQ ID NO. 107) p4286
    VDVLQSLS
    Fr12/3/55 ext2 C-FGFPSHLIIDRA (SEQ ID NO. 177) p4294
    QSLS
    Fr12/3/55 ext2 W instead of R  (SEQ ID NO. 178) p4324
    C-FGFPSHLIIDWAQSLS
    Fr12/3/55 ext2 WL instead of   (SEQ ID NO. 179) p4325
    RAC-FGFPSHLIIDWLQSLS
    Fr12/3/84 ext2 C-FGFPAHVSIDWL  (SEQ ID NO. 184) p4298
    QSLS
    Fr12/3/40 ext4 C-FGFPQHLTTDRA (SEQ ID NO. 171) p4302
    QSLS
    Fr12/2/6 ext6 C-FGFPTHYYADFS  (SEQ ID NO. 87) p4278
    QSLS
    Fr12/2/11 ext7 C-FGFPGHLIWDSL  (SEQ ID NO. 96) p4282 
    HSLS
    Fr12/3/1/19/88 ext4 C-FGFPYHHL (SEQ ID NO. 102) p4284
    VDQLHSLS
    Fr12/3/68 ext5 C-FGFPSHHLQDSL (SEQ ID NO. 113) p4289
    QSLS
    Fr12/3/83 ext5 C-FGFPLHFRSDRI (SEQ ID NO. 120) p4292
    QSLS
    Fr12/3/63 ext4 C-FGFPKHLYADMS (SEQ ID NO. 125) p4296
    QSLS
    Fr12/3/47 ext4 C-FGFPAHLSRDL (SEQ ID NO. 130) p4300
    RQSL
    Fr12/3/35 ext4 C-FGFPFHFAQDSW (SEQ ID NO. 136) p4304
    QSLS
  • FIGS. 8 a and 8 b show the results of two representative competition ELISA after screening phage display library Ph.D. 7C7 with monoclonal antibody “Frida”.
  •
    FGFPEHLLVDFLQSLS SEQ ID NO. 146
    FGFPEHLLVDFLQSLS SEQ ID NO. 147
    ACSFAYLYRC SEQ ID NO. 137
    ACYMGQQFVC SEQ ID NO. 140
    ACLTAYLHWC SEQ ID NO. 141
    ACTLFPVAYC SEQ ID NO. 142
    ACWLFPYAHC SEQ ID NO. 143
    ACQTINRWLC SEQ ID NO. 145
  • FIG. 9 shows an in vitro ELISA test for the detection of the binding between “Frida” and cyclic mimotopes.
  •
    FGFPEHLLVDFLQSLS SEQ ID NO. 147
    ACSFAYLYRC SEQ ID NO. 137
    ACYMGQQFVC SEQ ID NO. 140
    ACLTAYLHWC SEQ ID NO. 141
    ACTLFPVAYC SEQ ID NO. 142
    ACWLFPYAHC SEQ ID NO. 143
    ACQTINRWLC SEQ ID NO. 145
  • FIGS. 10 a and 10 b show the results of an inhibition ELISA assay with FGFPSHLIIDWLQSLS (SEQ ID NO. 179), FGFPAHVFIDWLQSLS (SEQ ID NO. 222) and FGFPAHVYIDWLQSLS (SEQ ID NO. 223).
  • FIG. 10 a (Coat 1 μM peptide. Detection αIgG1)
  • 2.5 ng mAb Frida
    Frida
    2 μg 20 μg
    pept N° peptide peptide
    buffer only 1.05 0.96
    p4073 original epitope C-FGFPEHLLVDFLQSLS 0.44 0.1
    p1358 irrelevant peptide irrelevant peptide 1.08 0.91
    p4361 FGFPAHVFIDWLQSLS Fr12/3/84 ext2 VSI
    Figure US20140179900A1-20140626-P00001
    VFI    		 0.82 0.16
    p4362 FGFPAHVYIDWLQSLS Fr12/3/84 ext2 VSI
    Figure US20140179900A1-20140626-P00001
    VYI    		 0.75 0.15
  • FIG. 10 b (Coat 1 μM peptide. Detection αIgG1)
  • 2.5 ng mAb Firda
    Frida
    2 μg 20 μg
    pept No peptide peptide
    buffer only 0.84 0.75
    p4073 original epitope C-FGFPEHLLVDFLQSLS 0.64 0.15
    p1358 irrelevant peptide irrelevant peptide 0.88 0.77
    p4325 FGFPSHLIIDWLQSLS Fr12/3/55 ext2 RA
    Figure US20140179900A1-20140626-P00002
    WL    		 0.42 0.1
  • FIG. 11 shows the in vivo induction of antibodies directed to CETP by mimotopes of the invention that are administered to mice. Balb/c mice/30 μg Peptide, 2 injections in 2 week intervals. S3=2 weeks after 3rd injection. Alum as adjuvant. Titers against original epitope (p4073) induced by injection of mimotopes. Well coating: 50 μl of 1 μM p4073-BSA or 1 μg/ml activated KLH. Detection: αIgG:
  • injected original irrelevant
    peptide- epitope-peptide-
    BSA BSA BSA
    group
     1 KLH KLH 2.040 400 
    group 2 original epitope p4073-KLH 8.600 10
    group 3 C-FGFPQHLTTDWLQSLS p4369-KLH 14.000 12.900 10
    (SEQ ID NO. 174)
    group 4 C-FGFPSHLIIDWAQSLS p4324-KLH 12.570 7.600 10
    (SEQ ID NO. 178)
    group 5 C-FGFPSHLIIDWLQSLS p4325-KLH 2.930 1.820 10
    (SEQ ID NO. 179)
    group 6 C-FGFPSHLIIDWSQSLS p4366-KLH 4.700 3.600 10
    (SEQ ID NO. 180)
    group 7 C-FATPSHLIIDWLQSLS p4345-KLH 8.380 1.270 10
    (SEQ ID NO. 181)
    group 8 C-FAFPAHVSIDWLQALA p4328-KLH 10.100 2.740 400 
    (SEQ ID NO. 186)
    group 9 C-PGFPAHVSIDWLQSLS p4340-KLH 18.100 15.640 10
    (SEQ ID NO. 200)
    group C-WGFPAHVSIDWLQSLS p4341-KLH 10.350 5.500 10
    10 (SEQ ID NO. 201)
    group C-FSFPAHVSIDWLQSLS p4342-KLH 4.620 1.610 10
    11 (SEQ ID NO. 203)
    group C-FYFPAHVSIDWLQSLS p4343-KLH 5.580 2.900 10
    12 (SEQ ID NO. 204)
    group C-FDFPAHVSIDWLQSLS p4344-KLH 12.200 3.580 10
    13 (SEQ ID NO. 205)
    group C-FGFPAHVSIDWLQLLS p4347-KLH 12.000 9.160 10
    14 (SEQ ID NO. 207)
    group C-FGFPAHVSIDWLQYLS p4351-KLH 2.950 2.400 10
    15 (SEQ ID NO. 211)
    group C-FGFPAHVSIDWLQSIS p4352-KLH 19.680 12.070 10
    16 (SEQ ID NO. 212)
    group C-FGFPAHVSIDWLQSLT p4353-KLH 11.200 8.650 10
    17 (SEQ ID NO. 213)
    group C-FGFPAHISIDWLQSLS p4358-KLH 16.500 12.940 10
    18 (SEQ ID NO. 219)
    group C-FGFPAHIIIDWLQSLS p4359-KLH 8.540 5.340 10
    19 (SEQ ID NO. 220)
    group C-FGFPAHVFIDWLQSLS p4361-KLH 17.940 9.530 10
    20 (SEQ ID NO. 222)
  • FIGS. 12 a and 12 b show the in vivo induction of CETP specific antibodies by the administration of the mimotopes of the invention. Titers to p4073 and its correlation to titers to CETP of selected groups (which show high titers against p4073): gr.4, gr.9, gr.10, gr.14, gr.16-20/gr.1 (KLH), gr.2 (original epitope) as controls. Coating: recombinant GST-CETP or purified rabbit CETP, respectively:
  • FIG. 12 a
  • recombinant rabbit
    GST-CETP CETP
    group
     1 KLH KLH/ 0.35 0.19
    Alum
    group
     2 original epitope p4073- 1.49 1.25
    KLH/
    Alum
    group 3 C-FGFPQHLTTDWLQSLS p4369- 0.45 0.21
    (SEQ ID NO. 174) KLH/
    Alum
    group 4 C-FGFPSHLIIDWAQSLS p4324- 0.58 0.28
    (SEQ ID NO. 178) KLH/
    Alum
    group 9 C-PGFPAHVSIDWLQSLS p4340- 0.49 0.21
    (SEQ ID NO. 200) KLH/
    Alum
    group 10 C-WGFPAHVSIDWLQSLS p4341- 0.39 0.18
    (SEQ ID NO. 201) KLH/
    Alum
    group 14 C-FGFPAHVSIDWLQLLS p4347- 0.35 0.2
    (SEQ ID NO. 207) KLH/
    Alum
    group 16 C-FGFPAHVSIDWLQSIS p4352- 0.48 0.28
    (SEQ ID NO. 212) KLH/
    Alum
    group 17 C-FGFPAHVSIDWLQSLT p4353- 0.57 0.39
    (SEQ ID NO. 213) KLH/
    Alum
    group 18 C-FGFPAHISIDWLQSLS p4358- 0.68 0.58
    (SEQ ID NO. 219) KLH/
    Alum
    group 19 C-FGFPAHIIIDWLQSLS p4359- 0.79 0.54
    (SEQ ID NO. 220) KLH/
    Alum
    group 20 C-FGFPAHVFIDWLQSLS p4361- 1.64 1.51
    (SEQ ID NO. 222) KLH/
    Alum

    FIG. 12 b
  • recombinant rabbit
    GST-CETP CETP
    group
     1 KLH KLH/ 0.18 0.47
    Alum
    group
     2 original epitope p4073- 1.26 1.42
    KLH/
    Alum
    group 5 C-FGFPSHLIIDWLQSLS p4325- 0.59 0.85
    (SEQ ID NO. 179) KLH/
    Alum
    group 6 C-FGFPSHLIIDWSQSLS p4366- 0.4 0.65
    (SEQ ID NO. 180) KLH/
    Alum
    group 7 C-FATPSHLIIDWLQSLS p4345- 0.39 0.46
    (SEQ ID NO. 181) KLH/
    Alum
    group 8 C-FAFPAHVSIDWLQALA p4328- 0.45 0.43
    (SEQ ID NO. 186) KLH/
    Alum
    group 11 C-FSFPAHVSIDWLQSLS p4342- 0.38 0.41
    (SEQ ID NO. 203) KLH/
    Alum
    group 12 C-FYFPAHVSIDWLQSLS p4343- 0.61 1.05
    (SEQ ID NO. 204) KLH/
    Alum
    group 13 C-FDFPAHVSIDWLQSLS p4344- 0.35 0.43
    (SEQ ID NO. 205) KLH/
    Alum
    group 15 C-FGFPAHVSIDWLQYLS p4351- 0.54 0.59
    (SEQ ID NO. 211) KLH/
    Alum
  • FIG. 13 shows the in vivo induction of antibodies directed to CETP by mimotopes of the invention that are administered to mice.
