WO1998031788A1 - Injectable formulations for treatment of osteoporotic bone - Google Patents

Injectable formulations for treatment of osteoporotic bone Download PDF

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Publication number
WO1998031788A1
WO1998031788A1 PCT/US1998/001143 US9801143W WO9831788A1 WO 1998031788 A1 WO1998031788 A1 WO 1998031788A1 US 9801143 W US9801143 W US 9801143W WO 9831788 A1 WO9831788 A1 WO 9831788A1
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WIPO (PCT)
Prior art keywords
bone
bmp
rhbmp
active agent
proteins
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PCT/US1998/001143
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French (fr)
Inventor
Alexandre Valentin-Opran
Stephen B. Trippel
John M. Wozney
Howard Seeherman
Thomas Turek
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Genetics Institute, Inc.
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Application filed by Genetics Institute, Inc. filed Critical Genetics Institute, Inc.
Priority to AU62458/98A priority Critical patent/AU6245898A/en
Publication of WO1998031788A1 publication Critical patent/WO1998031788A1/en

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    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K38/00Medicinal preparations containing peptides
    • A61K38/16Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
    • A61K38/17Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from animals; from humans
    • A61K38/18Growth factors; Growth regulators
    • A61K38/1875Bone morphogenic factor; Osteogenins; Osteogenic factor; Bone-inducing factor
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61LMETHODS OR APPARATUS FOR STERILISING MATERIALS OR OBJECTS IN GENERAL; DISINFECTION, STERILISATION OR DEODORISATION OF AIR; CHEMICAL ASPECTS OF BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES; MATERIALS FOR BANDAGES, DRESSINGS, ABSORBENT PADS OR SURGICAL ARTICLES
    • A61L27/00Materials for grafts or prostheses or for coating grafts or prostheses
    • A61L27/14Macromolecular materials
    • A61L27/22Polypeptides or derivatives thereof, e.g. degradation products
    • A61L27/227Other specific proteins or polypeptides not covered by A61L27/222, A61L27/225 or A61L27/24

Definitions

  • the present invention relates to the field of tissue repair, specifically, to the treatment of osteoporotic bone and/or prevention of osteoporosis.
  • Osteoporotic or osteopenic bone is often characterized by suboptimal bone density.
  • the osteoporotic condition may be related to diet, trauma or stress, or to degenerative or congenital disease.
  • the present invention may be useful in the treatment and/or the prevention of osteoporosis, or the treatment of osteoporotic or osteopenic bone.
  • Idiopathic osteoporosis is a disease of unknown etiology characterized by progressive loss of bone mass and increased fragility. It is a medical problem because it is associated with a marked increase in susceptibility to fractures. It is a public health problem for several reasons.
  • hip fractures are currently the most common fracture in the elderly.
  • Praemer et ai Ibid.
  • Estimates based on census projections indicate that this figure will increase to approximately 340,000 hip fractures per year by the year 2000.
  • One out of every six Caucasian women will have a hip fracture during her lifetime (Cummings et al, Arch Intern Med 49:2455-2458 (1989), and for those who attain the age of 90, this figure becomes one in three.
  • approximately 20 percent remain in a long term care institution for at least one year following the fracture.
  • proximal femur fracture During the first year following injury, the mortality rate is approximately 15% higher than for age and gender matched controls. Praemer et al., Ibid. The financial toll of these fractures is also high. In 1988, hip fractures cost the United States 8.7 billion dollars. Praemer et al., Ibid. The increased incidence of proximal femur fracture observed in elderly patients is mainly related to two factors: (1) a decreased bone density of their proximal femora; (2) an increased propensity to fall. There is an inverse relationship between the age-related bone loss in the proximal femur and the risk of hip fracture.
  • Bioactive agents that reduce the incidence of hip fractures or augment the healing of such fractures when they occur would substantially improve the health of the elderly.
  • the availability of an injectable agent would permit its use in fracture prevention, such as hip fracture, without the costs and morbidity of surgical intervention, such as for femoral neck fractures.
  • Such an agent would have application in fracture treatment, without increasing the extent or complexity of the surgical management.
