WO2004016148A2 - Shiga toxin b-subunit as a vector for tumor diagnosis and drug delivery to gb3 expressing tumors - Google Patents
Shiga toxin b-subunit as a vector for tumor diagnosis and drug delivery to gb3 expressing tumors Download PDFInfo
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- WO2004016148A2 WO2004016148A2 PCT/EP2003/009308 EP0309308W WO2004016148A2 WO 2004016148 A2 WO2004016148 A2 WO 2004016148A2 EP 0309308 W EP0309308 W EP 0309308W WO 2004016148 A2 WO2004016148 A2 WO 2004016148A2
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- A61K47/67—Enzyme prodrug therapy, e.g. gene directed enzyme drug therapy [GDEPT] or VDEPT
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- A61P43/00—Drugs for specific purposes, not provided for in groups A61P1/00-A61P41/00
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- B82Y5/00—Nanobiotechnology or nanomedicine, e.g. protein engineering or drug delivery
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- C07K14/00—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
- C07K14/195—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from bacteria
- C07K14/24—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from bacteria from Enterobacteriaceae (F), e.g. Citrobacter, Serratia, Proteus, Providencia, Morganella, Yersinia
- C07K14/25—Shigella (G)
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- C07K14/195—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from bacteria
- C07K14/36—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from bacteria from Actinomyces; from Streptomyces (G)
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Definitions
- the invention relates to new compounds for cancer therapy or diagnosis and more specifically to the use of a non-toxic Shiga toxin B subunit mutant as a vector for diagnostic products or drugs in Gb 3 over- expressing receptor cells.
- glycosphingolipids are major components of membrane microdomains (rafts) that play a central role in receptor aggregation and receptor interaction with signaling molecules, such as kinases of the Src family.
- rafts membrane microdomains
- signaling molecules such as kinases of the Src family.
- a role for glycosphingolipids and membrane microdomains in intracellular sorting is currently evaluated. According to the so-called "raft hypothesis" proposed by Simons and coworkers, asymmetry in the lipid and protein distribution in the lateral plane of membranes contributes to membrane sorting to distinct intracellular destinations.
- GSL globotriaosyl ceramide (Gb 3 or CD77) is expressed on a narrow range of committed B cells and associated B cell lymphomas (Gordon et al., 1983; Kalisiak et al., 1991; Mangeney et al., 1991 ; Murray et al., 1985; Oosterwijk et al., 1991). Indeed, it was recently reported that binding sites for Gb 3 -specific ligands could be detected on all grades of follicle centre cell lymphomas, with more than 70% of patient tumor samples being positive (LaCasse et al., 1999).
- Natural ligands of Gb 3 have been described, encompassing the bacterial protein toxins Shiga toxin from Shigella dysenteriae and the verotoxins from Escherichia coli (Lingwood, 1996; Sandvig and van Deurs, 1996). These toxins are composed of two subunits.
- the enzymatic A-subunit modifies ribosomal RNA thus leading to an inhibition of protein biosynthesis.
- the A-subunit has to interact with the non-toxic B-subunit, a homopentamer of 5 B-fragments.
- the B-subunit binds, under certain conditions in a cooperative manner, to 10-15 Gb 3 molecules.
- Shiga toxin and its non-toxic B-subunit are targeted by retrograde transport from the plasma membrane to the endoplasmic reticulum, via the early endosome and the Golgi apparatus (for a review, see (Johannes, 2002)).
- the A-subunit passes via retrotranslocation across the membrane into the cytosol.
- Shiga Holotoxin has been described as an anti-tumor agent in xenograft transplants in mice (Arab et al., 1999). Furthermore, it eliminates clonogenic tumor cells in purging applications (LaCasse et al., 1996).
- the use of the holotoxin as a therapeutic agent has important limitations.
- First, the action of the A-subunit of the toxin is not tumor cell specific.
- Second, the holotoxin is a large protein whose capacity to infiltrate solid tumors is limited.
- a large bacterial protein as the holotoxin leads to an efficient immune response. Forth, the necessity to maintain simultaneous Gb 3 and A-subunit binding limits the possibility to introduce mutations that favor immune evasion or intracellular targeting.
- Cysteine is added at the C-terminus of mature STxB.
- the protein when purified from bacteria, carries the internal disulfide bond, as wild type STxB, while the sulfhydryl group at the C-terminal Cys is free. Due to their nucleophilicity, free sulfhydryl groups are excellent acceptors for directed coupling approaches (Philippe Schelte et al., 1999).
- mutants can be used as universal carriers for targeting molecules to Gb 3 receptor expressing cells.
- the present invention relates to an hybrid compound for the diagnosis or therapy of cells over-expressing the receptor Gb 3 , having the following formula: STxB-Z(n)-Cys-Y(m)-T, wherein: - STxB is the Shiga Toxin B subunit or a functional equivalent thereof,
- n 0 or 1 and when n is 1 , Z is an amino-acid residue devoid of sulfydryl group or is a polypeptide, - Cys is the amino-acid residue for Cysteine,
- - T is a molecule linked by a covalent bound to the S part of Cys, selected in a group comprising:
- agents for in vivo diagnosis . cytotoxic agents, . prodrugs, or
- Y is a linker between T and Cys, said linker being either cleavable or not cleavable for the release of T after the internalization of the hybrid compound into said cells.
- T is thus operably linked to Cys either directly through covalent binding or indirectly through a linker, Y, allowing or not said release of T moiety.
- STxB-Z(n)-Cys moiety of the hybrid compound has the following sequence (SEQ ID No 1):
- Gb 3 is not present in normal intestinal epithelia in humans (Jones et al., 2000). Accordingly, it has been shown that Gb 3 is present in low to undetectable levels in mouse.
- Gb 3 is over-expressed in the human colon cancer cell line CaC02 (Jones et al., 2000). Thus, it constitutes an excellent marker to distinguish between tumor cells and normal intestinal cells both in humans as well as in murine models.
- This differential pattern of Gb 3 expression provides the basis for the new therapeutic and diagnostic developments of the present invention in colorectal cancer, and more generally in any Gb 3 over-expressing tumor or cancer cell.
- Over expression of Gb3 receptor on cells can be assessed by carrying out a method such as that disclosed in Example 1 when assessing the mouse model, especially starting from biopsy material.