  • Sera of each group (5 Balb/c mice each) were combined, diluted 1:100 and tested on ELISA plates coated with recombinant GST-CETP or rabbit CETP, respectively. Detection of bound antibodies was with algG.
  • recombinant rabbit
    GST-CETP CETP
    group
     1 KLH KLH/ 0.23 0.17
    Alum
    group
     2 original epitope p4073- 1.08 0.46
    KLH/
    Alum
    group 3 C-FGFAAHVSIDWLQSLS p4335- 0.26 0.14
    (SEQ ID NO. 188) KLH/
    Alum
    group 4 C-FGFPAHVSIDWLQWLS p4348- 0.33 0.16
    (SEQ ID NO. 208) KLH/
    Alum
    group 5 C-FGFPAHLTTDWLQSLS p4360- 0.4 0.23
    (SEQ ID NO. 221) KLH/
    Alum
    group 6 C-FGFPAHVYIDWLQSLS p4362- 0.86 0.94
    (SEQ ID NO. 223) KLH/
    Alum
    group 7 C-FGFPAHVSIDWLQSLY P4354- 0.29 0.23
    (SEQ ID NO. 214) KLH/
    Alum
    group 8 C-FGFPAHVSIRWLQSLS p4337- 0.24 0.14
    (SEQ ID NO. 195) KLH/
    Alum
  • FIG. 14 shows a CETP activity assay, wherein 0.6 μl human serum (with endogenous CETP activity) is mixed with serum from wild-type mice (not containing CETP activity) vaccinated with KLH/Alum (negative control group), p4703-KLH/Alum (original CETP epitope), or p4361 (or p4362 or p 4325) mimotope, respectively. It could be demonstrated that the addition of 1.2 μl and 0.6 μl serum from p4361-KLH/Alum vaccinated mice completely inhibits CETP activity and the addition of 0.2 μl serum reduces significantly said activity in contrast to the addition of serum from mice vaccinated with KLH/Alum-control only or with the original epitope (p4073-KLH/Alum).
  • SEQ ID NO. 146
    FGFPEHLLVDFLQSLS
    SEQ ID NO. 222
    FGFPAHVFIDWLQSLS
  • FIG. 15 shows that the addition of p4325-KLH/Alum to human serum inhibits significantly CETP activity.
  • SEQ ID NO. 179
    FGFPSHLIIDWLQSLS
  • FIG. 16 shows that the addition of p4361-KLH/Alum to human serum inhibits significantly CETP activity.
  • SEQ ID NO. 146
    FGFPEHLLVDFLQSLS
    SEQ ID NO. 222
    FGFPAHVFIDWLQSLS
  • FIG. 17 shows that the addition of p4362-KLH/Alum to human serum inhibits significantly CETP activity.
  • SEQ ID NO. 146
    FGFPEHLLVDFLQSLS
    SEQ ID NO. 221
    FGFPAHLTTDWLQSLS
    SEQ ID NO. 223
    FGFPAHVYIDWLQSLS
  • FIG. 18 a shows an inhibition ELISA with mimotopes (Coat. 1 μM 4073 peptide, detection α IgG1).
  • Frida 2.5 ng mAB Frida
    pept No low high
    buffer only buffer only buffer only 1.084 1.079
    4% DMSO 4% DMSO 4% DMSO 1.180 1.201
    p4073 C-FGFPEHLLVDFLQSLS p4073 0.537 0.094
    (SEQ ID NO. 147),
    positive control
    peptide
    p1208 positive control p1208 0.712 0.093
    peptide FGFPEH-
    LLVDFLQSLS-C
    (SEQ ID NO. 146)
    p1358 negative control p1358 1.158 1.050
    peptide
    p4474 C-PAVVYIDWLQSLS Fr12/3/84 ext2 1.452 0.179
    (SEQ ID NO. 257) VSI
    Figure US20140179900A1-20140626-P00003
    VFI SLS
    Figure US20140179900A1-20140626-P00003
    SLN
    p4475 C-FGFPAHFSIDWLQSLS Fr12/3/84 ext2 2.211 1.429
    (SEQ ID NO. 231) VSI
    Figure US20140179900A1-20140626-P00003
    FSI
    p4476 C-FGFPAHVSFDWLQSLS Fr12/3/84 ext2 2.000 1.417
    (SEQ ID NO. 232) VSI
    Figure US20140179900A1-20140626-P00003
    VSF
    p4477 C-FGFPEHVFIDWLQSLS Fr12/3/84 ext2 0.808 0.116
    (SEQ ID NO. 233) VSI
    Figure US20140179900A1-20140626-P00003
    VFI PAH
    Figure US20140179900A1-20140626-P00003
    PEH
    p4478 C-FKPAHVFIDWLQSLS Fr12/3/84 ext1 2.231 1.206
    (SEQ ID NO. 266) VSI
    Figure US20140179900A1-20140626-P00003
    VFI
    p4479 C-GFKPAHVFIDWLQSLS Fr12/3/84 ext1 2.165 1.591
    (SEQ ID NO. 267) VSI
    Figure US20140179900A1-20140626-P00003
    VFI plus G
    on N-terminus
    p4480 C-DFGPAHVFIDWLQSLS Fr12/3/84 ext2 0.521 0.103
    (SEQ ID NO. 234) VSI
    Figure US20140179900A1-20140626-P00003
    VFI plus D
    on N-terminus; =
    4361 plus D
    p4481 C-FGFPQHLFTDWLQSLS Fr12/3/40 ext4 0.551 0.156
    (SEQ ID NO. 237) RA
    Figure US20140179900A1-20140626-P00003
    WL LTT
    Figure US20140179900A1-20140626-P00003
    LFT =
    p4369 with exchange
    T
    Figure US20140179900A1-20140626-P00003
    F
  • FIG. 18 b shows an inhibition ELISA with mimotopes (Coat. 1 μM 4073 peptide, detection α IgG1).