  • the inventors have provided a novel method using bioactive agents to decrease the occurrence and/or severity of fractures to osteoporotic bone, such as an osteoporotic hip.
  • the present invention provides methods and compositions for increasing bone mass and quality, and for minimizing or reducing the incidence or severity of osteoporosis-related fractures. Accordingly, the present invention provides methods and compositions useful for decreasing the incidence of fractures of osteoporotic or osteopenic bone.
  • the present invention comprises methods of treating patients with osteoporosis, or with other evidence of osteoporosis or osteopenic condition.
  • Preferred embodiments where the present invention may prove particularly useful include treatment of metaphyseal bone, including proximal femur (hip), proximal humerus (upper arm), distal radius (wrist), and vertebral bodies (spine), particularly the vertebral body.
  • the method comprises administering to a site of osteopenic or osteoporotic bone, or a site of low bone mass or density, an effective amount of a composition comprising at least one active agent which is capable of inducing growth of bone or increasing the formation of bone tissue or reducing bone loss at the site.
  • Bone mass is commonly designated “bone mineral content” or BMC and is measured in grams.
  • Bone density is commonly designated “bone mineral density” or BMD and is expressed as grams per unit area or grams per unit volume.
  • the mode of administration is by intraosseous injection.
  • the active agent is one or more proteins selected from the group of proteins known as the Transforming Growth Factors-Beta (TGF- ⁇ ) superfamily of proteins, preferably selected from the Bone Morphogenetic Proteins (BMPs), the Growth and Differentiation Factors (GDFs), as well as other proteins, as described more fully herein.
  • TGF- ⁇ Transforming Growth Factors-Beta
  • BMPs Bone Morphogenetic Proteins
  • GDFs Growth and Differentiation Factors
  • the methods and compositions of the present invention are advantageous in that they provide a localized treatment for osteoporosis or osteopenic bone, rather than systemic treatment.
  • the present invention is further advantageous in that it utilizes as active agents osteogenic proteins, which may be produced via recombinant DNA technology, and therefore are of potentially unlimited supply.
  • the methods and compositions of the present invention are further advantageous in that regeneration of the bone tissue increases the bone mass/density, increase the bone strength, and thereby reduce the severity of osteoporosis or incidence of osteoporotic lesions, ultimately lessening the incidence of bone fractures.
  • the active agents are administered locally through injection using a suitable buffer and/or carrier.
  • a suitable buffer comprises glycine, sucrose, and glutamic acid hydrochloride, at a pH of less than 6.0.
  • this formulation comprises about 2.5% glycine (g/100 ml (w/v)), about 0.5% sucrose (w/v), about 5 mM glutamic acid hydrochloride (about 0.1% w/v), and about 0.01 % (w/v) polysorbate 80, at a pH of about 4.5.
  • This buffer is referred to later in this application as "MFR 842.” Further buffers suitable for use in the present invention are described in United State Patent 5,385,887, the disclosure of which is hereby incorporated by reference.
  • Suitable carriers include collagen gels, hyaluronate, alginates and hyaluronic acids, injectable calcium phosphates, polyols, demineralized bone matrix and combinations of the above.
  • Other carriers which may be useful for the present invention include blood as well as clotting proteins, such as fibrin or thrombin, and oils.
  • the active agent further comprises, in addition to one or more proteins selected from the TGF- ⁇ superfamily of proteins, one or more auxiliary proteins, such as Hedgehog, Noggin, Chordin, Frazzled, Cerberus and
  • compositions of the present invention may be useful for injectable formulations of BMPs for uses such as injection into joints for treatment and repair of osseous defects, cartilage defects, inhibition of cartilage degradation and to promote cartilage repair.
  • the formulations may also be injected into tendons, ligaments and/or their attachment sites to bone.
  • injectable formulations of BMPs may also find application to other bone sites such as bone cysts, implants into bones, closed fractures and distraction osteogenesis.
  • the methods comprise applying to the osteoporotic or osteopenic site an amount of a composition comprising one or more purified osteogenic proteins which is effective to induce the formation and/or maintenance of bone.
  • the active agent is preferably selected from the family of proteins known as the transforming growth factors-beta (TGF- ⁇ ) superfamily of proteins, which includes the activins, inhibins and bone morphogenetic proteins (BMPs).