- Another method encompasses performing an MRI for determination of Gb3 distribution. In some situations however, confirmation that the tumor to be treated is a Gb3 over-expressing tumor is not specifically sought prior to initiating the treatment.
- the expression "therapeutic treatment” encompasses the action of the hybrid compound of the invention which results in a beneficial effect for the patient undergoing the treatment, said effect being either obtained at a cellular level or at a clinical level, including encompassing as a result an improvement of the condition of the patient or a remission state or a recovery of a health state.
- said therapeutic treatment is provided to a patient having a tumour and especially suffering from a cancer.
- the expression "diagnosis” encompasses the detection of a pathological state or the detection of one or several parameters which may be correlated either directly or indirectly, possibly in combination with other parameters, to a pathological state and which may provide information useful in a diagnostic protocol.
- the expression also encompasses the possible quantitative detection of parameters related to such a pathological state.
- the hybrid compounds of the invention can bear a T moiety which is a contrast agent for the detection of Gb 3 - expressing cancer cells by life-imaging techniques such as Magnetic Resonance Imaging (MRI).
- life-imaging techniques such as Magnetic Resonance Imaging (MRI).
- Other non-invasive life imaging techniques include two-photon microscopy, contrast enhanced ultrasound, contrast enhanced X-ray, computed tomography, isotope scanning, contrast enhanced thermography.
- said contrast agents can be selected in a group comprising paramagnetic compounds, such as porphyrin-gadolinium, porphyrin-manganese, synthetic polymer-gadolinium, gadolinium- ethoxybenzyl-diethylenetriaminepentaacetic acid, DOPTA-gadolinium, ferrofluide and nanoparticules, which are then administrated to humans or animals.
- paramagnetic compounds such as porphyrin-gadolinium, porphyrin-manganese, synthetic polymer-gadolinium, gadolinium- ethoxybenzyl-diethylenetriaminepentaacetic acid, DOPTA-gadolinium, ferrofluide and nanoparticules, which are then administrated to humans or animals.
- the present invention also pertains to the use of such compounds for in vivo diagnosis of tumors, more specifically for MRI diagnosis.
- the use is advantageous for intestinal and colorectal cancers as far as it has been shown that Gb 3 receptors are expressed specifically in cancer cells but not in normal cells.
- the hybrid compounds of the invention can bear as a T moiety a tumor specific drug or pro-drug which is vectorized to tumor-specific transport pathways in Gb 3 -positive cancer cells allowing the increase of the efficiency and/or specificity of these treatments.
- T moiety might also be a pro-drug activator while the pro-drug alone is administered directly by any known drug delivery system, i.e. by systemic, transdermic, oral, rectal administration.
- the use of the B-subunit as a cancer targeting means has the following advantages. First, due to its small size, tissue penetration with the B-subunit is efficient. Second, the antibody response to the B- subunit is inefficient. Third, tumor-selective compounds can be coupled to the B-subunit. Forth, tumor-specific transport pathways can be exploited to increase the efficiency of the treatment. Fifth, when modifications of the B- subunit are done, only Gb 3 binding ability needs to be preserved.
- the drug is a photosensitizing drug suitable for Dynamic Phototherapy (DPT).
- DPT is a recently developed technique for the treatment of solid human tumors. It is based on the targeting to and photoactivation of dyes such as porphyrins or related system within tumor tissue. The molecular events are beginning to be understood, such as cellular death through apoptosis and other mechanisms, implicating mitochondria, nuclei, ...
- Some photosensitizing drugs are already used in the clinics (Photofrin®, Foscan®, ). However, these substances have a number of drawbacks, most notably the absence of tumor-specific targeting.
- Several strategies have been proposed to improve the tumor selectivity of photosensitizers.
- Suitable delivery systems such as liposomes, lipoproteins, monoclonal antibodies, nanoparticules to modify biodistribution of dyes.
- Another approach developed at the Institute Curie is to modulate the amphiphilicity of the macrocycle. Structural modifications induced by glycoconjugation of the tetrapyrrolic system is an effective means to create a balance between hydrophilicity and hydrophobicity. Following this approach, neutral tri- and tetra-glycoconjugated tetrapyrrolic macrocycles were prepared and evaluated in vitro for their photocytotoxicity (Momenteau et al., 1999).
- a glycoconjugated, relatively hydrophilic tetrapyrrolic macrocycle (porphyrin) has been synthesized, which carries a bromo-benzyl group that allows coupling to STxB/Cys. Synthesis, coupling to STxB/Cys, and purification of the resulting compound are described hereunder.
- the therapeutic compound composed of STxB/Cys and the glycoconjugated porphyrin accumulates stably in the endoplasmic reticulum and the Golgi apparatus.
- the phototoxicity of the porphyrin can then be activated locally by irradiation with visible light after the clearance of the cytotoxic compound from cells that need to be preserved, such as dendritic cells in which STxB does not target the retrograde route (Falguieres et al., 2001).
- T is a cytotoxic agent.
- Said cytotoxic agent might be toxic for the cell after internalization either directly , or indirectly through the action of a second component, said second component acting as a mean for transforming a pro-drug into a cytotoxic drug.
- cytotoxic agent is Neocarzinostatin (NCS).
- NCS Neocarzinostatin
- Holo-neocarzinostatin is the prototype of the protein antibiotic family. It is a 11.3 kDa complex consisting of a dodecadiyne antibiotic (NCSchrom) which contains the cytotoxic activity, reversibly bound to a carrier protein known as apo-neocarzinostatin (apo- NCS) (for a review, see (Favaudon, 1982)).
- NCSchrom dodecadiyne antibiotic
- apo- NCS apo-neocarzinostatin
- Holo-NCS is active in the nanomolar range, and NCSchrom cleaves DNA in the course of a suicide reaction leaving no residual active drug after a few minutes incubation. No resistance to NCSchrom associated with reduced drug import (MDR) has been reported.
- the major DNA lesions induced by NCSchrom in DNA result from radical attack and consist of a blunt end break bearing a thymidine- ⁇ '-aldehyde residue on one strand, with an abasic site at two nucleotide interval on the complementary strand.
- This abasic site is substrate for endonuclease III in such a way that NCSchrom-induced damage is very rapidly converted into DNA double-strand breaks in living cells.