  •
    p1208 positive control p1208 0.264 0.079
    peptide
    p1358 negative control p1358 1.902 1.661
    peptide
    p4629 C-PAHVYIDWLQSLS C-terminus of p4362; 0.313 0.118
    (SEQ ID NO. 257) p4362 minus 3 aa on N-terminus
    p4630 C-FGFPAHVYIDWLQ N-terminus of p4362 2.131 2.115
    (SEQ ID NO. 258) (minus 3 aa on C-terminus)
    p4631 C-FGFPAHVFIDWLQ N-terminus of p4361 2.111 2.147
    (SEQ ID NO. 259) (minus 3 aa on C-terminus)
    p4642 C-DFGFPHSHLIIDWLQSLS Fr12/3/55 ext2 RA → 0.171 0.082
    (SEQ ID NO. 235) WL plus D; p4325
    plus D on N-terminus
    p4818 C-DFGFPAHVFIDWLQSLN FR12/3/84 ext 2 VSI → 0.332 0.091
    (SEQ ID NO. 260) VFI SLS → SLN plus D; =
    4361 N hinten plus D vorne
    p4819 C-PSHLIIDWLQ = 4325 minus 3AA am N 2.226 2.158
    (SEQ ID NO. 261) und am C-Terminus
    p4820 C-PAHVFIDWLQ = 4361 minus 3AA am N 2.310 2.374
    (SEQ ID NO. 262) und am C-Terminus
    p4989 C-DFGFPAHVTIDWLQSLN Fr12/3/84 ext2 VSI → 0.932 0.274
    (SEQ ID NO. 263) VTI; = p4361 F replaced by T,
    plus D on N-term and N
    instead of S on C-term
    p4990 C-DFGFPAHVLIDWLQSLN Fr12/3/84 ext2 VSI → 0.263 0.073
    (SEQ ID NO. 264) VLI; = p4361 F replaced by L,
    plus D on N-term and N
    instead of S on C-term
    p5067 FGFPAHVYIDWLQSLS-C p4362 C on C-terminus 0.563 0.217
    (SEQ ID NO. 223)
    p5068 FGFPAHVFIDWLQSLN-C p4474 C on C-terminus 0.757 0.271
    (SEQ ID NO. 230)
  • FIG. 18 c shows a inhibition ELISA with mimotopes screen PhD12 Frida and Ala-exchange for mimotope characterisation/mAb Frida (Coat 1 μM 4073. Detection αIgG1.)
  • Frida 2.5 ng mAb Frida
    pept No low high
    buffer only buffer only 0.964 0.964
    4% DMSO 4% DMSO 0.973 0.923
    positive control p4073 0.554 0.088
    peptide
    p1208 p1208 0.942 0.101
    negative control p1358 0.986 0.93
    peptide
    p4432 C-FGFPSHIIIDWLQSLS Fr12/3/55 ext2exch2 0.635 0.096
    (SEQ ID NO. 239) L −> I
    p4433 C-FGFPSHLIIEWLQSLS Fr12/3/55 ext2exch2 1.114 0.672
    (SEQ ID NO. 240) D −> E
    p4434 C-AAFPAHLLADAAQALA Ala-exchange for 1.74 1.461
    (SEQ ID NO. 241) mimotope characterisation
    p4435 C-AAFPAHAAADFLQALA Ala-exchange for 1.281 1.969
    (SEQ ID NO. 242) mimotope characterisation
    p4436 C-AAFAAHLLADFLQAAA Ala-exchange for 1.632 1.691
    (SEQ ID NO. 243) mimotope characterisation
    p4437 C-AAAPAHLLVDAAQAAA Ala-exchange for 1.84 1.674
    (SEQ ID NO. 244) mimotope characterisation
  • FIG. 19 a shows a peptide ELISA, immunisation with C-DFGFPAHVYIDWLQSLS (p4628-KLH/Alum) (SEQ ID NO. 236), titre to original epitope.
  • FIG. 19 b shows a peptide ELISA, immunisation with C-FGFPAHVFIDWLQSLN (p4474-KLH/Alum) (SEQ ID NO. 230), titre to original epitope.
  • FIG. 19 c shows a peptide ELISA, immunisation with C-FGFPAHVFIDWLQSLN (p4474-KLH/Alum) (SEQ ID NO. 230), titre to injected mimotope.
  • FIG. 19 d shows an anti-protein ELISA. Mice were injected 3 times with 30 μg of the indicated mimotopes coupled to KLH with Alum as adjuvant. Sera from each group (comprising 5 mice) were pooled, diluted 1:100 and tested on ELISA plates coated with purified rabbit CETP.
  • SEQ ID NO. 245
    FAFPAHVFIDWLQSLS
    SEQ ID NO. 246
    FGFPAHVFIDWLQALS
    SEQ ID NO. 247
    FGFPAHVFIDWLQSLA
    SEQ ID NO. 248
    GFPAHVFIDWLQSLS
    SEQ ID NO. 249
    FPAHVFIDWLQSLS
    SEQ ID NO. 250
    PAHVFIDWLQSLS
    SEQ ID NO. 251
    FAFPAHVFIDWLQALA
  • FIG. 19 e shows an anti-protein ELISA, wherein mice were injected 3 times with 30 μg of the indicated mimotopes coupled to KLH with Alum as adjuvant. Mouse sera (from single mice) were diluted 1:100 and tested on ELISA plates coated with purified rabbit CETP.
  • SEQ ID NO. 252
    FGFPEHLFVDFLQSLS
    SEQ ID NO. 253
    FGFPAHVHIDWLQSLS
    SEQ ID NO. 254
    FGFPAHVPIDWLQSLS
    SEQ ID NO. 269
    FGFPAHVWIDWLQSL
    SEQ ID NO. 255
    FGFPSHLFIDWAQSLS
    SEQ ID NO. 268
    FPGFPAHVFIDWLQLIT
    • EXAMPLES
  • There exists a strong inverse relationship between the plasma concentration of cholesterol in high density lipoproteins (HDLs) and the development of coronary heart disease (CHD). Thus, the risk for CHD is higher when HDLs decrease. Although 33% of patients with CHD have low plasma levels of HDLs, there is currently no effective therapy for increasing the plasma concentration of HDLs. Diet and moderate exercise are ineffective, statins only achieve a low 5 to 7% increase in HDL, and niacin has side efects and compliance profiles limiting its use.
  • The inhibition of CETP activity has been suggested as therapeutic approach to increase plasma HDL levels. CETP is a plasma glycoprotein that facilitates transfer of neutral lipids and phospholipids between lipoproteins and regulates the concentration of plasma HDL. The inhibition of CETP activity is expected to increase plasma HDL concentrations for several reasons. CETP lowers HDL concentrations by moving cholesteryl esters from HDLs to VLDLs and LDLs. Transient inhibition of CETP in rabbits and hamsters by monoclonal antibodies, small molecules (Sikorski, J. A., J. Med. Chem. 49 (1) (2006): 1-22), or antisense oligonucleotides causes HDL increase. Sustained CETP inhibition with antisense nucleotides increased plasma HDL and reduced atherosclerotic lesions in a rabbit model of atherosclerosis. CETP-transgenic mice and rats show decreased plasma HDL. Humans with reduced CETP activity have elevated plasma HDL.
  • Recently, a vaccine approach has been proposed. Rabbits were immunized with a human CETP-derived peptide containing a region of CETP critical for neutral lipid transfer function. Vaccinated rabbits had reduced CETP activity and an altered lipoprotein profile with lower LDL and higher HDL concentration. Furthermore, CETP-vaccinated rabbits were shown to have smaller atherosclerotic lesions than control animals.
  • The problem of the anti-CETP vaccine approach discussed above is that the vaccine formulation comprises a self peptide and therefore must break natural tolerance against self antigens. The invention describes a CETP mimotope that can be used for vaccination: The mimotope shall induce the production of antibodies against CETP. The CETP mimotope does not have a self sequence and therefore does not need to break tolerance. Thus, the induction of an anti-CETP antibody response is greatly facilitated. The mimotope is identified with a monoclonal antibody (mAb) and (commercially available) peptide libraries. An anti-CETP monoclonal antibody is used that neutralizes CETP activity. This mAb detects a sequence within the C-terminal 26 amino acids of CETP necessary for neutral lipid transfer activity.
    • Example 1 Generation of Monoclonal Antibodies to be Used for Screening of Phage Display Libraries
  • A.) 2 Antibodies Derived from “Fusion F”:
  • Balb/c mouse were immunized with original CETP epitope C-FGFPEHLLVDFLQSLS (SEQ ID NO. 147) (16 C-terminal amino acids of CETP protein) coupled to KLH and Alum as adjuvant.
  • 2 hybridoma clones (both IgG1) were purified and used for screening: F5AF9G4 (“Paula”) and F6F11D1 (“Felix”).
  • These 2 monoclonal antibodies recognize the injected epitope as well as CETP protein in ELISA. They can also be used in Western Blot to detect CETP protein (recombinant protein expressed in bacteria as well as protein isolated from rabbit serum). Both antibodies do not inhibit CETP enzyme activity (tested with Roar CETP Activity Assay Kit, see e.g. U.S. Pat. No. 5,585,235; U.S. Pat. No. 5,618,683; U.S. Pat. No. 5,770,355).
  • B.) 2 Antibodies Derived from “Fusion I”:
  • Balb/c mouse were immunized with original CETP epitope C-FGFPEHLLVDFLQSLS (SEQ ID NO. 147) (16 C-terminal amino acids of CETP protein) coupled to KLH and Alum as adjuvant.
  • 2 hybridoma clones (both IgG1) were purified and used for screening: 12G6H5 (“Frida”) and 12G6H7 (“James”).
