DE102004035606A1 - Carrier for drugs for obtaining oral bioavailability - Google Patents

Abstract

The present invention relates to a protein complex comprising at least one hemagglutinin, at least one of the Clostridium botulinum types A, B, C, D, E, F or G and a polypeptide-Hc conjugate, wherein the polypeptide-Hc conjugate from a selected polypeptide linked to the heavy chain or its N-terminal fragment of botulinum toxin.

Description

The The present invention relates to a protein complex consisting of at least one hemagglutinin from at least one of the Clostridium botulinum types A, B, C, D, E, F or G and a polypeptide-Hc conjugate, wherein the polypeptide-Hc conjugate from a selected one Polypeptide linked to the heavy chain or its N-terminal fragment of botulinum toxin.

A Variety of pharmaceutical agents is indeed highly active, you but therapeutic use is significantly affected by that these substances are not oral but only parenterally - ie per Injection - administered can be. In particular, the oral administration of protein drugs fails because of these substances over the oral route can not get to their site of action. The proteins follow oral administration to two difficult to overcome hurdles: the denaturing conditions in the gastrointestinal tract lead to Inactivation of the protein ensures a variety of proteases for the Degradation of polypeptides and even if a protein is resistant to these conditions is, a high molecular substance can not to overcome the barrier of the intestinal mucosa, to enter the blood and to get to the site of action. Proteins are in the stomach or in the small intestine cleaved by proteases and the cleavage products, amino acids and Peptides, resorbed or excreted. Protein drugs are thus orally administered ineffective.

numerous Efforts have been made to eliminate this disadvantage and to make protein drugs orally bioavailable. Some approaches are briefly mentioned here: Attempts have been made by mixtures of protease inhibitors the Protect drug from proteolytic degradation. So were at the same time with protein drug protease inhibitors such as aprotinin, bestatin, Puromycin, soybean trypsin inhibitor, should be administered with it the degradation prevented and the protein active ingredient without being absorbed absorbable be.

It was also tried by formulations the local pH in the stomach / intestine to modulate. Also on the protein drug itself has one is set to by chemical modification of amino acids their stability to increase degradation and absorbability. The latter wanted to go through increase lipophilicity (eg, by palmitoylation). As an an example Here is the coupling of insulin with an amphiphilic oligomer called (hexyl insulin monoconjugate Fa. NOBEX Corporation). Another approach is to increase the permeability of the mucosa, eg. B. by the administration of chelators or surface-active substances such as Sodium lauryl sulfate, sodium deoxycholate. Also part of this concept the concurrent administration of concentrated low molecular weight Carrier molecules (e.g. B. 4- (4-2-hydroxybenzoyl) aminophenyl) butyric acid). Another approach tries to exploit specific transport mechanisms in the intestinal wall. So Is available for the absorption of vitamin B12 is a transport mechanism responsible for protein agents should be used by the active ingredients coupled to vitamin B12 become. All these different approaches have not yet led to an approved protein drug that is orally bioavailable.

One Another approach to providing orally bioavailable proteins is described in WO 03/101484. According to the description of the C-terminal residue of the botulinum toxin heavy chain with a Polypeptide connected. The C-terminal residue could transport through the accomplish epithelial membranes. For oral administration of the Hybrid protein can do this with the botulinum toxin naturally surrounding auxiliary proteins.

Further WO 02/05844 describes the provision of orally bioavailable proteins and low molecular weight drugs that are in a complex of at least a hemagglutinin and possibly non-toxic, non-hemagglutinating protein (NTNH) the botulinum toxin complexes of Clostridium botulinum are incorporated. The incorporation of polypeptides with a molecular weight of <50 However, kDa proved for a profitable marketing as not effective enough.

Therefore The present invention is based on the object, a means to provide orally bioavailable with the polypeptides can be.

The The object is achieved by the subject matter defined in the claims solved.

The the following illustrations explain the Invention.