- Mutants of E. coli, yeast or mammalian cells defective in any pathway of double-strand break repair, most notably through a defect in DNA- dependent protein kinase are consistently hypersensitive to induced cell kill by NCS.
- Prodrugs are defined as therapeutics agents which are inactive but are transformed in active metabolites by biotransformation.
- the pro-drug is then transformed by a second component inside the cell after internalization of the hybrid compound.
- Said second component might be a cell metabolite such as an enzyme.
- T is a cytotoxic drug such as anthracyclins (daunomycin, doxorubicin, daunorubicin%), idarubicin, cis-platinium, mitomycin C, desacetylvinblastine, methotrexate, N-acetylmelphan, 5-fiuorouracil, nitrogen mustards, calicheamicin, maytansinodids, and Y is a linker sensitive to an endogeneous enzyme such as a mannosidase.
- Another embodiment includes the approach described by (Saxon and Bertozzi, 2000).
- a sugar precursor containing an azido group is targeted to cancer cells via STxB/Cys. After liberation of the azido-carrying sugar in the Golgi apparatus, the later is integrated into carbohydrate chains of the cancer cell.
- a phosphin-carrying prodrug In interaction with a phosphin-carrying prodrug, a therapeutic compound is released that specifically acts in the tumor environment
- Another embodiment includes the use of amidoximes (N-
- Hydroxyamidines as pro-drugs, cleavable by endogeneous reductases.
- reductases are responsible for the reduction of amidoximes to amidines.
- a microsomal enzyme system has been purified from pig and human liver consisting of cytochrome b5, its reductase and a P450 isoenzyme (Clement B et al., 1997).
- a similar enzyme system is present in mitochondria. Reductive activities are located in several organs such as liver, kidney, lung and even brain.
- prodrugs are made incorporating linkages that are sensitive to mannosidase.
- the prodrugs are coupled to STxB/Cys and targeted to Gb 3 expressing cancer cells.
- the activation of the prodrug occurs in the Golgi apparatus of the cancer cell using endogenous mannosidase without prior vectorization of the enzyme.
- prodrugs that contain glucoronic acid conjugated through a linker moiety to the aminoglycoside of doxorubicin.
- prodrugs are synthesized as described in (Bakina and
- the anthracycline prodrug can be converted to doxorubicin by ⁇ -glucuronidase.
- the T moiety of the second coumpound is the ⁇ -glucuronidase.
- ⁇ -glucuronidase is coupled to STxB/Cys as described hereunder for BSA and NCS.
- the coupling product is targeted to the Golgi apparatus ( Figure 13) and the endoplasmic reticulum of Gb 3 expressing tumors cells and retained in this compartment. In other cells, such as dendritic cells, the coupling product is rapidly degraded (Falguieres et al., 2001).
- the prodrug is coupled to STxB/Cys.
- the product can be activated in cells that have retained the STxB/Cys- ⁇ -glucuronidase coupling product (cancer cells), but not in cells that have lost this product (dendritic cells).
- the prodrug is a nucleotide analog which, after enzymatic transformation, can be incorporated into the replicating DNA and stop said replication.
- Such prodrugs for gene suicide cancer therapy are reviewed in Singhal S. et al. (1999).
- One example is an hybrid compound wherein T is Ganciclovir (GCV) or acyclovir (ACV), and Y is a linker cleavable by an endogeneous enzyme such as mannonidase.
- the second component is a second hybrid compound wherein T is the Thymidine kinase of Herpes Simplex Virus (HSV-i-TK). This enzyme can convert GCV or ACV to GCV monophosphate or ACV-monophosphate.
- GCV-triphosphate lacks the 3' OH on the deoxyribose as well as the bond between the 2' and 3' carbons which are necessary for DNA chain elongation. A a result, GCV-triphosphate integration causes premature
- the present invention encompasses also:
- Y is an enzyme cleavable linker selected in a group comprising reduced and non-reduced folates cleavable by carboxypeptidase G, phosphate groups from phosphorylated prodrugs cleavable by alkaline phosphatase, hydrolytic cleavable compounds by carboxypeptidase A, nitroreductase for prodrug activation, hydrolysis of lactam ring cleavable by beta-lactamase, amide cleavable by penicillin amidase, cytosine deamidase for prodrug activation, glucoronic acid cleavable by beta-glucoronidase, galactose cleavable by galactosidase, mannose cleavable by mannosidase.
- Y is an enzyme cleavable linker selected in a group comprising reduced and non-reduced folates cleavable by carboxypeptidase G, phosphate groups from
- Y is selected in a group comprising non-selective linkers such as glutaric acid, dianhydride of diethylenetriaminepentaacetic acid, carbodiimide..., acid cleavable linker such as cis-aconitic anhydride, acyl hydrazones, Schiff bases, trityl linkers, lysosomally degradable, disulfide, linkers such as SPDP.
- non-selective linkers such as glutaric acid, dianhydride of diethylenetriaminepentaacetic acid, carbodiimide...
- acid cleavable linker such as cis-aconitic anhydride, acyl hydrazones, Schiff bases, trityl linkers, lysosomally degradable, disulfide, linkers such as SPDP.
- the skilled person can easily adapt this strategy of pro-drug conversion using the Hybrid compounds according to the invention to any known pro-drug principle, and more particularly to the multiple and complementary suicide therapies.
- the synergistic effect of the multiple suicide strategy enables lower doses or individual drugs for maximum sensitivity and reduces cytotoxicity in nontransduced cells. Furthermore, development of resistance to the suicide strategy is greatly reduced when two (or more) separate pathways are targeted.
- the present invention pertains to the use of an hybrid compounds of the formula STxB-Z(n)-Cys-Y(m)-T for the therapies of Gb 3 expressing cells.
- Gb 3 expressing cells are intestinal, and particularly colorectal cells which express Gb 3 receptor only when they are tumor cells.
- STxB-Z(n)Cys-Y(m)-T as defined in the present invention provides means for therapy of pathogenic states including tumors or cancer associated with over-expression of Gb3 receptor on tumor cells.
- the present invention also pertains to pharmaceutical compositions containing at least one hybrid compound of the formula STxB-
- compositions apply either for in vivo diagnosis or for therapy of cancers cells or tumors and might contain any of the hybrid compounds described herein.