  • TGF- ⁇ transforming growth factors-beta
  • BMPs bone morphogenetic proteins
  • the active agent includes at least one protein selected from the subclass of proteins known generally as BMPs, which have been disclosed to have osteogenic activity, and other growth and differentiation type activities.
  • BMPs include BMP proteins BMP-2, BMP-3, BMP-4, BMP-5, BMP-6 and BMP-7, disclosed for instance in United States Patents 5,108,922; 5,013,649; 5,116,738; 5,106,748; 5,187,076; and 5,141,905; BMP-
  • TGF- ⁇ proteins which may be useful as the active agent in the present invention include Vgr-2, Jones et al., Mol.
  • GDFs growth and differentiation factors
  • PCT applications WO94/15965; WO94/15949; WO95/01801; WO95/01802; WO94/21681 ; WO94/15966; WO95/10539; WO96/01845; WO96/02559 and others.
  • Also useful in the present invention may be
  • BIP disclosed in WO94/01557; HP00269, disclosed in JP Publication number: 7-250688; and MP52, disclosed in PCT application WO93/16099.
  • BMPs which are presently preferred for use in the present invention include BMP-2, BMP-4, BMP-5, BMP-6, BMP-7, BMP- 10, BMP-12 and BMP- 13.
  • the active agent is most preferably BMP-2, the sequence of which is disclosed in United States Patent 5,013,649, the disclosure of which is hereby incorporated by reference.
  • Other BMPs and TGF- ⁇ proteins known in the art can also be used.
  • the active agent may be recombinantly produced, or purified from a protein composition.
  • the active agent if a TGF- ⁇ such as a BMP, or other dimeric protein, may be homodimeric, or may be heterodimeric with other BMPs (e.g., a heterodimer composed of one monomer each of BMP-2 and BMP-6) or with other members of the TGF- ⁇ superfamily, such as activins, inhibins and TGF- ⁇ 1 (e.g., a heterodimer composed of one monomer each of a BMP and a related member of the TGF- ⁇ superfamily). Examples of such heterodimeric proteins are described for example in
  • the active agent may further comprise additional agents such as the Hedgehog, Frazzled, Chordin, Noggin, Cerberus and Follistatin proteins. These families of proteins are generally described in Sasai et al., Cell, 79:779-790 (1994) (Chordin);
  • the amount of active agent useful herein is that amount effective to stimulate increased osteogenic activity of present or infiltrating progenitor or other cells, and will depend upon the size and nature of the defect being treated, as well as the carrier being employed.
  • the amount of protein to be delivered is in a range of from about 0.1 to about 100 mg; preferably about 1 to about 100 mg; most preferably about 10 to about 80 mg.
  • CARRIER Materials which may be useful as the carrier in practicing the present invention include pharmaceutically acceptable materials having viscosity and polarity such that, when added to the bone morphogenetic protein, form a composition that possesses appropriate handling characteristics for injectable application to the site of osteoporotic or osteopenic bone. Adding the carrier to the bone morphogenetic protein allows the protein to remain in the diseased or lesioned site for a time sufficient to allow the protein to increase the otherwise natural rate of regenerative osteogenic activity of the infiltrating mammalian progenitor or other cells, and to form a space in which new tissue can grow and allow for ingrowth of cells.
  • the carrier may also allow the bone morphogenetic protein to be released from the disease or lesion site over a time interval appropriate for optimally increasing the rate of regenerative osteogenic activity of the progenitor cells.
  • the carrier may also supply a framework on which to induce new formation in severely osteoporotic bone.
  • the most preferred family of carriers comprises collagenous materials. These are preferably in a form suitable for injection, such as a gel. Such gels may be cross- linked or non-cross-linked. Other forms of collagen, such as dispersions or fibrillar collagen, may also be useful in the methods of the present invention.
  • Another preferred family of carriers is cellulosic materials such as alkylcellulose, including hydroxyalkylcellulose, methylcellulose, ethylcellulose, hydroxyethylcellulose, hydroxypropylcellulose, hydroxypropylmethylcellulose, and carboxymethylcellulose, the most preferred being the cationic salts of carboxymethylcellulose (CMC).