1 shows in a diagram the result of a glucose tolerance test on rats. 4 animals were treated with 2 U insulin-Hc conjugate and 4 animals with 2 U insulin-Hc conjugate incorporated into the complex (insulin complex) by oral (gavage), after 60 min the animals were treated with 2 g / kg glucose loaded. 3 additional groups were treated with 0.1 U, 0.6 U, 2 U insulin ip and were also given 2 g / kg glucose at the same time. The glucose level was determined at intervals of about 30 minutes.

2 shows in a graph the result of comparing the effect of insulin-Hc conjugate, insulin-Hc conjugate integrated into the complex (insulin complex) and ip-administered insulin. The experimental conditions are identical to those in 1 , Shown is the area under the curve of glucose concentrations (AUC).

Of the As used herein, the term "protein complex" refers to a vehicle with the other one selected Polypeptides are transported into the blood system of humans and animals can be. The protein complex consists of at least one hemagglutinin and possibly non-toxic, non-hemagglutinating protein (NTNH) the botulinum toxin complex of at least one of Clostridium botulinum Types A, B, C, D, E, F or G. The hemagglutinins and the NTNH provide the proteins found in clostridia that are naturally occurring form the botulinum toxin complex with botulinum toxin. The clarity however, it should be noted that the protein complex is not a botulinum toxin contains.

Of the As used herein, the term "botulinum toxin complex" means naturally occurring protein aggregate type A, B, C, D, E, F or G from Clostridium botulinum comprising botulinum toxin, hemagglutinins and non-toxic, non-hemagglutinating Protein (NTNH).

Of the As used herein, "polypeptide" or "selected polypeptide" means a peptide at least 2 amino acids. The polypeptide may be linear, circular or branched. Further For example, the polypeptide may consist of more than one amino acid chain, the Chains e.g. above a disulfide bond may be linked together. The Polypeptides can further modified amino acids and the usual post-translational modifications such as glycosylation. The polypeptides may be pharmacologically or immunologically active polypeptides or polypeptides used for diagnostic purposes e.g. antibody be.

Of the As used herein, "carrier" or "carrier" means the entire heavy chain (Hc) or an N-terminal fragment of the heavy chain of Botulinum toxin selected from botulinum toxin complexes of types A, B, C, D, E, F or G.

Of the As used herein, "polypeptide-Hc conjugate", "Hc conjugate" or "conjugate" refers to one Carrier covalently linked to a selected polypeptide is. For example, Insulin-Hc conjugate is a molecule consisting from insulin linked to the heavy chain or its N-terminal Fragment of botulinum toxin.

Of the As used herein, "neocomplex" refers to a Complex of protein complex in which a Hc conjugate is integrated.

The Clostridium botulinum bacterium has an efficient mechanism designed to be a protein over to channel the oral route into an organism where this protein is then absorbed by its target cells. With this protein it is the most toxic substance known so far: Clostridium botulinum toxin, subsequently also botulinum toxin called. Naturally lies Botulinum toxin in a botulinum toxin complex with a number of others of Clostridium botulinum expressed proteins. Will the botulinum toxin complex administered orally, the high molecular nerve drug botulinum toxin absorbed in the intestine and then reaches the target cell, the motor neuron at the motor end plate. At its site of action prevents the neurotoxin the payout of acetylcholine and leads thus paralysis of the respective muscle.

Clostridium botulinum is divided into 7 serogroups, due to their toxins be distinguished: type A, B, C, D, E, F, G. When the toxins act these are proteins with a molecular weight of about 150,000 Dalton (Da). The botulinum toxin complex is usually contaminated with food absorbed, enterally absorbed and reaches its site of action, the motor end plate.

The Botulinum toxin consists of two subunits. The two subunits have a different function: the heavy chain (molecular weight 100 kDa) binds to the nerve cell in a highly specific manner and later enables the Translocation of the light chain into the cytoplasm of the cell. The heavy one Chain (Hc) is in native botulinum toxin via a disulfide bridge with linked to the light chain (Lc) is. The light chain serves as a protease that cuts proteins (SNARE proteins), the for the fusion of secretory vesicles with the nerve cell membrane are responsible. The secretory vesicles can thus do not dispense acetylcholine: the activation of the muscle is blocked.