- a pharmaceutical composition according to the invention advantageously comprises one or more components to be administered in one step or sequentially in time.
- a first component of the pharmaceutical composition contains as an active component an hybrid compound wherein T is an enzyme, and for example ⁇ -glucoronidase which is first administrated to a patient bearing a tumor having over-expressing T is an enzyme, and for example ⁇ -glucoronidase which is first administrated to a patient bearing a tumor having over-expressing
- this first component is administered once to such patients;
- the second component of the pharmaceutical composition contains an hybrid compound according to the invention wherein T is a prodrug and Y is glucoronic acid; this second component of the pharmaceutical composition might be administered to the patient sequentially in the time with repetited administrations to obtain a long term effect of the therapy.
- a pharmaceutical composition according to the invention is particularly interesting for the treatment of intestinal tumors and more particularly for colorectal tumors as far as, it has been demonstrated herein, first that these tumors express specifically Gb 3 receptor and second that the pharmaceutical compositions bearing pharmaceutical carriers for oral or rectal administration are effective after an oral or rectal administration of the pharmaceutical composition.
- the present invention also pertains to a method for inducing the death of cancer cells bearing over expressing Gb 3 receptors, the method comprising administering an effective amount of at least one hybrid compound described herein above, such that cancer cells death occurs. Accordingly, the invention relates in particular to means suitable for in vivo diagnosis of tumor or in vivo diagnosis of cancer.
- the invention also pertains to a method for in vivo diagnosis of cancer or tumor cells over-expressing Gb 3 receptor, this method comprising administering an effective amount of an hybrid compound having a T moiety which is a contrast agent.
- the universal part of the hybrid compound i.e, STxB-Z(n)-Cys might be manufactured by a recombinant cell line obtained by transformation with a recombinant vector or plasmid comprising a polynucleotide sequence encoding the STxB-Z(n)-Cys part of the hybrid compound.
- sequence including such molecule is an isolated polynucleotide selected from the group of: (a) a polynucleotide comprising the nucleotide sequence STxB encoding the Shiga Toxin B subunit or a functional equivalent thereof bearing at its 3'end the codon TGT, or the codon TGC encoding Cysteine; b) a polynucleotide comprising a nucleotide sequence having at least 80% sequence identity to a nucleotide sequence encoding the
- a first method that can be embodied is the use of SPDP hetero-bi-functional cross-linker described par Carlsson et al.
- SPDP is capable of being cleavable by serum thiolases that is a cause of decreasing the yield of the reaction.
- a second method for covalent coupling of STxB -Z(n)-Cys peptides with another peptide of interest is to produce bromoacetyl or maleimide functions on the latter as described by P. Schelte et al. Briefly, the peptide of interest is chemically activated with bromoacetate anhydride or by a maleimide group respectively. In appropriate reaction conditions (pH, temperature, incubation times), these groups are eliminated by cis- elimination, yielding respectively to -S-S, -S-CH 2 -, to -S-CO- or to -S-NH- covalents linkages.
- the polypeptide or the peptide to be coupled to the -SH moiety the C-terminal Cysteine of the universal carrier has its N-terminus activated with bromoacetic anhydride following the reaction scheme:
- the resulting thioether-linkage is stable to hydrolysis.
- Another method for coupling a molecule to the universal carrier of the invention is to use MBS (m-Maleimidobenzoyl-N- hydroxysuccinimide ester) as shown in figure 9. This coupling allows the transport and processing of large molecules such as enzymes.
- MBS m-Maleimidobenzoyl-N- hydroxysuccinimide ester
- Figure 1 Uptake of STxB by intestinal tumors after 2.5 h, comparison with normal tissue. Upper panels: normal duodenum, lower panels: tumor from the periampullar region. Left panels: nuclei are stained with Hoechst dye. Right panels: anti-STxB staining.
- FIG. 2 In normal tissue, enteroendocrine cells take up STxB. A region from normal duodenum is shown, nuclear staining with Hoechst (upper left panel), anti-chromogranin A/B antibody (upper right panel) and anti-STxB antibody (lower left panel). Lower right panel shows a superposition of the three stainings: nuclei (blue), chromogranin A/B (red), STxB (green). Yellow color demonstrates colocalisation of chromogranin and STxB.
- Figure 3 Uptake of STxB by intestinal tumors after 24 h, comparison with normal tissue. Upper panels: normal duodenum. Lower panels: tumor from the periampullar region. Left panels: nuclei are stained with Hoechst dye.
- FIG. 4 Right panels: anti-STxB staining.
- Figure 4 STxB is not present in control tissue (liver), even after 24 h.
- Figure 5 Structure of the water-soluble metallo-porphyrin that is coupled to STxB/Cys.
- Figure 6 Synthesis of compounds that are coupled to STxB/Cys to function as a contrast agents in RMI (ll-M) or as an anti-tumor cytotoxic drugs for PDT (II).
- Figure 7 Optical absorption spectrum of holo-NCS/STxB after incorporation of NCS c h r om and filtration over sephadex G25 to remove excess, non-specifically bound NCS chrom-
- Figure 8 Summary of the effect of low temperature (0°C) and PPMP on the response of HeLa cells to 4 nM (relative to NCS c hro m) holo- NCS or holo-NCS/STxB. Blanks are treated on ice for control.
- Figure 9 Scheme of MBS coupling method.
- FIG 10 Overexpression of Gb 3 by murine and human tumors.
- A STxB overlay experiment on neutral GSL extracted from normal (Ctrl) and tumor tissue samples obtained from Ras-APC mice.
- B Quantification of Gb 3 expression in normal (white bars) or tumor (grey bars) intestinal tissue samples. The averages are shown in black bars.
- C STxB overlay experiment on neutral GSL extracted from normal human colon (Ctrl) and tumor tissue.
- D Representation of Gb 3 overexpression by human colon tumors. Results are expressed as the ratio of Gb 3 expression in tumors over Gb 3 expression in normal adjacent tissue obtained from the same patient. Six independent experiments (white bars) and their average (black bar) are represented.
- FIG. 11 Tumor imaging using multiphoton microscopy.
- A,B,C Appearance of untreated intestinal tissue, revealed by autofluorescence on un-fixed, unstained tissue.
- A Villi in the duodenum.