  • These 2 monoclonal antibodies recognize the injected epitope as well as CETP protein in ELISA. They can also be used in Western Blot to detect CETP protein (recombinant protein expressed in bacteria as well as protein isolated from rabbit serum). In contrast to the antibodies derived from “Fusion F” (see A.)) both antibodies “Frida” and “James” inhibit CETP enzyme activity (tested with Roar CETP Activity Assay Kit).
    • Example 2 Phage Display, In Vitro Inhibition ELISA and In Vivo Testing of Mimotopes
  • Phage Display libraries used in this example were:
  • Ph.D. 7: New England BioLabs E8102L (linear 7mer library)
  • Ph.D. C7C: New England BioLabs E8121L (7mer library, cyclized peptides)
  • Ph.D. 12: New England BioLabs E8111L (linear 12mer library)
  • Phage Display was done according to manufacturer's protocol (www.neb.com).
  • After 2 or 3 subsequent rounds of panning, single phage clones were picked and phage supernatants were subjected to ELISA on plates coated with the antibody that was used for the panning procedure. Phage clones that were positive in this ELISA (strong signal for the target, but no signal for unspecific control) were sequenced. From DNA sequences, peptide sequences were deduced. These peptides were synthesized and characterised in inhibition ELISA.
  • 1. In Vitro Inhibition Assay (ELISA)
  • Different amounts of peptides (2 and 20 μg, as indicated in the respective figures) derived from Phage Display were incubated with the monoclonal antibody that was used for the screening procedure. Peptides diminishing subsequent binding of the antibody to the original CETP epitope (C-terminal 16 amino acids of CETP protein) coated on ELISA plates were considered as inhibiting. (Results see i.a. FIGS. 19 a to 19 c)
  • 2. In Vivo Testing of Mimotopes
  • Inhibiting as well as some non-inhibiting peptides were coupled to KLH and injected into mice (wildtype or CETP-transgenic mice; subcutaneously into the flank or intra-dermaly into the ears) or rabbits (subcutaneously into the flank) together with an appropriate adjuvant (aluminium hydroxide and Gerbu 100 for mice and aluminium hydroxide or CFA/IFA for rabbits).
  • Titers to injected peptides as well as to the original CETP epitope were determined. In addition, for selected sera also immune response to CETP protein was measured (Results see FIGS. 7 a to 7 d and FIGS. 19 a to 19 e).
  • 3. Results
  • 3.1. Screening with 2 Antibodies Derived from “Fusion F”: “Paula” and “Felix”
  • 3.1.1. Phage Display Library Ph.D. 7
  • 3.1.1.1. Screening with Monoclonal Antibody “Paula”
  • 17 Sequences were identified in this screen:
  • (SEQ ID NO. 2)
    P2_8 SYHATFL
    (SEQ ID NO. 3)
    P2_9 TMAFPLN 
    (SEQ ID NO. 4)
    P2_11 HYHGAFL
    (SEQ ID NO. 5)
    P2_12 EHHDIFL
    (SEQ ID NO. 44)
    P2_15 SSLELFL
    (SEQ ID NO. 6)
    P2_16 TGLSVFL
    (SEQ ID NO. 7)
    P3_2 WMPSLFY
    (SEQ ID NO. 8)
    P3_6, 14, 28 SMPWWFF
    (SEQ ID NO. 9)
    P3_9 TMPLLFW
    (SEQ ID NO. 10)
    P3_13 DTWPGLE
    (SEQ ID NO. 11)
    P3_16 SMPPIFY
    (SEQ ID NO. 12)
    P3_17 MPLWWWD
    (SEQ ID NO. 13)
    P3_18 SMPNLFY
    (SEQ ID NO. 14)
    P3_19 RMPPIFY
    (SEQ ID NO. 15)
    P3_21 NPFEVFL
    (SEQ ID NO. 16)
    P3_25 TLPNWFW
    (SEQ ID NO. 17)
    P3_26 SMPLTFY
  • The result of a representative competition ELISA is shown in FIG. 1.
  • 3.1.1.2. Screening with Monoclonal Antibody “Felix”
  • 6 sequences were identified that inhibit binding of monoclonal antibody “Felix” in in vitro competition experiments:
  • F2-9 C SFLDTLT (SEQ ID NO. 45)
    F3-6 C NFLKTLS (SEQ ID NO. 46)
    F3-18 C DFLRTLT (SEQ ID NO. 47)
    F3-23 C AFLDTLV (SEQ ID NO. 48)
    F3-34 C TFLSSLA (SEQ ID NO. 49)
    F3-38 C GFLDSLM (SEQ ID NO. 50)
  • Additional 12 sequences were identified that do not inhibit binding of monoclonal antibody “Felix” in in vitro competition experiments:
  • F2-2 + 5 SPHPHFL (SEQ ID NO. 51)
    F2-6 NFMSIGL (SEQ ID NO. 19)
    F2-16/F3-30 SQFLASL (SEQ ID NO. 20)
    F2-29 SNFLKTL (SEQ ID NO. 52)
    F3-1-_ TGFLATL (SEQ ID NO. 53)
    F3-11-_ WSWPGLN (SEQ ID NO. 21)
    F3-17- IAWPGLD (SEQ ID NO. 22)
    F3-32- SKFMDTL (SEQ ID NO. 23)
    F3-41- SDFLRAL (SEQ ID NO. 54)
    F3-44-_ SMPMVFY (SEQ ID NO. 24)
    F3-49- YEWVGLM (SEQ ID NO. 25)
    F3-64- KGFLDHL (SEQ ID NO. 26
  • All mimotopes inhibiting the binding of monoclonal antibody “Felix” in vitro were coupled to KLH and injected subcutaneously (into the flank; s.c.) or intradermally (i.d.) into wild-type mice (mice do not have CETP protein), CETP-tg mice, or rabbits, respectively, and induced immune response to the injected peptide with all adjuvants that were tested (Alum and CFA (Complete Freund's adjuvant); Gerbu).
  • For all in vitro inhibiting mimotopes listed above, antibodies reacting to the original CETP epitope could be detected in mice and in rabbits.
  • For 5 out of 6 mimotopes (see below and Table 1) antibodies reacting with purified human CETP and recombinantly expressed human CETP could be detected in ELISAs from rabbit sera:
  • F2-9 C SFLDTLT (SEQ ID NO. 45)
    F3-6 C NFLKTLS (SEQ ID NO. 46)
    F3-18 C DFLRTLT (SEQ ID NO. 47)
    F3-34 C TFLSSLA (SEQ ID NO. 49)
    F3-38 C GFLDSLM (SEQ ID NO. 50)
  • Subcutaneous injections in the flank were performed in week 1, week 3 and week 7 with 30 μg peptide-KLH per mouse. Intradermal injections in the ear were performed in week 1, week 3 and week 6 with 10 μg peptide-KLH per mouse. Sera were taken 2 weeks after the 3rd injection. Vaccine formulation with Alum (always 1 mg per mouse): up to 250 μl, injected into one flank. The Alum formulation with 1 ml per mouse (500 μl into each flank) was in 1×PBS as buffer.
  • Vaccine formulation with Gerbu Adjuvant 100 (Gerbu Cat. Nr. #3100; always 50 μl adjuvant per mouse): 200 μl, 100 μl injected into each flank comprising 1×HEPES as buffer.
  • TABLE 1
    Results of the titer determination
    P4073
    injected (FGFPEH- p irrel-
    Adjuvant KLH mimotope LLVDFLOSLS) evant
    Alum s.c. (30 KLH 1:20.000 n.a. 1:400 no titer
    μg peptide)
    p4073-KLH C- 1:70.000 n.a. 1:20.000 no titer
    FGFPEHLLVD-
    FLQSLS (SEQ
    ID NO. 147)
    p4223-KLH F2-9; C- 1:15.000 1:15.000 1:6.400 no titer
    SFLDTLT (SEQ
    ID NO. 45)
    p4181-KLH F3-6 C- 1:8.000 1:6.400 1:800 no titer
    NFLKTLS (SEQ
    ID NO. 46)
    p4184-KLH F3-18 C- 1:5.000 1:10.000 1:3.000 1:2.500
    DFLRTLT (SEQ
    ID NO. 47)
    p4187 F3-34 C- 1:3.200 1:9.000 1:4.000 no titer
    TFLSSLA (SEQ
    ID NO. 49)
    p4188-KLH F3-38 C- 1:10.000 1:9.000 1.5.000 no titer
    GFLDSLM (SEQ
    ID NO. 50)
    p4227-KLH P12-19; C- 1:12.800 1:10.000 1:5.000 no titer
    SANPRDFLETLF
    (SEQ ID NO.
    55)
    p4228-KLH P12-21; C- 1:10.000 1:4.000 1:1.000 1:400
    RMFPESFLDTLW
    (SEQ ID NO.