The both chains arise from the originally synthesized polypeptide by proteolytic cleavage. For some types of clostridium, the Cleavage already by clostridia-own proteases (type A, C, partial B) while in other types, the cleavage only in the digestive tract (trypsin) or Tissue of the recipient expires. The heavy chain in insulated form and without contamination of lighter Chain or total toxin is completely Noxious, it alone is able to release the secretion of nerve cells Do not block acetylcholine.

The clostridia synthesize a number of other proteins that interact with the botulinum toxin Complex (botulinum toxin complex), which is stable in an acidic environment and protects the neurotoxin from denaturation and proteolytic degradation and also allows uptake by the intestinal mucosa.

at the other proteins, called in the following complex proteins are a series of hemagglutinins and a non-toxic, non-haemagglutinating Protein (NTNH), which has a molecular weight of about 120,000 Da. The other proteins form the protein complex. In the botulinum toxin complex of type A were the following hemagglutinins described: Ha2 with about 16,900 Da, Ha3a with about 21,000 Da, Ha3b with about 52,000 Da and Ha1 with about 35,000 Da.

The Botulinum toxin complexes of types B to G are similar Scheme constructed. An example is the botulinum toxin complex of type B. Besides the NTNH here are HA-70 with a molecular weight of about 70,000 Da, Ha-17 with a molecular weight of about 17,000 Da and Ha-33 are described with a molecular weight of about 33,000 Da (Bhandari, M. et al., (1997) Current Microbiology 35, pp. 207-214).

Further described East, A.K. et al. ((1994) System Appl. Microbiol. 17 306-312) compared the sequence of Ha-33 of type B with the sequence of Type A and C. For the type C and type D are in addition to the Ha 33 (= Ha1) also - analog Type A - a Ha3b with a molecular weight of about 33,000 Da also the Ha3b with about 53,000 Da and Ha3a with about 22-24,000 Da and Ha2 with about 17,000 Da (see Inoue, K. et al. (1999) Microbiology 145, pp. 2533-2542).

Surprisingly The inventors found out in reconstitution experiments that only the botulinum toxin heavy chain, so without the light chain Chain, alone or coupled to a polypeptide, quantitatively in the protein complex is incorporated.

The Polypeptide can chemically bind to the heavy chain of a botulinum toxin coupled and so in a protein complex consisting of at least integrated into a complex protein. To couple the protein to the heavy chain a variety of chemical methods are available. It There is a wide range of bifunctional reagents that one shortcut of two different proteins. Preference is given to reagents used a disulfide bridge with a cysteine of the tying partner knot. In the next step, then the Binding with the carrier, the heavy chain, done. Suitable for such Coupling are, for example, reagents such as SPDP (N-succinimidyl 3- [2-pyridyldithio] propionate) or DTDP (4,4'-dithiodipyridine), in which only a disulfide bridge without a spacer between linked to the proteins becomes. This link has the advantage of being in vivo under reducing conditions e.g. in the cytoplasm over the thioredoxin system can be cleaved. The coupling will be there chosen so that the incorporation of the heavy chain into the protein complex is not impaired and the biological activity the polypeptide is retained. Alternatively, the connection the heavy chain with the polypeptide can be achieved by Both peptides as a recombinant fusion protein in a suitable Expression system can be synthesized.