- Figure 12 Vectorization of glyco-porphyrin H2TPP(p-O-b-D- GluOAc)3(p-CH2Br) to cancer cells.
- the upper blue line (open squares) reports the response of Hela cells in which the expression of Gb3 was inhibited using PPM P.
- the lower red line (open circles) reports on control HeLa cells. Note that the survival is significantly affected only in HeLa cells in which Gb3 is expressed, showing the receptor-dependent delivery of the glyco-porphyrin H2TPP(p-O-b-D-GluOAc)3(p-CH2Br) to cancer cells, via STxB.
- Figure 13 Analysis of STxB-dependent ⁇ -GUS targeting to the retrograde route of cancers cells. Note the perfect overlay of the labeling (yellow, lowest panel) obtained with the antibodies directed against STxB (red, uppermost panel) and ⁇ -GUS (green, middle panel).
- Figure 14 Vectorizartion of ⁇ -GUS activity onto cancer cells.
- ⁇ -GUS activity is given in arbitrary units. Note that Gb3 expressing HeLa cells (Gb3+ cells) show a significant increase of ⁇ -GUS activity comparatively to non-expressing cells (Gb3- cells). The activity of purified ⁇ -GUS is shown as a control.
- Figure 15 Computed quantitative T2 map of the four cell preparations. Note that cells with which NP have associated appear dark. Non-coated NP readily and non-specifically bind to HeLa cells. BSA-coating (NP-BSA) reduces non-specific binding. STxB-functionalized NP (STxB- Cys-MBS-BSA-NP) bind to HeLa cells in a receptor dependent manner.
- FIG 16 Targeting of STxB-EDEKKK coupled biotin to the Golgi apparatus of HeLa cells.
- Biotin is coupled to STxB-EDEKKK according to the manufacturer instructions (Pierce). After binding to HeLa cells on ice (30 min), STxB-EDEKKK is internalized for 45 min at 37°C. The cells are fixed, and double-stained for STxB (13C4 antibody) and streptavidin to detect vectorized biotin. Note that vectorized biotin accumulates in the perinuclear Golgi apparatus.
- EXAMPLE 1 VALIDATION OF THE MOUSE MODEL FOR IN VIVO DIAGNOSTIC AND THERAPEUTIC ADMINISTRATION OF HYBRID COMPOUNDS
- the murine model bears a colorectal cancer.
- transgenic animals that express oncogenic Ras under control of the villin promoter in intestinal epithelium, with the genetic background B6D2 (Tg villin-K-ras V12G; (Janssen et al., 2002) and the mouse line Apc 1638N that carries a heterozygous mutated allele of the Ape (adenomatous polyposis coli) locus in the C57BI/6 background (Fodde et al., 1994). Furthermore, a double transgenic line RasAPC is created by crossing the two transgenic lines. The animals used have an age of >6 months and a weight of 25-35 grams at the time of injection. The mice are maintained under a 12 hour light-dark cycle and fed with standard diet and water ad libitum.
- Intestinal specimens are processed immediately after sacrificing the animal.
- Small and large intestines are opened longitudinally, tumorous regions are dissected together with surrounding normal tissue and either embedded for cryosections (see below), or fixed in AFA (75% ethanol, 20% formalin, and 5% acetic acid) for 24 hours.
- AFA 75% ethanol, 20% formalin, and 5% acetic acid
- After embedding, three ⁇ m thick sections are cut from the tissue blocks, dewaxed, rehydrated and processed by routine H&E staining. Tumors are classified and graded according to the World Health Organization classification of tumors (Hamilton and Aaltonen, 2000).
- Adenocarcinomas are considered invasive if malignant epithelial cells, arranged in glandular and/or trabecular structures, are found invading at least the submucosa.
- Lipid extraction is done according to the method of Bligh and Dyer (Bligh and Dyer, 1959). Human and mouse tumor tissue and adjacent non-tumoral specimen are weighted, mechanically homogenized in 1 ml of aqueous buffer and injeceted into 3.75 ml of chlmoroform:methanol (1 :2).
- Dried plates are soaked in 0.1% polyisobutylmetacrylate in hexane, floated for 1 hour in blocking solution, followed by incubation with STxB (20 nM), primary polyclonal anti-STxB and secondary horse radish peroxidase- or alkaline phosphatase-coupled anti-rabbit antibodies. Reactive bands are revealed using enhanced chemiluminescence or chemifluorescence (Amersham Pharmacia, Little Chalfont, UK) and Phosphorlmager.
- Gb 3 expression levels are compared between normal and tumor tissue.
- FIG. 10 shows overexpression of Gb 3 by murine and human tumors 1.2: Gb 3 is strongly over-expressed in intestinal tumors: STxB-
- STxB-Cy3 labeling of cryosections is carried out to detect endogenous Gb 3 in normal intestinal and tumor tissue of otherwise untreated animals.
- a stock solution of STxB-Cy3 (0.22 mg/ml) is diluted 22 fold in PBS+0.2 % BSA (final concentration 10 ⁇ g/ml), and is incubated on sections for 30 min either before or after PFA fixation at room temperature for 20 min. Subsequently, the paraformaldehyde-fixed sections are treated with 50 mM NH 4 CI in PBS for 20 min, and solubilized with 0.1% Triton X- 100 for 5 min. Counterstaining with FITC-phalloidin and Hoechst dye as described above.
- Normal tissue is overall negative, except for a faint staining that was sometimes observable in the crypts, and occasional staining of single cells within the normal tissue. These cells may constitute enteroendocrine / lymphatic cells, based on morphological criteria. In contrast, tumors are strongly stained. 1.3: Orally administered STxB reaches intestinal tumors in vivo
- a pilot experiment is undertaken with a color marker to follow the distribution of injected fluid in the murine intestine: 0.5 ml of trypan blue is injected. The animal is sacrificed after 45 min, and the intestinal tract is removed and analyzed for distribution of trypan blue. The blue staining has clearly progressed through the largest part of the small intestine.
- Two animals are then injected with STxB, using in one animal a dose of 0.5 ml of a 1 mg/ml solution (animal A), or a smaller dose of 0.5 ml of a 0.1 mg/ml solution (animal B).
- a flexible plastic needle with a length of 40 mm and a diameter of 0.4 mm is used (Marquat Genie Biomedical, Boissy St Leger, Reference V010440).