  • CMC carboxymethylcellulose
  • the carrier be in the form of a hydrated cellulosic viscous gel. Viscosity may be increased through mechanical means, such as high agitation for a suitable period of time, followed by autoclaving, or chemically.
  • the active agent and cellulosic carrier is preferably in a solution of suitable buffer.
  • One preferred buffer solution is a composition comprising, in addition to the active agent, about 1.0 to about 10.0%
  • (w/v) glycine about 0.1 to about 5.0% (w/v) of a sugar, preferably sucrose, about 1 to about 20 mM glutamic acid hydrochloride, and optionally about 0.01 to about 0.1% of a non-ionic surfactant, such as polysorbate 80.
  • Preferred solutions are from about 1 % to about 20% w/v cellulosic carrier/buffer. If desired, a salt may be added.
  • a preferred viscous gel carrier is described in Example 2 below.
  • the amount of osteogenic protein useful with viscous gel carrier is generally in a range of from about 0.1 to about 100 mg, preferably about 1 to about 100 mg; most preferably about 10 to about 80 mg per cubic centimeter of implant material required.
  • Resorbable hydroxyapatites as well as minerals, ceramics and phosphates.
  • Resorbable hydroxyapatites can be formulated at various porosities with varying resorption rates; their handling characteristics vary from hard implantable types, to gel-like consistency, to those that are injectable but harden at body temperature.
  • Suitable hydroxyapatite and ceramic carriers are described, for example in WO96/36562; and United States Patents 5,543,019; 5,306,305; 5,258,044; 5,496,399;
  • injectable polymers which may be viscous and which may optionally include a sequestering agent as well.
  • Suitable polymers and sequestering agents include those described in United States Patent 5,171,579, the entire disclosure of which is incorporated herein by reference.
  • Other polymers include the pluronics, such as Poloxamer 407 gel.
  • Pluronics are a class of water soluble ABA type block surfactant copolymers which exhibit the unique property of reverse thermal gelation. They are liquid (and hence syringeable) at 4°C and gel at body temperature.
  • Poloxamer 407 MW 12,500, is excreted unchanged in the urine after systemic absorption and has supposedly been shown to be non-toxic in animals.
  • Polylactides and/or polyethylene glycols including poly(lactide)/poly(ethylene glycol) gels.
  • Polylactides may be dissolved in polyethylene glycols, such as low molecular weight (2000) PLA dissolved in PEG to produce a syringeable solution that precipitates PLA upon injection into an aqueous environment, resulting in a relatively firm gel.
  • the literature cites conjugates, such as Poly(lactic acid)-poly(ethylene glycol) conjugates, as appropriate carriers for BMPs (Miyamoto et al., Clin. Orthop. Rel. Res.
  • fibrin-based polymers in liquid or gel form.
  • materials useful as sequestering agents are hyaluronic acid, sodium alginate, poly(ethylene glycol), polyoxyethylene oxide, carboxyvinyl polymer and poly( vinyl alcohol), and cellulosic materials, such as hydroxycelluloses.
  • One such preferred agent is carboxymethylcellulose.
  • the solid material may be combined with a viscous liquid carrier for ease and uniformity of administration.
  • the carrier may optionally be combined with a diluent, such as aqueous glycerol, preferably the carrier diluent would be present in concentrations of about 10 to about 80% (v/v).
  • a diluent such as aqueous glycerol
  • the carrier diluent would be present in concentrations of about 10 to about 80% (v/v).
  • the above materials may be combined in particular embodiments of the present invention.
  • polymers such as porous particulate polymers, may be dissolved or suspended in cellulosic or gel carriers to increase viscosity.
  • the active agents are administered locally through injection using only a suitable buffer as carrier.
  • a suitable buffer comprises glycine, sucrose, and glutamic acid hydrochloride, at a pH of less than 6.0.
  • Preferred compositions of buffer solutions comprise about 1.0 to about 10.0% (w/v) glycine, about 0.1 to about 5.0% (w/v) of a sugar, preferably sucrose, about 1 to about 20 mM glutamine, glutamic acid, or glutamic acid hydrochloride, and optionally about 0.01 to about 0.1 % of a non-ionic surfactant, such as polysorbate 80.