The polypeptides associated with the carrier are preferably pharmacological or immunologically active polypeptides obtained by means of the protein complex according to the invention be administered orally, which may be therapeutically or preventively effective can. The selected ones Polypeptides can e.g. Hormones, cytokines, enzymes, growth factors, antigens, antibodies, inhibitors, Receptor agonists or antagonists or coagulation factors. It does not matter whether the polypeptides are recombinantly produced or from their natural sources were isolated. Preferred polypeptides are insulin, erythropoietin, Interferons, interleukins, HIV protease inhibitors, GM-CSF (granulocyte / macrophage-stimulating factor), NGF (Nerve Growth Factor), PDGF (Platelet derived growth factor), FGF (fibroblast growth factor), plasminogen activators, e.g. TPA (tissue plasminogen activator), renin inhibitors, human Growth factor, IGF (insulinlike growth factor), vaccines like e.g. Tetanus vaccine, hepatitis B vaccine, diphtheria vaccine, antibodies e.g. Herceptin (Antibody against Her2), antibodies against TNF (tumor necrosis factor), antibodies against EGF receptor, antibodies against VEGF, antibodies against IgE, antibodies against CD11a, calcitonin, urokinase, streptokinase, angiogenesis inhibitors, factor VIII, Factor Xa antagonists, metalloproteinase inhibitors.

The polypeptides used for diagnostic purposes may be, for example, antibodies or ligands, which polypeptides may be labeled. As a marker is any mark in question, which can be detected in the body of the human or animal. Preferred labels are isotopes, for example C ¹³ , or radioactive labels. The labeled antibodies can be used for the detection of tumors, the labeled ligands for the detection of eg pathological receptors.

The carrier linked to the polypeptide is incorporated into the protein complex. The protein complex is composed of at least one hemagglutinin and, if desired, at least one NT NH. The hemagglutinins and the NTNH are selected from the naturally occurring botulinum toxin complexes of types A, B, C, D, E, F or G of Clostridium botulinum. However, the protein complex can also contain other than its natural composition, eg it can only be composed of hemagglutinin without the NTNH proteins. Further, the protein complex may be composed of less hemagglutinin species than the naturally occurring botulinum toxin complex, preferably of three different types of hemagglutinins, preferably two, more preferably one hemagglutinin type, which protein complex may or may not each contain the NTNH protein. The protein complex may also be composed of a mixture of one or more types of hemagglutinin and / or NTNH proteins of the various serotypes.

Prefers are protein complexes that are naturally occurring protein complexes (without Botulinum toxin) from Clostridium botulinum types A, B, C, D, E, F or G correspond, for example a protein complex with Ha1, Ha2, Ha3a, Ha3b and NTNH of Clostridium botulinum type B. The protein complex can also be composed of Ha1, Ha2, Ha3a and NTNH, from Ha1, Ha2, Na3b and NTNH, as well as Ha1 and Ha3a, Ha3b and NTNH, further from Ha2, Ha3a, Ha3b and NTNH, from Ha1, Ha2 and NTNH, from Ha1, Ha3a and NTNH, from Ha1, Ha3b and NTNH, from Ha2, Ha3a and NTNH, from Ha2, Ha3b and NTNH from Ha3a, Ha3b and NTNH or from any other Combinations of listed Complex proteins. The protein complex can also be composed from one of the hemagglutinins and NTNH, as well The protein complex may be composed of the listed combinations hemagglutinins without NTNH. According to the exemplary protein complexes of the type B are further preferred protein complexes from the hemagglutinins and / or NTNH types A, C, D, E, F or G.

One Another aspect of the present invention is the provision a method for producing the protein complex according to the invention, comprising the following steps: a) separate isolation of at least a botulinum toxin complex of the type A, B, C, D, E, F or G from Clostridium botulinum at a pH in the range of about 2.0 to about 6.5, b) Increase of the pH to a value in the range of about 7.0 to about 10.0, c) Separating the respective botulinum toxin from the complex proteins by means of chromatographic methods, d) mixing the in step c) complex proteins obtained with a selected polypeptide-Hc conjugate, or e) separating the complex proteins obtained in step c) and mixing at least one complex protein with a polypeptide-Hc conjugate, f) dialyzing the mixture from step d) or e) against a Buffer at a pH in the range of about 6.5 to about 2.0, preferably in the range of about 4.0 to about 6.0, more preferably at 6.0.