    56)
    KLH/Gerbu s.c. KLH 1:70.000 n.a. 1:6.000 1:800
    (30 μg pep-
    tide)
    p4073-KLH C- 1:25.000 n.a. 1:15.000 1:200
    FGFPEHLLVD-
    FLQSLS (SEQ
    ID NO. 147)
    p4223-KLH F2-9; C- 1:40.000 1:25.000 1:50.000 1:1.000
    SFLDTLT (SEQ
    ID NO. 45)
    p4181-KLH F3-6 C- 1:20.000 1.20.000 1:8.000 1:400
    NFLKTLS (SEQ
    ID NO. 46)
    p4184-KLH F3-18 C- 1:27.000 1.35.000 1:15.000 1:6.000
    DFLRTLT (SEQ
    ID NO. 47)
    p4187-KLH F3-34 C- 1.20.000 1.20.000 1:15.000 no titer
    TFLSSLA (SEQ
    ID NO. 49)
    p4188-KLH F3-38 C- 1:40.000 1:35.000 1:35.000 1:400
    GFLDSLM (SEQ
    ID NO. 50)
    p4227-KLH P12-19; C- 1.20.000 1:30.000 1.3.000 1:400
    SANPRDFLETLF
    (SEQ ID NO.
    55)
    p4228-KLH P12-21; C- 1:27.000 1:8.000 1:5.000 no titer
    RMFPESFLDTLW
    (SEQ ID NO.
    56)
    p4073-KLH C- 1:10.000 1:10.000 no titer
    FGFPEHLLVD-
    FLQSLS (SEQ
    ID NO. 147)
    KLH/Alum i.d. KLH 1:12.800 n.a. no titer no titer
    (10 μg pep-
    tide)
    p4073-KLH C- 1:10.000 n.a. 1:3.200 no titer
    FGFPEHLLVD-
    FLQSLS (SEQ
    ID NO. 147)
    p4223-KLH F2-9; C- 1:6.400 1:3.200
    SFLDTLT (SEQ
    ID NO. 45)
    p4181-KLH F3-6 C- 1:10.000 1:1.500 1:600 no titer
    NFLKTLS (SEQ
    ID NO. 46)
    p4184-KLH F3-18 C- 1:15.000 1:5.000 1:1.500 no titer
    DFLRTLT (SEQ
    ID NO. 47)
    p4187-KLH F3-34 C- 1:50.000 1:6.400 1:3.200 1:500
    TFLSSLA (SEQ
    ID NO. 49)
    p4188-KLH F3-38 C- 1:12.000 1:5.000 1:2.000 no titer
    GFLDSLM (SEQ
    ID NO. 50)
    p4227-KLH P12-19; C- 1:6.400 1:6.400 no titer no titer
    SANPRDFLETLF
    (SEQ ID NO.
    55)
    p4228-KLH P12-21; C- 1:20.000 1:2.000 1:1.600 no titer
    RMFPESFLDTLW
    (SEQ ID NO.
    56)
    p4298-KLH Fr12/3/84ext2; 1:25.000 1:3.200 1:1.600 no titer
    C-
    FGFPAHVSID-
    WLQSLS (SEQ
    ID NO. 184)
  • 3.1.2. Phage Display Library Ph.D. 12
  • 3.1.2.1. Screening with Monoclonal Antibody “Paula”
  • Out of 20 amino acid sequences derived from this screen, 3 were inhibiting in in vitro inhibition experiments:
  • P12-19 SANPRDFLETLF (SEQ ID NO. 55)
    P12-21 RMFPESFLDTLW (SEQ ID NO. 56)
    P12-37 TIYDSFLDSLAS (SEQ ID NO. 57)
  • Not inhibiting peptides were:
  • P12-5/44/46/49 HQSDDKMPWWFF (SEQ ID NO. 27)
    P12-9 KPYLLKDFLEAL (SEQ ID NO. 58)
    P12-24/43-_ AMGPYDALDLFL (SEQ ID NO. 59)
    P12-25 TWNPIESFLESL (SEQ ID NO. 60)
    P12-28 + 42 YVWQDPSFTTFF (SEQ ID NO. 28)
    P12-30 QYQTPLTFLEAL (SEQ ID NO. 61)
    P12-35- RHISPATFLEAL (SEQ ID NO. 62)
    P12-39- HTDSFLSTFYGD (SEQ ID NO. 63)
    P12-42- YVWQDPSFTTFF (SEQ ID NO. 29)
    P12-45- ADSTFTSFLQTL (SEQ ID NO. 64)
    P12-50-_ GPVSIYADTDFL (SEQ ID NO. 65)
    P12-51-_ DSNDTLTLAAFL (SEQ ID NO. 66)
    P12-52-_ NGSPALSHMLFL (SEQ ID NO. 33)
    P12-53- TDYDPMWVFFGY (SEQ ID NO. 34)
    P12-56- IFPLDSQWQTFW (SEQ ID NO. 35)
    P12-58- NESMPDLFYQPS (SEQ ID NO. 36)
    P12-61- DWGDKYFSSFWN (SEQ ID NO. 37)
  • Results of 2 typical competition ELISAs are shown in FIGS. 2A and 2 b.
  • All 3 mimotopes were coupled to KLH and injected into wildtype mice (mice do not have CETP protein), CETP-tg mice, or rabbits, respectively, and induced immune response to the injected peptide with all adjuvants that were tested (Alum and CFA; Gerbu).
  • Mimotope P12-19; C-SANPRDFLETLF (SEQ ID NO. 55) and P12-21; C-RMFPESFLDTLW (SEQ ID NO. 56) induced an immune response to the original CETP epitope in wt mice and in rabbits.
  • In contrast thereto, mimotope P12-37 C-TIYDSFLDSLAS (SEQ ID NO. 57) did not induce an antibody response to the original epitope.
  • 3.2 Screening with 2 Antibodies Derived from “Fusion I”: “Frida” and “James”
  • 3.2.1. Phage Display Library pH.D. 7
  • 3.2.1.1. Screening with Monoclonal Antibodies “Frida” and “James”
  • Two different peptide sequences were identified in these screens, 11 of 12 clones that were sequenced had identical sequences. These peptides are not inhibiting in in vitro competition experiments.
  • Fr7-2-2
    Fr7-2B-65
    Fr7-3-7
    Fr7-3-13
    Fr7-3-26
    Fr7-3-32
    Ja7-2-22
    Ja7-3-28
    Ja7-3-41
    Ja7-3-52
    Ja7-3-56 VSAYNNV (SEQ ID NO. 38)
    Ja7-3-89 WPLHLWQ (SEQ ID NO. 39)
  • The results of 2 representative competition ELISAs with mAb “Frida” are shown in FIGS. 3A and 3 b. The same pattern was seen with mAb “James”.
  • 3.2.2. Phage Display Library pH.D. 12
  • 3.2.2.1. Screening with Monoclonal Antibody “Frida”
  • Fr12/2/6 TPTHYYADFSQL (SEQ ID NO. 67)
    Fr12/2/11 LPGHLIWDSLHY (SEQ ID NO. 68)
    Fr12/2/27 LPQTHPLHLLED (SEQ ID NO. 69)
    Fr12/3/1
    Fr12/3/19
    Fr12/3/88 IPYHHLVDQLHH (SEQ ID NO. 70)
    Fr12/3/26
    Fr12/3/65 YPYHVQVDVLQN (SEQ ID NO. 71)
    Fr12/3/68 IPSHHLQDSLQL (SEQ ID NO. 72)
    Fr12/3/12 EYAHHTSLDLRQ (SEQ ID NO. 73)
    Fr12/3/83 EPLHFRSDRIQA (SEQ ID NO. 74)
    Fr12/3/55 ATPSHLIIDRAQ (SEQ ID NO. 75)
    Fr12/3/63 APKHLYADMSQA (SEQ ID NO. 76)
    Fr12/3/84 FKPAHVSIDWLQ (SEQ ID NO. 77)
    Fr12/3/47 MPAHLSRDLRQS (SEQ ID NO. 78)
    Fr12/3/80 NPKHYSIDRHQA (SEQ ID NO. 79)
    Fr12/3/40 SPQHLTTDRAQA (SEQ ID NO. 80)
    Fr12/3/35 TPFHFAQDSWQW (SEQ ID NO. 81)
  • None of the 15 amino acid sequences identified in this screen were inhibiting in in vitro competition experiments. However, sequence analysis revealed rather high homology to the original protein sequence for many of the mimotopes. On the other hand, for some peptides binding of monoclonal antibody “Frida” to ELISA plates coated with mimotope-BSA could be shown (see FIGS. 4 a and 4 b).
  • This shows that binding of monoclonal antibody to immobilised mimotopes does not necessarily allow to predict inhibition in in vitro competition ELISA.
  • In vitro inhibition experiments with variations of the original sequence FGFPEHLLVDFLQSLS (SEQ ID NO. 147) (16 C-terminal AA of CETP protein) showed that removing more than 2 amino acids from the N-terminus or more than 1 amino acid from the C-terminus abolishes inhibition (for monoclonal antibodies “Frida” and “James”. “Paula” and “Felix” recognise a different part of the original sequence).
  • In addition, simultaneously removing 2 amino acids from the N-terminus and 1 amino acid from the C-terminus also results in a peptide that is not inhibiting in vitro any more.