  • this formulation comprises about 2.5% glycine (g/100 ml (w/v)), about 0.5% sucrose (w/v), about 5 mM glutamic acid hydrochloride (about 0.1% w/v), and about 0.01% (w/v) polysorbate 80, at a pH of about 4.5.
  • This buffer has been described as MFR 842.
  • buffers suitable for use in the present invention are described in United State Patent 5,385,887, the disclosure of which is hereby incorporated by reference.
  • Preferred solutions may also include combinations of buffer and other carrier, such as a combination of buffer and cellulosic carrier. Preferred ranges for this combination are from about 1% to about 20% w/v cellulosic carrier/buffer. If desired, a salt may be added.
  • the injectable compositions of the present invention may be administered in any clinically acceptable manner of injection.
  • a number of commercially available syringes may be suitable for use in the present invention, and for administration of the compositions of the present invention.
  • suitable syringes are available the Calasept R syringe [JS Dental Manufacturing, Ridgefield CT] comprises sterile calcium hydroxide paste in isotonic saline solution, in a non-aspirating or modified aspirating cartridge syringe; Henke-Ject Aspirating Syringe and Hypo Brand Dental Syringes/Needles [Smith & Nephew MPL, Franklin Park, LL]; intraosseous needles from MPL, Inc., Chicago LL; and Luer-Lok R Syringes [Becton Dickinson, Franklin Lakes, NJ], may all be appropriate syringes for use in the present invention.
  • bone morphogenetic proteins are used as an osteoinductive agent in the process known as distraction osteogensis.
  • This process is an alternative to segmental bone regeneration in response to implanted osteoinductive agents.
  • the osteoinductive agent and carrier are placed in the defect created between the parent bone ends.
  • the osteoinductive agent has to have sufficient residence time in the defect to stimulate differentiation of sufficient numbers of bone forming cells to support new bone formation.
  • the carrier also has to have sufficient residence time to serve as a scaffold for bone forming cells to attach (osteoconduction).
  • the carrier also has to have sufficient porosity to allow cells and blood vessels to penetrate into the defect for bone formation to occur.
  • the process of distraction osteogenesis creates a regenerate construct between the distracted parent bone ends that is highly vascular and contains a large population of mesenchymal stem cells destined to become bone forming cells.
  • the regenerate construct represents a much more ideal environment for cell differentiation growth factors such rhBMP-2 to stimulate rapid bone induction relative to induction of bone within a segmental defect.
  • the process of distraction osteogenesis begins with an initial latency period allowing a fibrous connection to form between the bone ends to be distracted.
  • the bone ends are slowly distracted at a controlled rate of up to 1 mm per day in human clinical cases.
  • a prolonged consolidation period is required to allow the regenerate to form bone. This prolonged consolidation period which can be on the order 4 to 6 months is associated with considerable morbidity.
  • a frequent complication is the occurrence of pin track infections resulting from the extended length of time the external fixator used to generate the distraction must remain in place.
  • the regenerate does not form properly and a delayed union or non-union occurs.
  • the regenerate contains a responsive cell population and is already highly vascularized following the initial distraction phase, the use of bone morphogenetic proteins may rapidly accelerate the rate of bone formation during the normally prolonged consolidation phase of distraction osteogenesis. Acceleration of the distraction phase is limited by stretching of the soft tissues associated with bone.
  • the cells created using distraction osteogenesis may also be harvested in order to provide a source of cells which are primed for osteogenesis. These cells can be cultured to prepare immortalized cell lines. If desired, these cells can also be immunotolerized using agents such as CTLA4 receptors [U.S. Patent 5,434,131] or CTLA4 ligands or B7 monoclonal antibodies [WO 96/40915]. Methods and materials for such immunotolerization are disclosed in the above references, and include co- transfection or treatment with these factors. The disclosure of these references is hereby incorporated herein by reference.
  • the oophorectomized rat is a well-established model of osteoporosis and its use is recommended by the FDA as one of the animal models to be employed in demonstrating efficacy of potential therapeutic agents for osteoporosis.