The Complex proteins can from the natural Botulinum toxin complexes are isolated. An exemplary process for isolation is the following: First, the botulinum toxin complex of clostridia at acidic pH, preferably at a value in the range of about 2.0 to about 6.5, more preferably in the range of about 4.0 to about 6.5, especially preferably at pH 6.0 isolated. After increasing the pH to a value in the range of about 7.0 to about 10.0, preferably to a pH in the range of about 7.0 to about 8.0 becomes Botulinum toxin over common in protein chemistry separated chromatographic process. This method is feasible since the complex at a pH <6.5 is stable, decays at neutral or at alkaline pH and the toxin is released. The toxin-free complex proteins can then be added with a polypeptide-Hc conjugate and the pH by dialysis against a buffer customary in protein chemistry, especially preferred a phosphate, acetate or citrate buffer to a pH in Range from about 2.0 to about 6.5, preferably in the range of about 4.0 to about 6.0, particularly preferably reduced to pH 6.0. In the process, a protein complex is formed which contains the polypeptide-Hc conjugate contains and so the oral bioavailability of the selected Polypeptide ensures.

Other common in protein chemistry chromatographic methods, concentration methods and precipitations can for the Isolation of complex proteins can also be used.

Due to their known DNA sequences, the complex proteins can also be produced recombinantly by means of recombinant DNA techniques in special host organisms. The complex proteins thus produced may also have modifications, ie they may be derivatives of complex proteins. Modifications here mean not only deletions, additions, insertions or substitutions but also also chemical modifications of amino acids, eg methylations, or acetylations, as well as post-translational modifications, eg glycosylations or phosphorylations. The expression of desired proteins in different hosts is well known to those of ordinary skill in the art and need not be described separately here. In this case, the complex proteins required for the protein complex can be expressed separately or simultaneously in a host organism. Preference is given to the production of the recombinant complex proteins in bacteria, for example in E. coli, Bacillus subtilis or Clostridium difficile, or in eukaryotic cells, eg in CHO cells, in insect cells, eg using the baculovirus system, or in yeast cells. The complex proteins can be isolated and spiked with the selected polypeptide conjugate according to the procedure described above. Furthermore, the selected polypeptide HC conjugate may be expressed as a fusion protein together with the complex proteins in the host organism simultaneously. Particularly preferred is the simultaneous or separate production of the respective complex proteins together with the selected polypeptide-Hc conjugate via a YAC in yeast.

The Protein complexes according to the invention can furthermore from a mixture of recombinantly produced and from natural Botulinum toxin complexes composed of isolated complex proteins be.

The explain the following examples the invention and are not to be construed as limiting.

Example 1: Isolation the heavy chain of Clostridium botulinum toxin type A.

Clostridium botulinum toxin type A (strain ATCC 3502) was published after Process with the modifications listed below cultivated (see. The Gupta & Sathyamoorthy, 1984, Toxicon 22, pp. 415 - 424). After 72 hours of growth, the toxin was precipitated by adding 3N sulfuric acid. To Extraction of the precipitate and separation of nucleic acids the toxin was precipitated by ammonium sulfate. After solubilization and Dialysis was carried out by DEAE-Sepharose chromatography (2.6 × 15 cm). at pH 6.0. The bound toxin was eluted with 150 mM NaCl, against Dialyzed 50 mM Tris / HCl and another ion exchange chromatography on a Sepharose Q-pillar (2.6 × 10.0 cm). The neurotoxin was incubated with a NaCl gradient (0-300 mM NaCl) eluted. The neurotoxin-containing fractions were pooled and dialysed against 10 mM NaPhosphate pH 7.0. The dialysate was on a Sepharose S-pillar (1.6 x 11 cm) and eluted with your NaCl gradient (0-300 mM NaCl). Chromatography yielded the high purity neurotoxin.