  • (SEQ ID NO. 147)
    C-FGFPEHLLVDFLQSLS
    “original” sequence (peptide derived
    from CETP)/inhibiting in vitro
    C-GFPEHLLVDFLQSLS sequence N-1/
    inhibiting in vitro
    C-FPEHLLVDFLQSLS sequence N-2/
    inhibiting in vitro
    C-PEHLLVDFLQSLS sequence N-3/
    evtl. slightly inhibiting in vitro
    C-FGFPEHLLVDFLQSL sequence C-1/
    inhibiting in vitro
    C-FGFPEHLLVDFLQS sequence C-2/
    not inhibiting in vitro
    C-FPEHLLVDFLQSL sequence N-2 and
    C-1/not inhibiting in vitro!
    “original” FGFPEHLLVDFLQSLS
    Fr12/2/6 TPTHYYADFSQL (SEQ ID NO. 67)
    Fr12/2/11 LPGHLIWDSLHY (SEQ ID NO. 68)
    Fr12/2/27 LPQTHPLHLLED (SEQ ID NO. 69)
    Fr12/3/1 IPYHHLVDQLHH (SEQ ID NO. 70)
    Fr12/3/19 IPYHHLVDQLHH (SEQ ID NO. 70)
    Fr12/3/88 IPYHHLVDQLHH (SEQ ID NO. 70)
    Fr12/3/26 YPYHVQVDVLQN (SEQ ID NO. 71)
    Fr12/3/65 YPYHVQVDVLQN (SEQ ID NO. 71)
    Fr12/3/68 IPSHHLQDSLQL (SEQ ID NO. 72)
    Fr12/3/12 EYAHHTSLDLRQ (SEQ ID NO. 73)
    Fr12/3/83 EPLHFRSDRIQA (SEQ ID NO. 74)
    Fr12/3/55 ATPSHLIIDRAQ (SEQ ID NO. 75)
    Fr12/3/63 APKHLYADMSQA (SEQ ID NO. 76)
    Fr12/3/84 FKPAHVSIDWLQ (SEQ ID NO. 77)
    Fr12/3/47 MPAHLSRDLRQS (SEQ ID NO. 78)
    Fr12/3/80 NPKHYSIDRHQA (SEQ ID NO. 79)
    Fr12/3/40 SPQHLTTDRAQA (SEQ ID NO. 80)
    Fr12/3/35 TPFHFAQDSWQW (SEQ ID NO. 81)
  • Consequently, using the original CETP sequence as a template, peptide sequences obtained in this Phage Display procedure were elongated on the N-terminus and/or C-terminus to check whether in vitro inhibition is possible with longer peptides.
  • 3.2.2.2. Mimotopes Frida pH.D.12 and Variations Thereof:
  • Fr12/2/6 TPTHYYADFSQL (SEQ ID NO. 67)
    Fr12/2/6 ext1 TPTHYYADFSQLLS (SEQ ID NO. 82)
    Fr12/2/6 ext2 TPTHYYADFSQSLS (SEQ ID NO. 83)
    Fr12/2/6 ext3 GTPTHYYADFSQLL (SEQ ID NO. 84)
    Fr12/2/6 ext4 GTPTHYYADFSQSL (SEQ ID NO. 85)
    Fr12/2/6 ext5 FGTPTHYYADFSQSLS (SEQ ID NO. 86)
    Fr12/2/6 ext6 FGFPTHYYADFSQSLS (SEQ ID NO. 87)
    Fr12/2/11 LPGHLIWDSLHY (SEQ ID NO. 68)
    Fr12/2/11 ext1 LPGHLIWDSLHYL (SEQ ID NO. 89)
    Fr12/2/11 ext2 LPGHLIWDSLHYLS (SEQ ID NO. 90)
    Fr12/2/11 ext3 LPGHLIWDSLHSL (SEQ ID NO. 91)
    Fr12/2/11 ext4 LPGHLIWDSLHSLS (SEQ ID NO. 92)
    Fr12/2/11 ext5 GLPGHLIWDSLHYL (SEQ ID NO. 93)
    Fr12/2/11 ext5 GLPGHLIWDSLHSL (SEQ ID NO. 94)
    Fr12/2/11 ext6 FGLPGHLIWDSLHSLS (SEQ ID NO. 95)
    Fr12/2/11 ext7 FGFPGHLIWDSLHSLS (SEQ ID NO. 96)
    Fr12/2/27 LPQTHPLHLLED (SEQ ID NO. 69)
    Fr12/3/1/19/88  IPYHHLVDQLHLS (SEQ ID NO. 99)
    ext1
    Fr12/3/1/19/88  IPYHHLVDQLHSLS (SEQ ID NO. 100)
    ext2
    Fr12/3/1/19/88  FGIPYHHLVDQLHHLS (SEQ ID NO. 101)
    ext3
    Fr12/3/1/19/88  FGFPYHHLVDQLHSLS (SEQ ID NO. 102)
    ext4
    Fr12/3/26/65ext1 YPYHVQVDVLQNLS (SEQ ID NO. 104)
    Fr12/3/26/65ext2 YPYHVQVDVLQSLS (SEQ ID NO. 105)
    Fr12/3/26/65ext3 FGYPYHVQVDVLQNLS (SEQ ID NO. 106)
    Fr12/3/26/65ext4 FGFPYHVQVDVLQSLS (SEQ ID NO. 107)
    Fr12/3/68 ext1 IPSHHLQDSLQLLS (SEQ ID NO. 109)
    Fr12/3/68 ext2 IPSHHLQDSLQSLS (SEQ ID NO. 110)
    Fr12/3/68 ext3 GIPSHHLQDSLQLL (SEQ ID NO. 111)
    Fr12/3/68 ext4 FGIPSHHLQDSLQLLS (SEQ ID NO. 112)
    Fr12/3/68 ext5 FGFPSHHLQDSLQSLS (SEQ ID NO. 113)
    Fr12/3/83 ext1 EPLHFRSDRIQALS (SEQ ID NO. 116)
    Fr12/3/83 ext2 EPLHFRSDRIQSLS  (SEQ ID NO. 117)
    Fr12/3/83 ext3 GEPLHFRSDRIQAL (SEQ ID NO. 118)
    Fr12/3/83 ext4 FGEPLHFRSDRIQALS (SEQ ID NO. 119)
    Fr12/3/83 ext5 FGFPLHFRSDRIQSLS (SEQ ID NO. 120)
    Fr12/3/55 ext1 ATPSHLIIDRAQSLS (SEQ ID NO. 176)
    Fr12/3/55 ext2 FGFPSHLIIDRAQSLS (SEQ ID NO. 177)
    Fr12/3/55 ext2  FGFPSHLIIDWAQSLS (SEQ ID NO. 178)
    R->W
    Fr12/3/55 ext2  FGFPSHLIIDWLQSLS (SEQ ID NO. 179)
    RA->WL
    Fr12/3/63 ext1 APKHLYADMSQALS (SEQ ID NO. 122)
    Fr12/3/63 ext2 APKHLYADMSQSLS (SEQ ID NO. 123)
    Fr12/3/63 ext3 GAPKHLYADMSQAL (SEQ ID NO. 124)
    Fr12/3/63 ext4 FGFPKHLYADMSQSLS (SEQ ID NO. 125)
    Fr12/3/84 ext1 FKPAHVSIDWLQSLS (SEQ ID NO. 183)
    Fr12/3/84 ext2 FGFPAHVSIDWLQSLS (SEQ ID NO. 184)
    Fr12/3/47 ext1 MPAHLSRDLRQSL (SEQ ID NO. 127)
    Fr12/3/47 ext2 MPAHLSRDLRQSLS (SEQ ID NO. 128)
    Fr12/3/47 ext3 GMPAHLSRDLRQSL (SEQ ID NO. 129)
    Fr12/3/47 ext4 FGFPAHLSRDLRQSLS (SEQ ID NO. 130)
    Fr12/3/40 ext1 SPQHLTTDRAQALS (SEQ ID NO. 168)
    Fr12/3/40 ext2 SPQHLTTDRAQSLS (SEQ ID NO. 169)
    Fr12/3/40 ext3 GSPQHLTTDRAQAL (SEQ ID NO. 170)
    Fr12/3/40 ext4 FGFPQHLTTDRAQSLS (SEQ ID NO. 171)
    Fr12/3/35 ext1 TPFHFAQDSWQWLS (SEQ ID NO. 133)
    Fr12/3/35 ext2 TPFHFAQDSWQSLS (SEQ ID NO. 134)
    Fr12/3/35 ext3 GTPFHFAQDSWQWL (SEQ ID NO. 135)
    Fr12/3/35 ext4 FGFPFHFAQDSWQSLS (SEQ ID NO. 136)
  • Representative examples of inhibition ELISA are shown in FIGS. 5A and 5 b. The elongated peptides Fr12/3/84 ext2 and Fr12/3/55 ext3 showed a significant inhibition:
  • C-FGFPSHLIIDRAQSLS Fr12/3/55 ext3 (SEQ ID NO. 177)
    C-FGFPAHVSIDWLQSLS Fr12/3/84 ext2 (SEQ ID NO. 184)
  • Three additional peptides were also inhibiting in this assay:
  • C-FGFPYHVQVDVLQSLS Fr12/3/26/65ext4 (SEQ ID NO. 107)
    C-FKPAHVSIDWLQSLS Fr12/3/84 ext1 (SEQ ID NO. 183)
    C-FGFPQHLTTDRAQSLS Fr12/3/40 ext4 (SEQ ID NO. 171)
  • After sequence analysis comparing the original epitope and all mimotopes derived from Phage Display screens additional 2 peptides were created.