  • Preclinical studies testing the efficacy of rhBMP-2 in the oophorectomized rat model of osteoporosis demonstrated that 100 Mg rhBMP-2 in MFR 842 buffer, injected into the intramedullary space of the tibial shaft, was associated with extensive bone formation. Further evaluation with this model is conducted at lower doses.
  • rat tibiae are injected with 0, 10, or 50 Mg of rhBMP-2 in 20 ML MFR 842 buffer.
  • Controls include sham ovariectomized animals [surgery performed, but ovaries are not removed], buffer injections and sham surgeries.
  • the femora are harvested and groups analyzed by DEXA, biomechanics, and histornorphometry.
  • Intraosseous administration of injectable rhBMP-2 is accomplished in the non-fractured (contralateral) femur using an operating room, biplanar fluoroscopy, and patient positioning on a fracture table. Each patient undergoes the necessary surgical treatment of the fractured femur. At the completion of surgical procedure, but before termination of the anesthesia, the lower extremities are repositioned on the fracture table to gain access to the uninjured contralateral hip. Under sterile conditions and biplanar image intensifier visualization, the designated dose of rhBMP-
  • Example 2 is delivered by percutaneous, intraosseous route into the proximal femur.
  • Follow-up evaluations include radiographic assessment, clinical evaluation of infection and fracture, and DEXA evidence of bone formation.
  • Example 6 Rabbit Ulnar Osteotomy and Fracture Models. In the osteotomy model, the ulna is simply exposed, the periosteum is stripped, and a 2 to 5 mm osteotomy created using an oscillating saw. The incision is then closed, and the appendage bandaged to provide additional stability. Bilateral surgeries may be used in order to compare active agent against untreated or control substances.
  • the rabbit ulnar fracture model is similar to the rat femoral fracture model.
  • the rabbit ulnar fracture model relies on a weight-driven blunt instrument to create the fracture essentially using incident three-point bending.
  • the fracture is created by fully extending and clamping the forelimb to an aluminum rod containing two vertical bars.
  • a 23G needle is placed in between the radius and ulna to serve as a guide pin.
  • the blunt guillotine is then positioned, and a 850 gm weight raised to 45 cm and allowed to fall to create the fracture.
  • Poly(lactide)/poly(ethylene glycol) gels Low molecular weight (2000) PLA dissolved in PEG produces a syringeable solution that precipitates PLA upon injection into an aqueous environment, resulting in a relatively firm gel. Two different percentages were tested. 4. Poly(lactic acid)-poly(ethylene glycol) conjugates. Each material was implanted with 0, 10, and 80 ⁇ g rhBMP-2. Lyophilized rhBMP-2 was mixed with the gels using a mortar and pestle. The buffer, Pluronic gels, and PEG/PLA gels were first injected into blood clots. The PLA-PEG conjugates were implanted directly into the subcutaneous space. Six implants (three animals) were used per group. In addition, the intramuscular injection technique was investigated using the PLA/PEG gel and one Pluronic gel (both at the high dose only).
  • Bone score is a semi-quantitative measurement of the area of bone present in representative histological sections; the score ranges from 0 for no bone present, to 5 when the entire section consists of bone.
  • the Pluronics produced relatively little bone at the lower dose of rhBMP-2, and induced none when placed intramuscularly. Presumably the material does not have a long enough residence time, or does not sequester rhBMP-2 sufficiently. In addition, a significant inflammatory response was noted.
  • the PLA/PEG gels produced reasonable quantities of bone, with some residual matrix observed (presumably the precipitated PLA) along with a foreign body giant cell response.
  • the PLA-PEG conjugates produced well-defined ossicles of bone with bone marrow. Of the gels tested, this material performed best. Based on the samples tested, the intramuscular implantation appeared to be a more rigorous test of materials. In this experiment, rhBMP-2 in buffer simply injected into blood clot performed the best overall; presumably the rhBMP-2 is able to rapidly distribute and bind to the blood clot.
  • Various collagen materials tested include 2% LLS dispersion, 2% HeliteneTM dispersion, 2% Helistat® dispersion, the Zimmer collagen gel, and another collagen gel (6.5%) from Matrix Pharmaceuticals. All have been placed at 0, 20, and 80 ⁇ g rhBMP-2 and analyzed histologically.