The Isolation of the heavy chain from the neurotoxin was analogous the published literature with the following amendments (cf. Kozaki et al., 1981, J. Med. Sci Biol. 34, pp. 61-68). This was the high purity Neurotoxin type A dialyzed against borate / phosphate buffer pH 8.5 and on a pillar (1 × 5 cm) filled bound with QAE-Sephadex. After washing with the borate / phosphate buffer, the additional 10 mM DTE, the column became overnight incubated with 3 mL borate / phosphate buffer containing 150 mM DTE and 2 M urea contained. After the subsequent elution of the light chain with the borate / phosphate buffer + 10mM DTE + 2N urea became the heavy Chain eluted with the same buffer and 200 mM NaCl. to Separation of residues from incompletely separated active neurotoxin The pooled fractions were pumped four times over an affinity column. The Affinity column was filled with Sepharose, to which an antibody coupled to the light chain of Clostridium botulinum toxin type A. was. After this chromatography, a heavy chain was available which contained no contaminants from light chain or native toxin. Even in high concentrations the activity test (mouse diaphragmatic assay) showed no activity.

Example 2: Preparation the complex proteins of Clostridium botulinum type B

The Complex proteins of Clostridium botulinum type B are obtained after fermentation of Clostridium botulinum type B (strain okra) according to published method isolated (see Evans et al., 1986, European Journal of Bioch. 409-416), with some steps modified: as in example 1 were after extraction of the acid precipitated biomass the nucleic acids from the extract like and the toxic botulinum toxin complex from the supernatant with ammonium sulfate precipitated. The precipitate was dissolved in 0.05 M sodium citrate + 1 mM EDTA pH 5.5 taken up and after dialysis over a DEAE Sephadex chromatography, the high molecular weight Complex on the pillar (5 x 12 cm) was not bound and passed quantitatively through the column. The complex-containing eluate was after dialysis against 50 mM Tris / HCl, 1 mM EDTA pH 7.9 a Sepharose Q-pillar chromatographed, with the complex proteins not on the column were tied during the neurotoxin on the column remained bound and eluted first with a salt gradient. Further purification of the complex proteins took place on a Q Hyper D-pillar (2.6 x 13 cm) equilibrated with the same buffer (50 mM Tris / HCl, 1 mM EDTA) was. The toxin-free protein complex was treated with a sodium chloride gradient (0 - 300 mM NaCl) eluted.

Latest Traces of neurotoxin were removed by affinity chromatography. This was the complex solution four times over a column pumped that as an affinity matrix one with an antibody (IgG fraction) against botulinum neurotoxin type B coupled Sepharose contained. In the activity test (mouse hemodiaphragm analysis) was then no biological activity (Toxicity) more detectable.

Example 3: Integration the heavy chain of botulinum toxin type A into a protein complex of C. botulinum type B

100 μg (34 μl) of the highly purified Complex proteins of type B from example 2 were mixed with 200 μg (690 μl) of the isolated ones heavy chain of type A from example 1. The mixture was 3 days at 2-8 ° C dialyzed against 1 L of 50 mM NaPhosphate buffer pH 6.0 with 150 mM NaCl. Subsequently were 450 μL by adding 150 μl 4 M ammonium sulphate precipitated. Under these conditions of precipitation remains the heavy chain not incorporated into the protein complex in solution during Protein complex (with or without incorporated heavy chain) quantitatively fails. To re-incubation over At night, the pellet was spun down and placed in 120 μL NaPhosphate, mm NaCl, 2mM EDTA pH 6.0 resuspended. The formation of the protein complex was tested by "gel filtration" on a BioSep-S-3000. The Chromatogram showed only a single peak (at a molecular weight of about 500,000 daltons). SDS polyacrylamide gel electrophoresis revealed that the peak fractions contained both the complex proteins of type B as well as the botulinum toxin heavy chain type A.

Example 4: Coupling of Insulin to the heavy chain of botulinum toxin type A synthesis of SPDP insulin

12.5 mg insulin (Roche, recombinant) was added to 6.3 mL buffer (10 mM sodium carbonate pH = 6.9). These were used to block α-amino groups 3 μL citaconic anhydride (Fluka) pipetted and the mixture incubated at room temperature, wherein the pH was followed. By addition of 1 M NaOH was the pH at 6.8 - 7.0 held. The reaction mixture was then heated at 4 ° C overnight against 50 mM sodium phosphate, dialyzed 100 mM sodium chloride pH = 7.3.