  • For mimotope Fr12/3/55 ext3 C-FGFPSHLIIDRAQSLS (SEQ ID NO. 177) (inhibiting in ELISA, see above) amino acid exchanges were tested in inhibition ELISA:
  • Strongly inhibiting:
    C-FGFPAHVSIDWLQSLS (SEQ ID NO. 184)
    Fr12/3/84 ext2
    Slightly inhibiting:
    C-FGFPSHLIIDRAQSLS (SEQ ID NO. 177)
    Fr12/3/55 ext3
    Peptides with altered 
    sequences
    (inhibiting, see FIG. 6):
    C-FGFPSHLIIDWAQSLS (SEQ ID NO. 178)
    Fr12/3/55 ext2 W instead of R
    C-FGFPSHLIIDWLQSLS (SEQ ID NO. 179)
    Fr12/3/55 ext2 WL instead 
    of RA

    Further preferred mimotopes have been characterised by the following example-set-up:
  • Exp. Nr. C42-1 KLH/Alum
    CETP-42
    C42-2 p4073-KLH/ C-FGFPEHLLVDFLQSLS
    Alum (SEQ ID NO. 147
    C42-3 p4073 LLV->LFV p4468-KLH/ C-FGFPEHLFVDFLQSLS
    Alum (SEQ ID NO. 252)
    C42-4 Fr12/3/84 ext2 VSI->VFI P4361-KLH/ C-FGFPAHVFIDWLQSLS
    Alum (SEQ ID NO. 222)
    C42-5 Fr12/3/84 ext2 VSI->VHI p4469- C-FGFPAHVHIDWLQSLS
    KLH/Alum (SEQ ID NO. 253)
    C42-6 Fr12/3/84 ext2 VSI->VPI p4470- C-FGFPAHVPIDWLQSLS
    KLH/Alum (SEQ ID NO. 254)
    C42-7 Fr12/3/84 ext2 VSI->VWI p4471- C-FGFPAHVWIDWLQSLS
    KLH/Alum (SEQ ID NO. 229)
    C42-8 Fr12/3/55 ext2 R->W LII->LFI p4472- C-FGFPSHLFIDWAQSLS
    KLH/Alum (SEQ ID NO. 255)
    C42-9 Fr12/3/84 ext2 VSöVFI FGF- p4473- C-PGFPAHVFIDWLQLIT
    >PGF SLS->LIT KLH/Alum (SEQ ID NO. 256)
    C42-10 Fr12/3/84 ext2 VSI->VYI P4362-KLH/ C-FGFPAHVYIDWLQSLS
    Alum (SEQ ID NO. 223)
    Exp. Nr. C45-1 KLH/Alum
    CETP-45
    C45-2 p1358-KLH/ neg. control peptide
    Alum
    C45-3 p4073-KLH/ C-FGFPEHLLVDFLQSLS
    Alum (SEQ ID NO. 147)
    C45-4 Fr12/3/84 ext2 VSI->VFI SLS- p4474-KLH/ C-FGFPAHVFIDWLQSLN
    >SLN Alum (SEQ ID NO. 230)
    C45-5 Fr12/3/84 ext2 VSI->FSI p4475-KLH/ C-FGFPAHFSIDWLQSLS
    Alum (SEQ ID NO. 231)
    C45-6 Fr12/3/84 ext2 VSI->VSF p4476-KLH/ C-FGFPAHVSFDWLQSLS
    Alum (SEQ ID NO. 232)
    C45-7 Fr12/3/84 ext2 VSI->VFI PAH- p4477-KLH/ C-FGFPEHVFIDWLQSLS
    >PEH Alum (SEQ ID NO. 233)
    C45-8 Fr12/3/1/19/88 ext4 p4284-KLH/ C-FGFPYHHLVDQLHSLS
    Alum (SEQ ID NO. 102)
    C45-9 Fr12/3/84 ext1 VSI->VFI plus  p4479-KLH/ C-GFKPAHVFIDWLQSLS
    G on N-terminus Alum (SEQ ID NO. 270)
    C45-10 Fr12/3/84 ext2 VSI->VFI plus  p4480-KLH/ C-DFGFPAHVFIDWLQSLS
    D on N-terminus; =4361 plus D Alum (SEQ ID NO. 234)
    C45-11 Fr12/3/40 ext4 RA->WL LTT->LFT p4481-KLH/ C-FGFPQHLFTDWLQSLS
    =p4369 with exchange TöF Alum (SEQ ID NO. 237)
    C45-12 Fr12/3/55 ext2 RA->WL (see C- p4325-KLH/ C-FGFPSHLIIDWLQSLS
    31 and C-33; sera inhibiting Alum (SEQ ID NO. 179)
    activity)
    C45-13 Fr12/3/84 ext2 FGF->FYF (see p4343-KLH/ C-FYFPAHVSIDWLQSLS
    C-33: recogn. protein/not in- Alum (SEQ ID NO. 204)
    hibiting activity)
    C45-14 rabbit sequence p4125-KLH/ C-FGFPKHLLVDFLQSLS
    Alum (SEQ ID NO. 238)
  • 3.2.2.3. In Vivo Testing of Mimotopes
  • Female Balb/c mice, five mice per group, were subcutaneously immunized with 30 μg peptide coupled to KLH. Control groups were administered KLH or C-FGFPEHLLVDFLQSLS (SEQ ID NO. 147). As adjuvant alum was used. The peptides administered were all able to bind to “Frida” and to induce an immune response for CETP, although some of these peptides did not inhibit the binding of CETP to “Frida” in vitro (in an in vitro inhibition assay). The in vitro ELISA assay to determine the antibody titer was performed with pooled sera after two vaccinations in a two week interval (S2; see FIGS. 7 a to 7 d). The wells of the ELISA plate were coated with KLH (positive control), mimotope-BSA conjugate, C-FGFPEHLLVDFLQSLS (SEQ ID NO. 147) and a irrelevant peptide-BSA conjugate (negative control). The detection was performed with anti-mouse IgG.
  • 3.2.3. Phage Display Library pH.D. 7C7
  • 3.2.3.1. Screening with Monoclonal Antibodies “Frida” and “James”
  • Fr2-1 ACSFAYLYRC (SEQ ID NO. 137)
    Fr2-5
    Fr2-6
    Fr2-18
    Fr2-19
    Fr2-28
    Ja2-5
    Ja2-20
    Ja2-23
    Ja2-24
    Ja2-30 ACFMGDKWVC (SEQ ID NO. 138)
    Fr2-7
    Fr2-9 ACVLYPKAIC (SEQ ID NO. 139)
    Fr2-11
    Ja2-19 ACYMGQQFVC (SEQ ID NO. 140)
    Fr2-16 ACLTAYLHWC (SEQ ID NO. 141)
    Fr2-20 ACTLFPVAYC (SEQ ID NO. 142)
    Fr2-25 ACWLFPYAHC (SEQ ID NO. 143)
    Fr2-26 ACKSINMWLC (SEQ ID NO. 144)
    Fr2-27 ACQTINRWLC (SEQ ID NO. 145)
  • Due to their cyclic nature of these mimotope-peptides their synthesis is more complicated than the synthesis of linear peptides. Seven out of 9 cyclic sequences were chosen for in vitro analysis in inhibition ELISA (see FIGS. 8 a and 8 b). None of these sequences inhibited binding of the monoclonal antibody that was used for Phage Display Screening to the original CETP epitope. In addition, when these peptides were coupled to BSA and coated onto ELISA plate they were not detected by the monoclonal antibody (see FIG. 9). This was in contrast to data with mimotopes derived from the Ph.D.7 or Ph.D.12 libraries, where the monoclonal antibodies bound to most of the identified mimotopes when these peptides were coupled to BSA and coated onto ELISA plates.
    • Example 3 CETP Activity Assay
  • The CETP activity assay was performed with assays commercially available (e.g. ROAR CETP Activity Assay) and described, for instance, in the U.S. Pat. No. 5,585,235, U.S. Pat. No. 5,618,683 and U.S. Pat. No. 5,770,355. The assay is performed according to the manufacturers' recommendations.