  • BMP-2 may accelerate the consolidation (bone formation or mineralization) phase in a rabbit model of limb lengthening. Osteotomies are created in rabbit tibia.
  • the tibia are then be distracted 2 cm over a period of approximately ten days. Following the distraction phase, rhBMP-2 is administered. Two modes of application are tested. One set of animals has rhBMP-2/ACS (1.5 mg/mL; 0.075 mg/tibia) surgically placed within the regenerate. The second group of animals has rhBMP-2/MFR842 buffer (0.75 mg/mL; 0.075 mg/tibia) percutaneously injected into three sites within the regenerate. A third group of control animals has surgical intervention similar to the rhBMP-2/ACS-treated animals, with placement of ACS/buffer within the regenerate. Additional sets of animals have distraction performed, with no surgical intervention. Groups of animals are sacrificed at 5, 14 and 24 days. Radiographs are taken following the distraction phase and at sacrifice and are used to evaluate new bone formation in response to treatment and control.
  • Bone density within the defect is determined with Dual Energy X-Ray Absorptiometry and Peripheral Quantitative Computed Tomography (pQCT).
  • pQCT Peripheral Quantitative Computed Tomography
  • the three dimensional distribution of bone within the defect is evaluated with pQCT. Histological evaluation of non-decalcified specimens is used to quantify histomorphometric parameters. Results to date indicate a visually detectable acceleration of bone induction in rhBMP-2/ ACS treated animals compared to untreated surgical controls at 5 days and 14 days based on radiographic evaluation.
  • the DXA and pQCT images confirm these findings.
  • the pQCT images indicate greater three-dimensional distribution of bone within the regenerate and evidence of early stages of corticalization in the rhBMP-2/ACS treated animals at 14 days.
  • rhBMP-2/ ACS treatment effect of significant acceleration of the consolidation phase of distraction osteogenesis. Formation of an intact cortex is the primary indicator for removal of the external fixator and associated return to unprotected full weight bearing.
  • the rhBMP-2/MFR842 injection buffer treatment is the preferred route of administration having more wide spread application in primary distraction osteogenesis.

Abstract

Methods and compositions are provided for the treatment of defects and disease involving osteoporosis, or osteopenic conditions. The methods comprise applying to the site of osteoporotic or osteopenic conditions a composition comprising an active agent, preferably from the TGF-β superfamily of proteins. The advantages of the invention include a reduction or avoidance of the severity and/or incidence of bone fractures. Also, the methods of the present invention are advantageous in that administration is local, rather than systemic.

Description

INJECT ABLE FORMULATIONS FOR TREATMENT OF OSTEOPOROTIC BONE
FIELD OF THE INVENTION The present invention relates to the field of tissue repair, specifically, to the treatment of osteoporotic bone and/or prevention of osteoporosis. Osteoporotic or osteopenic bone is often characterized by suboptimal bone density. The osteoporotic condition may be related to diet, trauma or stress, or to degenerative or congenital disease. Thus, the present invention may be useful in the treatment and/or the prevention of osteoporosis, or the treatment of osteoporotic or osteopenic bone.
BACKGROUND OF THE INVENTION Background of the incidence and etiology of need: Idiopathic osteoporosis is a disease of unknown etiology characterized by progressive loss of bone mass and increased fragility. It is a medical problem because it is associated with a marked increase in susceptibility to fractures. It is a public health problem for several reasons.