- STxB is purified from bacteria (Mallard and Johannes, 2002) and dialyzed against PBS before injection. Animals are injected in the oesophagus with a single dose of 0.5 ml of a solution of varying concentrations STxB in PBS without anaesthesis. After the force-feeding, animals are kept for various time points and are allowed to feed with standard diet and water ad libitum.
- mice are sacrificed by cervical dislocation and tissues are removed for subsequent analyses. Tissue samples are taken along the intestinal tract, as well as tumors from each animal. The resected normal and tumoral tissue are prepared for cryosections, or processed for lipid extraction and subsequent overlay experiments, as described above. Animals are analyzed on serial cryosections with the monoclonal as well as the polyclonal antibodies for STxB. Mouse tissues embedded in Tissue-tek OCT (Sakura) are cut in serial sections at 5 ⁇ m thickness, air dried, and fixed with 3% paraformaldehyde at room temperature for 20 min.
- the paraformaldehyde- fixed sections are treated with 50 mM NH 4 CI in PBS for 20 min, and solubilized with 0.1% Triton X-100 for 5 min.
- Antibodies used are: monoclonal and polyclonal antibodies specific for STxB, diluted 1/100
- Hoechst 33258 (Sigma) to stain nuclei. Tumoral regions are identified by standard histological criteria, and they are positive for the proliferative marker Ki67. Epithelial cells are identified with a monoclonal anti-villin antibody. No STxB staining is observable in normal intestinal epithelial cells ( Figure 1), but strong staining occurrs in some occasional single cells that are interspersed in the epithelial layer, and present morphological characteristics of enteroendocrine cells, and are found to be positive for chromogranin A/B staining, a marker of enteroendocrine cells ( Figure 2). Furthermore, a few cells are labeled that might be of lymphatic origin (macrophages or dendritic cells).
- This staining pattern is found in the duodenum, jejunum, and ileum, but is absent from the colon. Peyer's patches are also essentially unmarked.
- a periampullar adenocarcinoma from animal A is very strongly labeled ( Figure 1).
- the labeling comprises about 50% of the whole tumor surface area, and is found in epithelial cells lining trabecular or glandular structures.
- stromal regions with signs of inflammation sometimes show staining, labeled cells are of putative lymphoid origin. The stroma is otherwise negative. However, two different lesions from the same animal are negative, apart from the staining in cells of putative lymphoid origin in the stroma.
- the animal B receives the weaker dose of STxB and shows essentially the same results, normal tissue is negative with the exception of a few single cells.
- a periampullar tumor is not marked, but a second tumor from the duodenum is labeled in tumor cells of epithelial origin (as evidenced by anti-villin staining). However, the overall intensity of the staining is markedly decreased as compared to animal A (dosis of 1.0 mg/ml).
- STxB in PBS The mice are sacrificed after 24 hours. Tissue samples are taken from control tissue (liver), and the intestinal tract: duodenum, jejunum, ileum, proximal colon. Tumors are isolated from both animals, and prepared for cryosections, and stained with polyclonal Ab anti-STxB and anti-chromogranin A/B. Even after 24 hours, STxB is still detectable in occasional cells in the otherwise negative epithelium, and is still very strongly present in tumors (Figure 3). No staining is observable in liver sections from both animals ( Figure 4).
- a contrast agent that is commonly used for RMI studies are paramagnetic metalloporphyrins.
- the porphyrin I ( Figure 6) is prepared by condensation of pyrrole, para-2, 3,4,6-tetraacetyl glucosyloxy benzaldehyde (Halazy et al.,
- Glycoconjugated compound II (Figure 6) is obtained quantitatively from I by treatment with MeONa/MeOH (Zemplen, 1927).
- Coupling is verified by MALDI-TOF, and coupled protein is purified by gel filtration and stored at -80°C.
- Gb 3 distribution by MRI techniques requires administration of a compound composed of the receptor specific molecule, STxB, linked to an appropriate paramagnetic contrast agent (ferrofluid or porphyrin). Accumulation of this targeted contrast agent at the fixation site locally modifies the water relaxation rates R1 ,R2,R2 * leading to MRI signal modification using T1 and/or T2 and/or T2 * weighted imaging sequences. Significant signal difference in images acquired before and after administration of the contrast agent depicts the regions of Gb 3 over- expression when non-specific accumulation can be excluded.
- the protocol can be applied to different tumor types over-expressing Gb 3 .
- the typical measuring procedure described hereafter is optimized for imaging intestinal tumors developed by our transgenic mouse model. Image acguisition
- Tumors are first detected by MRI in a screening session without contrast agent administration. Imaging is performed on a high field mini-imaging system, in our case a Bruker Biospec 47/30 system equipped with a 4.7 Tesla horizontal magnet. For that, the mouse is anaesthetized (preferred anaesthetic: isoflurane) and placed in a cradle in supine position.
- a high field mini-imaging system in our case a Bruker Biospec 47/30 system equipped with a 4.7 Tesla horizontal magnet.
- the mouse is anaesthetized (preferred anaesthetic: isoflurane) and placed in a cradle in supine position.
- Tubes containing circulating warm water are placed close to the animal in order to maintain body temperature.
- the animal is introduced in an MRI probe adapted to the size of the animal.
- a tube containing a water solution with adjusted R1/R2 relaxation rates is also introduced into the MRI probe and serves as an external signal intensity reference.
- Respiratory triggering has to be performed in order to obtain images of the abdominal region with minimal motion artifacts.
- Our preferred high sensitivity triggering device is home-made and is based on an inflatable chamber placed on the mouse abdomen and connected to a pressure transducer which delivers the trigger signal via appropriate electronics to the MRI system.
- Tumor detection is performed by means of a 3D T2 weighted fast spin echo imaging sequence with a field of view covering typically the liver and the intestinal region. Under these conditions tumors appear as hypersignal regions.
- the image resolution is typically 0.1x0.1x0.5 mm 3 .
- Tumors are localized with respect to anatomical markers, for example the stomach - intestine junction. Tumors are then imaged with T1 and T2 * weighted fast gradient echo sequences. This terminates the first imaging session.
- the second imaging session is performed on the same mouse after administration of the contrast agent (preferred administration: oral).
- the imaging protocol matches exactly that of the first imaging session.