Claims (3)

1. Peptide consisting of at least one amino acid sequence selected from the group consisting of SYHATFL, TMAFPLN, HYHGAFL, EHHDIFL, SSLELFL, TGLSVFL, WMPSLFY, SMPWWFF, TMPLLFW, DTWPGLE, SMPPIFY, MPLWWWD, SMPNLFY, RMPPIFY, NPFEVFL, TLPNWFW, SMPLTFY, SFLDTLT, NFLKTLS, DFLRTLT, AFLDTLV, TFLSSLA, GFLDSLM, SPHPHFL, NFMSIGL, SQFLASL, SNFLKTL, TGFLATL, WSWPGLN, IAWPGLD, SKFMDTL, SDFLRAL, SMPMVFY, YEWVGLM, KGFLDHL, SANPRDFLETLF, RMFPESFLDTLW, TIYDSFLDSLAS, HQSDDKMPWWFF, KPYLLKDFLEAL, AMGPYDALDLFL, TWNPIESFLESL, YVWQDPSFTTFF, QYQTPLTFLEAL, RHISPATFLEAL, HTDSFLSTFYGD, YVWQDPSFTTFF, ADSTFTSFLQTL, GPVSIYADTDFL, DSNDTLTLAAFL, NGSPALSHMLFL, TDYDPMWVFFGY, IFPLDSQWQTFW, NESMPDLFYQPS, DWGDKYFSSFWN, VSAYNNV, WPLHLWQ, TPTHYYADFSQL, LPGHLIWDSLHY, LPQTHPLHLLED, IPYHHLVDQLHH, YPYHVQVDVLQN, IPSHHLQDSLQL, EYAHHTSLDLRQ, EPLHFRSDRIQA, ATPSHLIIDRAQ, APKHLYADMSQA, FKPAHVSIDWLQ, MPAHLSRDLRQS, NPKHYSIDRHQA, SPQHLTTDRAQA, TPFHFAQDSWQW, TPTHYYADFSQLLS, TPTHYYADFSQSLS, GTPTHYYADFSQLL, GTPTHYYADFSQSL, FGTPTHYYADFSQSLS, FGFPTHYYADFSQSLS, LPGHLIWDSLHY, LPGHLIWDSLHYL, LPGHLIWDSLHYLS, LPGHLIWDSLHSL, LPGHLIWDSLHSLS, GLPGHLIWDSLHYL, GLPGHLIWDSLHSL, FGLPGHLIWDSLHSLS, FGFPGHLIWDSLHSLS, LPQTHPLHLLED, IPYHHLVDQLHH, IPYHHLVDQLHLS, IPYHHLVDQLHSLS, FGIPYHHLVDQLHHLS, FGFPYHHLVDQLHSLS, YPYHVQVDVLQN, YPYHVQVDVLQNLS, YPYHVQVDVLQSLS, FGYPYHVQVDVLQNLS, FGFPYHVQVDVLQSLS, IPSHHLQDSLQL, IPSHHLQDSLQLLS, IPSHHLQDSLQSLS, GIPSHHLQDSLQLL, FGIPSHHLQDSLQLLS, FGFPSHHLQDSLQSLS, EYAHHTSLDLRQ, EPLHFRSDRIQA, EPLHFRSDRIQALS, EPLHFRSDRIQSLS, GEPLHFRSDRIQAL, FGEPLHFRSDRIQALS, FGFPLHFRSDRIQSLS, APKHLYADMSQA, APKHLYADMSQALS, APKHLYADMSQSLS, GAPKHLYADMSQAL, FGFPKHLYADMSQSLS, MPAHLSRDLRQS, MPAHLSRDLRQSL, MPAHLSRDLRQSLS, GMPAHLSRDLRQSL, FGFPAHLSRDLRQSLS, NPKHYSIDRHQA, TPFHFAQDSWQW, TPFHFAQDSWQWLS, TPFHFAQDSWQSLS, GTPFHFAQDSWQWL, FGFPFHFAQDSWQSLS, ACSFAYLYRC, ACFMGDKWVC, ACVLYPKAIC, ACYMGQQFVC, ACLTAYLHWC, ACTLFPVAYC, ACWLFPYAHC, ACKSINMWLC, ACQTINRWLC, FGFPEHLLVDFLQSLS, FGFPEHLLVDFLQSLS, FPEHLLVDFLQSL, AGFPEHLLVDFLQSLS, FAFPEHLLVDFLQSLS, FGAPEHLLVDFLQSLS, FGFAEHLLVDFLQSLS, FGFPAHLLVDFLQSLS, FGFPEALLVDFLQSLS, FGFPEHALVDFLQSLS, FGFPEHLAVDFLQSLS, FGFPEHLLADFLQSLS, FGFPEHLLVAFLQSLS, FGFPEHLLVDALQSLS, FGFPEHLLVDFAQSLS, FGFPEHLLVDFLASLS, FGFPEHLLVDFLQALS, FGFPEHLLVDFLQSAS, FGFPEHLLVDFLQSLA, FAFPAHLLVDFLQALA, AAFPAHLLADFLQALA, SPQHLTTDRAQA, SPQHLTTDRAQALS, SPQHLTTDRAQALS, GSPQHLTTDRAQAL, FGFPQHLTTDRAQSLS, FGFPQHLTTDWAQSLS, FGFPQHLTTDRLQSLS, FGFPQHLTTDWLQSLS, ATPSHLIIDRAQ, ATPSHLIIDRAQSLS, FGFPSHLIIDRAQSLS, FGFPSHLIIDWAQSLS, FGFPSHLIIDWLQSLS, FGFPSHLIIDWSQSLS, FATPSHLIIDWLQSLS, FKPAHVSIDWLQ, FKPAHVSIDWLQSLS, FGFPAHVSIDWLQSLS, AGFPAHVSIDWLQSLS, FAFPAHVSIDWLQSLS, FGAPAHVSIDWLQSLS, FGFAAHVSIDWLQSLS, FGFPAHVSADWLQSLS, FGFPAHVSIDWLQALS, FGFPAHVSIDWLQSLA, FAFPAHVSIDWLQALA, FGFAAHVSIDWLQSLS, FGFFAHVSIDWLQSLS, FGFPAHVSIRWLQSLS, FGFPAHVSIEWLQSLS, FGFPAHVSIDWLNSLS, FGFPAHVSIDWLHSLS, AGFPAHVSIDWLQSLS, PGFPAHVSIDWLQSLS, WGFPAHVSIDWLQSLS, FAFPAHVSIDWLQSLS, FGFPAHVSIDWLQSLS, FYFPAHVSIDWLQSLS, FDFPAHVSIDWLQSLS, FGAPAHVSIDWLQSLS, FGFPAHVSIDWLQLLS, FGFPAHVSIDWLQWLS, FGFPAHVSIDWLQNLS, FGFPAHVSIDWLQTLS, FGFPAHVSIDWLQYLS, FGFPAHVSIDWLQSIS, FGFPAHVSIDWLQSLT, FGFPAHVSIDWLQSLY, FAFPAHVSIDWLQALA, FGFPAHVSIDRAQSLS, FGFPTHVSIDWLQSLS, FGFPFHVSIDWLQSLS, FGFPAHISIDWLQSLS, FGFPAHIIIDWLQSLS, FGFPAHLTTDWLQSLS, FGFPAHVFIDWLQSLS, FGFPAHVYIDWLQSLS, FGFPAHVSLDWLQSLS, FGFPAHVSADWLQSLS, TPTHYYADFSQSLS, FGFPAHVSIDWSQSLS, FGFPAHVSIDFSQSLS, FGFPSHIIIDWLQSLS, FGFPSHLIIEWLQSLS, AAFPAHLLADAAQALA, AAFPAHAAADFLQALA, AAFAAHLLADFLQAAA, AAAPAHLLVDAAQAAA, FAFPAHVFIDWLQSLS; FGFPAHVFIDWLQALS, FGFPAHVFIDWLQSLA, GFPAHVFIDWLQSLS, FPAHVFIDWLQSLS, PAHVFIDWLQSLS, FAFPAHVFIDWLQALA, FGFPEHLFVDFLQSLS, FGFPAHVHIDWLQSLS, FGFPAHVPIDWLQSLS, FGFPSHLFIDWAQSLS, PGFPAHVFIDWLQLIT, PAHVYIDWLQSLS, FGFPAHVYIDWLQ, FGFPAHVFIDWLQ, DFGFPSHLIIDWLQSLS, DFGFPAHVFIDWLQSLN, PSHLIIDWLQ, PAHVFIDWLQ, DFGFPAHVTIDWLQSLN, DFGFPAHVLIDWLQSLN, FGFPAHVYIDWLQSLS, FGFPAHVFIDWLQSLN and FGFPAHVFIDWLQSLA.
2. Pharmaceutical formulation comprising at least one peptide according to claim 1.
3. Formulation according to claim 2, characterised in that the peptide is coupled to a pharmaceutically acceptable carrier, preferably KLH (Keyhole Limpet Hemocyanin).
US14/086,159 2007-08-10 2013-11-21 Treatment of atherosclerosis with cholesterol ester transport protein mimotopes Abandoned US20140179900A1 (en)

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Date Code Title Description
STCB Information on status: application discontinuation

Free format text: ABANDONED -- FAILURE TO RESPOND TO AN OFFICE ACTION