6.2 mg SPDP (N-succinimidyl 3- [2-pyridyldithio] propionate, Pierce) in 500 μL DMF solved. 274 μL of this solution were added to 6.3 mL of insulin derivative (adjusted to pH 8.3) and the mixture 1 ½ h incubated at room temperature on a blender. Still available SPDP was dialyzed against 50 mM sodium phosphate, 100 mM NaCl pH = 7.3 removed. To remove the protecting groups was added water dialyzed (2 h at room temperature) and then against 10 mM HCl for 5½ h at room temperature. After all was over Night against 50 mM sodium phosphate, 100 mM sodium chloride, 4 mM EDTA pH = 7.3 dialyzed (final volume of the SPDP solution: 7 mL).

Preparation of insulin-Hc conjugate

25 mg of the botulinum toxin heavy chain type A corresponding to Example 1 was isolated, were added to 8 mg of insulin SPDP (Final volume: 41.5 mg) and incubated for 4 days at 4 ° C (end-over-end mixer). To separate uncoupled insulin SPDP was compared to 50 dialysed mM Tris / HCl, 250 mM NaCl, 1 mM EDTA, the dialysis tubing had an exclusion limit of 50 kD.

The Product was analyzed in the Western blot. With antibodies against Insulin became a protein with molecular weight of ~ 100 kD identified. So it was the heavy chain conjugate and insulin (= insulin-Hc conjugate). At 3T3 cells was in vitro the activity of insulin.

Example 5: Installation of the Insulin-Hc conjugates into the protein complex from Clostridium botulinum Type B

In 52 mL were 7.4 mg insulin-Hc conjugate (from Example 4) with 21 mg protein complex (purified according to Example 2) and against 50 mM sodium phosphate, 250 mM NaCl, 1 mM EDTA pH 6.0 for 4 days Dialyzed at 4 ° C. A sample of 500 μL was in a gel filtration over a BioSep S-3000 column (Phenomenex) analyzed. It showed only a high molecular weight peak at one Molecular weight of ~ 600 kD. A sample of the peak fraction was analyzed in the Western blot. With antibodies to insulin, that insulin (as insulin-Hc conjugate) into the protein complex (out Complex proteins of C. botulinum) was integrated.

Example 6: Testing a Insulin neocomplex in rats in the glucose tolerance test

The Effectiveness of an insulin-Hc conjugate incorporated into a protein complex (hereinafter referred to as insulin neo complex) after oral Administration was tested in animals in rats.

Groups of 4 rats were treated with either insulin neo-complex or with free insulin-Hc conjugate (without complex proteins). As control served untreated animals. The dose of insulin was the same in both groups and was 2 U / animal. The solutions were administered by gavage. As further controls, 0.1 U, 0.6 U and 2.0 U insulin were administered ip. One hour after administration of insulin neocomplex and free insulin-Hc conjugate, the animals were challenged with glucose (2 g / kg per oral). At this time also the injection of the positive control (0.1 U, 0.6 U and 2.0 units insulin) took place. After 30, 60, 120 and 180 minutes, blood was taken and the glucose level was determined. After 60 min, the control animals achieved a maximum glucose concentration of approximately 140 mg / mL, whereas in the insulin-neocomplex treated animals the concentration only slightly increased (s. 1 ). Considering the course of the glucose concentration (area under the curve, AUC), the effect of the insulin neocomplex is comparable to ip administered insulin ( 2 ).

The Glucose concentration in animals using only insulin-Hc conjugate treated as well as in the case of control: the Concentration increased strongly until the time of 60 minutes. It can be conclude, that an insulin-Hc conjugate alone has no effect on insulin levels has, the administration of insulin-Hc conjugate without incorporation in The protein complex is thus not suitable for making insulin orally bioavailable do.