- Regions of interest (ROIs) covering the tumors are defined on co-localized slices from the two imaging sessions. Mean intensities of the ROI
- ROIs are measured and normalized with respect to intensity of the external reference. Significantly different signal intensity detected in tumors after contrast agent administration demonstrates therefore Gb 3 over-expression.
- cell sample preparation comprised the following main steps : 1. Incubation of cells and NP at 4°C for 30 min. (binding); 2. washing (3 times); 3. incubation at 37°C for 2 hours
- Resected tumoral tissu samples from villin-RasV12 mice are placed directly into an imaging chamber containing Dulbecco's modified Eagle's medium (DMEM) without phenol red.
- DMEM Dulbecco's modified Eagle's medium
- a tunable pulsed Ti:Sapphire laser (Tsunami; Spectra Physics) pumped by a Nd-YVO4 laser (Milennia, Spectra Physics) provides 70 fs pulses at 750 nm with a 80 MHz repetition. Fluorescence is detected with the built-in Fluoview photomultiplier (R928, Hamamatsu Photonics) in the descanned configuration.
- Functionalized STxB can be used to target and identify intestinal tumors by non-invasive in-depth imaging approaches.
- the fluorophore Cy3 when coupled to STxB, is strongly accumulated in intestinal tumors, demonstrating that STxB delivers contrast agents for in vivo diagnostics to Gb3-expressing tumors.
- villi of the duodenum of resected normal or cancerous tissue are observed without prior fixation or staining, using nonlinear autofluorescence (Figure 11 A-C).
- the regular alignment of nuclei (dark zones) in the epithelial cells is clearly visible ( Figure 11 B).
- nuclei appear enlarged and staggered in the de-differentiated tumor sample ( Figure 11 C).
- Transgenic mice are then force-fed with fluorophore-coupled STxB. After 6 hours, tumor samples as well as samples of normal mucosa are resected and observed by multiphoton imaging. Normal tissue appears dark, while tumor tissue is brightly labeled with internalized STxB ( Figure 11 D-E).
- glycoporphyrin H2TPP(p-O-D-D-GluOAc)3(p-CH2Br) is dissolved in DMSO at 0.7 mM and mixed with an equal volume of STxB-Cys at 5.3 mg/ml. The mixture is incubated for 2 hours at room temperature and then passed through an G25 gel filtration column. The coupling product is snap frozen in liquid nitrogen and kept at -80°C for storage.
- Human tumor cells (either HT29 colon carcinoma or Hela cervix adenocarcinoma) are cultivated in Dulbecco's MEM supplemented with 10% fetal calf serum (FCS). Cells from log-phase culture are seeded in
- 96-microwell plates (0.2 mL-3x10 4 cells/well) and kept at 37°C in a water- jacketed incubator for 3 hour under an air/CO 2 atmosphere (5% CO 2 ). Tested compounds are added under the minimum volume. Plates are incubated 3 hours, then medium is removed and cells are washed twice with phosphate buffered saline (PBS) before addition of fresh medium free of drug. Irradiation with visible light (2J/cm 2 ) is performed through the bottom of the plates using a home made "light box” fitted with an orange filter (0% T at 520 nm and 80%T at 590 nm and above) leading to a fluence of 2 mW/ cm 2 .
- PBS phosphate buffered saline
- NEOCARZINOSTATIN a Purification of neocarzinostatin Holo-NCS is purchased from Nippon Kayaku Co. (Tokyo,
- holo-NCS is dialyzed against distilled water acidified with 1 mM acetic acid, lyophilized to dryness and stored in the dark at -80°C.
- the holo-NCS preparation is > 98% pure from isoelectric focusing (pH 2.5-4.5 gradient) on polyacrylamide gel and free from contaminating apo-NCS from absorption and fluorescence spectrocopy.
- NCSchrom is mostly (> 90%) in "A” form according to the nomenclature of Napier et al. (Napier et al., 1981).
- NCS/STxB is essentially pure.
- the protein fractions are pooled, concentrated by centrifugation over a Centricon® centrifugal filter unit (3.000 Da cutoff), sterilized by filtration over a Millex® unit (0.2 ⁇ m pore size) and stored in the dark at liquid nitrogen temperature (for prolonged storage it is recommended to lower the pH down to pH 5.0).
- the final concentration of the reconstituted holo-NCS/STxB is 9.8 ⁇ M relative to the absorption of protein-bound NCSchrom a 340 nm. d) Cytotoxicity assays
- HeLa cells are maintained as exponentially growing monolayers in Dulbecco modified Eagle's minimum essential medium with 4.5 g/l glucose, 0.1 g/l pyruvate, 10 ⁇ Ul/I penicilline, 0.1 g/l streptomycine, 0.86 g/l Glutamax I and 10% v/v foetal calf serum
- PPMP DL-threo-1-phenyl-2-hexadecanoyl- amino-3-morpholino-1-propanol
- Cytotoxicity assays are performed in parallel using HeLa cells subcultured with or without PPMP. Briefly, cells are seeded at a density of
- cytotoxicity of holo-NCS or holo- NCS/STxB sterile aliquots of drug are thawed immediately prior to use, adjusted to the suitable concentration in pH 6.0 PBS and immediately introduced into culture flasks. All experiments are carried out in dim light to prevent photodecomposition of drugs. The inventors observe that full cytotoxic effect of holo-NCS develops within 6 min incubation only (37°C), and increasing the length of contact with drug beyond that time does not result in increased cell kill. For this reason the length of exposure to drug was limited to 15-min throughout. Following treatment, the flasks are washed twice with Hank's balanced salt solution, supplied with fresh medium, and returned to the incubator for 8 days.
- holo-NCS is known to be inactive at low temperature (Kappen et al., 1980) while STxB is still able to bind and saturate its receptor under these conditions (Johannes et al., 1997), and is expected to be internalized upon warming up.
- holo-NCS survival to holo-NCS is in the range 90% or more. Therefore, a low temperature effectively abolishes the cytotoxicity of holo-NCS. In contrast, the holo-NCS/STxB is still active at 0°C, in such a way that cell survival is ca. 30% only. PPMP induced marked resistance to holo- NCS/STxB.
- compositions are made using STxB as a carrier that allow for targeting of therapeutic compounds to Gb3 expressing tumors.