Example 7: Comparison the integration of insulin-Hc conjugate bound with insulin the C-terminus of heavy chain of botulinum toxin

The c-terminal fragment of the heavy chain (M _r ≈50 kD) of botulinum toxin type A was recombinantly expressed in E. coli. For this purpose, the DNA sequence for the c-terminal fragment of botulinum toxin type A As 871-1296 (NIINT... ERPL) linked to a His tag was cloned into the vector pBN29 4772 in order to allow E. coli N15 [pREP4 ] (Quiagen) and the expressed fragment purified on a Ni-NTA Sepharose column by affinity chromatography.

100 μg of the toxin-free complex proteins of C. botulinum type B were mixed with 200 μg (340 μL) of the recombinant c-terminal fragment and dialysed for 3 days at 2-8 ° C. against 50 mM Na phosphate pH 6.0 with 150 mM NaCl. It was then made up to 450 μL with H ₂ O and precipitated by the addition of 150 μl of 4 M ammonium sulphate. Under these precipitation conditions, the c-terminal fragment which is not incorporated into the protein complex remains in solution, while the protein complex (with or without incorporated c-terminal fragment) precipitates quantitatively. After re-incubation overnight, the pellet was spun down and resuspended in 150 μL 50 mM NaPhosphate, 150 mM NaCl, 2 mM EDTA pH 6.0. 100μL were separated on a Biosep S-3000 gel filtration column into the complex and possibly as a contaminant, unbound c-terminal fragment. Two peaks were eluted: the first peak (12.2 min) represents the protein complex. A very small peak represents the free c-terminal fragment fragment. The first peak was examined in the SDS-PAGE, only the complex proteins were present, so the c-terminal fragment was not integrated into the complex but remained in the ammonium sulfate precipitate unbound in solution. The c-terminal fragment of botulinutoxin can therefore not be integrated into the complex.

Claims (12)

A protein complex consisting of at least one hemagglutinin from at least one of the Clostridium botulinum types A, B, C, D, E, F or G and a polypeptide-Hc conjugate, wherein the polypeptide-Hc conjugate from a selected one Polypeptide linked to the heavy chain or its N-terminal Fragment of botulinum toxin. The protein complex of claim 1, wherein the hemagglutinins a mixture of hemagglutinins at least one of the Clostridium botulinum types A, B, C, D, E, F or G are. Protein complex according to any one of the preceding claims Claims, wherein the protein complex in addition non-toxic, non-hemagglutinating Contains protein. Protein complex according to any one of the preceding claims Claims, the heavy chain being from one of the botulinum toxin complexes of the Types A, B, C, D, E, F or G is isolated. Protein complex according to any one of the preceding claims Claims, wherein the heavy chain is produced recombinantly in a suitable expression system is. Protein complex according to any one of the preceding claims Claims, wherein the polypeptide is a hormone, cytokine, growth factor, antigen, Antibody, Inhibitor, receptor agonist or - antagonist or Coagulation factor is. Protein complex according to any one of the preceding claims Claims, wherein the selected polypeptide and the heavy chain or its N-terminal fragment as a fusion protein are produced recombinantly. Protein complex according to any one of claims 1-6, the selected one Polypeptide and the heavy chain or its N-terminal fragment via a chemical bond are connected. Protein complex according to claim 8, wherein the chemical Binding is a disulfide bond. Protein complex according to claim 8, wherein the chemical Binding is a peptide bond. A method of producing the protein complex of any one of the preceding claims comprising the steps of: a) isolating a botulinum toxin complex from Clostridium botulinum at a pH in the range of 2.0 to 6.5; b) adjusting the isolated botulinum toxin complex from step a) to a pH in the range of 7.0 to 10.0; c) separating the botulinum toxin from the complex proteins by chromatographic methods; d) mixing the complex proteins obtained in step c) with a polypeptide-Hc conjugate; or e) separating the complex proteins obtained in step c) and mixing at least one complex protein with a polypeptide-Hc conjugate; f) dialyzing the mixture from step d) or e) against a buffer at a pH in the range from 6.5 to 2.0. Use of the protein complex according to one of claims 1 to 10 as a transport vehicle for pharmacological active, immunologically active or used for diagnostic purposes Polypeptides.