- the effect of these compositions on tumor cells in vitro, on tumors in the described animal models, and on human tumors has been demonstrated.
- EXAMPLE 6 ENZYME DELIVERY FOR PRODRUG ACTIVATION Chemical coupling of ⁇ -Glucuronidase to STxB-Cys. 3 mg/ml of purified ⁇ -Glucuronidase ( ⁇ -GUS) in 100 mM HEPES, pH 7.4 is reacted with 90 ⁇ M of the heterobifunctional cross linker MBS for 30 min at room temperature. The unreacted MBS is separated from the formed complex ⁇ -GUS-MBS by gel filtration through a PBS-EDTA 10 mM equilibrated PD-10 column.
- ⁇ -GUS purified ⁇ -Glucuronidase
- the activated ⁇ -GUS is then concentrated to 2 mg/ml, mixed with a 35 excess molar of STxB-Cys, and incubated over night at room temperature.
- the formed conjugate STxB-Cys- ⁇ -GUS is purified by passage on a gel filtration column and an anti-STxB immunoaffinity column. Purified coupling product is highly pure, as tested by Western blotting, and the activity of the enzyme is not altered by the chemical modifications.
- the cells are then washed with ice-cold culture medium, shifted to 37°C for 40 min (internalization step), fixed with 4% PFA for 10 min, permeablized with saponin, stained with the indicated primary and secondary antibodies and analyzed by confocal microscopy. The obtained results are illustrated in figure 13.
- Hela cells (10 6 ) are incubated for 30 min at 4°C in presence or absence of 0.5 ⁇ M STxB-Cys- ⁇ -GUS (binding step). After washing with culture medium, cells are shifted to 37°C for 60 min (internalization step). Cell lysates are prepared in RIPA buffer (PBS 1X, NP40 1%, Doc 0.5%, SDS 0.5%).
- RIPA buffer PBS 1X, NP40 1%, Doc 0.5%, SDS 0.5%).
- the basal cellular ⁇ -GUS activity and ⁇ -GUS activity associated with ⁇ -GUS-STxB treated, Gb3 expressing and non-expressing Hela cells are summarized in figure 14.
- Gb3 expressing HeLa cells show a significant increase of ⁇ -GUS activity comparatively to non-expressing cells. These latters possess the same level of ⁇ -Glucuronidase activity as control cells (basal activity), indicating that cellular targeting of ⁇ -GUS activity is dependent on STxB/
- Alternatives to coupling via the sulfhydryl groups (-SH) are coupling via amino groups (-NH2), carbohydrates, carboxyls (-COOH), or hydroxyls (- OH).
- Examples of reactive groups on to-be-vectorized compounds are imidoesters (react on primary amines), N-hydroxysuccinimide esters (react on primary amines), maleimides (react on sulfhydryls), haloacetyls (react on sulfhydryls), hydrazines (react on oxidized carbohydrates), carbodiimides (react on carboxyls). Wild type STxB is not glycosylated.
- Glycosylated STxB for chemical coupling can be obtained by expressing a glycosylation site-carrying variant of STxB in glycosylation competent cells, such as the yeast Pichia pastoris. Amino groups, carboxylates, and hydroxyls are present in wild-type STxB, and chemical coupling results in heterogenous mixtures containing inactivated protein. To obtain some degree of site-directed coupling, amino acids with appropriate side chains are fused to the carboxyl terminus of
- the amino acid sequence EDEKKK (Glu-Asp-Glu- Lys-Lys-Lys) is fused to the carboxyl terminus of wild-type STxB. Reaction with N-hydroxysuccinimide ester-activated biotin allows to introduce biotin onto STxB-EDEKKK without inactivating the protein, as exemplified in figure 16 in which STxB-vectorized biotin can be detected in the Golgi apparatus of HeLa cells.
- Neocarzinostatin chromophore purification of the major active form and characterization of its spectral and biological properties. Biochemistry. 20:5602-5608. Ohtsuki, K., and N. Ishida. 1975. Neocarzinostatin-induced breakdown of deoxyribonucleic acid in HeLa-S3 cells. J. Antibiot. (Tokyo). 28:143-148.
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EP03775133A EP1525478B1 (en) | 2002-08-02 | 2003-07-31 | Shiga toxin b-subunit as a vector for tumor diagnosis and drug delivery to gb3-expressing tumors |
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EP1386927B1 (en) * | 2002-08-02 | 2005-03-30 | Institut Curie | Shiga toxin B-subunit as a vector for tumor diagnosis and drug delivery to GB3 expressing tumors |
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WO2018192719A1 (en) | 2017-04-20 | 2018-10-25 | Institut National De La Sante Et De La Recherche Medicale | Peptides, especially polypeptides, phage display screening method and associated means, and their uses for research and biomedical applications |
JP2020519244A (en) * | 2017-04-20 | 2020-07-02 | アンスティトゥート・ナシオナル・ドゥ・ラ・サンテ・エ・ドゥ・ラ・ルシャルシュ・メディカル・(インセルム) | Peptides for research and biomedical applications, particularly polypeptides, phage display screening methods and related tools, and uses thereof |
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AU2003283228A8 (en) | 2004-03-03 |
AU2003283228A1 (en) | 2004-03-03 |
ATE439597T1 (en) | 2009-08-15 |
EP1525478A2 (en) | 2005-04-27 |
JP2006509727A (en) | 2006-03-23 |
EP1386927B1 (en) | 2005-03-30 |
CA2494541A1 (en) | 2004-02-26 |
WO2004016148A3 (en) | 2004-10-28 |
DE60328789D1 (en) | 2009-09-24 |
ES2330429T3 (en) | 2009-12-10 |
US20110243914A1 (en) | 2011-10-06 |
US7981400B2 (en) | 2011-07-19 |
EP1386927A1 (en) | 2004-02-04 |
CA2494541C (en) | 2011-10-18 |
EP1525478B1 (en) | 2009-08-12 |
US7718601B2 (en) | 2010-05-18 |
JP4339251B2 (en) | 2009-10-07 |
DE60203491D1 (en) | 2005-05-04 |
ATE292144T1 (en) | 2005-04-15 |
US20060008475A1 (en) | 2006-01-12 |
US20100329992A1 (en) | 2010-12-30 |
US8313731B2 (en) | 2012-11-20 |
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