First, it is among the most prevalent of all musculoskeletal disorders. Fifty-six percent of women over 45 years of age are afflicted. Praemer et ah, Musculoskeletal Conditions in the United States, American Academy of Orthopaedic Surgeons, Park Ridge, IL (1992). Second, its incidence increases with age. Because the percentage of elderly in the population is increasing, osteoporosis will become more common with time. Third, osteoporosis presently has no known cure, and is difficult to treat locally. Fourth, it is a major economic burden to individuals and to society. Fifth, and most significantly, osteoporosis is associated with a substantial morbidity and mortality. The most serious fracture resulting from osteoporosis is that the of the proximal femur in the region of the hip joint. With an annual incidence of 250,000, hip fractures are currently the most common fracture in the elderly. Praemer et ai, Ibid. Estimates based on census projections indicate that this figure will increase to approximately 340,000 hip fractures per year by the year 2000. One out of every six Caucasian women will have a hip fracture during her lifetime (Cummings et al, Arch Intern Med 49:2455-2458 (1989), and for those who attain the age of 90, this figure becomes one in three. Of the patients who are independent and living at home at the time of hip fracture, approximately 20 percent remain in a long term care institution for at least one year following the fracture. During the first year following injury, the mortality rate is approximately 15% higher than for age and gender matched controls. Praemer et al., Ibid. The financial toll of these fractures is also high. In 1988, hip fractures cost the United States 8.7 billion dollars. Praemer et al., Ibid. The increased incidence of proximal femur fracture observed in elderly patients is mainly related to two factors: (1) a decreased bone density of their proximal femora; (2) an increased propensity to fall. There is an inverse relationship between the age-related bone loss in the proximal femur and the risk of hip fracture. Each decrease of one standard deviation (SD) in femoral neck bone density increases the age-adjusted risk of hip fracture 2.6 times (95% CI 1.9 - 3.6); and (3) women with bone density in the lowest quartile have an 8.5-fold greater risk of hip fracture than those in the highest quartile. Cummings et al., The Lancet 341:12-15 (1993). This relation between hip bone mass and hip fracture risk allows the screening and identification of patients at risk for fracture. Patients who are two standard deviations below peak hip bone mass have passed beneath the "fracture threshold."
Bioactive agents that reduce the incidence of hip fractures or augment the healing of such fractures when they occur would substantially improve the health of the elderly. The availability of an injectable agent would permit its use in fracture prevention, such as hip fracture, without the costs and morbidity of surgical intervention, such as for femoral neck fractures. Such an agent would have application in fracture treatment, without increasing the extent or complexity of the surgical management. The inventors have provided a novel method using bioactive agents to decrease the occurrence and/or severity of fractures to osteoporotic bone, such as an osteoporotic hip.
While several therapies for osteoporosis have been approved, there is none that addresses the localized treatment of proximal femur osteoporosis. Current therapies for osteoporosis are systemic. These include fluoride, bisphosphonates, calcitonin, estrogens and progestins, testosterone, vitamin D metabolites, and/or calcium. In the United States, only estrogens and alendronate, a bisphosphonate, are indicated for the prevention of hip fractures in postmenopausal osteoporotic women. Each of these agents requires continuous administration over a time period of years. Estrogen has undesirable side effects (WHO Study Group on Assessment of Fracture Risk and its Application to Screening for Postmenopausal Osteoporosis. WHO Technical Report Series 843, Assessment of fracture risk and its application to screening for postmenopausal osteoporosis. Geneva, World Health Organization (1992)), compliance is poor, and it is not indicated in males. Alendronate requires carefully separated administration of the drug and sources of calcium and is not recommended in patients with reduced renal function. A recent study found a reduction in hip fractures in elderly women with involutional osteoporosis after eighteen months of vitamin D and calcium (Chapuy et al. New Engl J. Med. 327:1637-1642 (1992)), but this treatment has not been conformed by independent sources, and lacks United States regulatory approval. While several treatments have effectively arrested or decreased bone loss, only the use of fluoride has been associated with rapid increases in bone density. However, fluoride treatment increased bone density less in the femoral region as compared to the spine and was associated with poor bone quality.
Hedlund et al., J. Bone Min. Res. 4:223-225 (1989). Fluoride treatment again has not received regulatory approval. Thus, no safe, effective, generally applicable local treatment is available which protects against the occurrence of hip fractures in osteoporosis by providing a reliable and durable increase in hip bone mass. Accordingly, despite substantial endeavors in this field, there remains a need for an effective method of repair and/or treatment of osteoporotic and osteopenic bone, and for treatment and/or prevention of osteoporosis.
SUMMARY OF THE INVENTION Accordingly, the present invention provides methods and compositions for increasing bone mass and quality, and for minimizing or reducing the incidence or severity of osteoporosis-related fractures. Accordingly, the present invention provides methods and compositions useful for decreasing the incidence of fractures of osteoporotic or osteopenic bone. In particular, the present invention comprises methods of treating patients with osteoporosis, or with other evidence of osteoporosis or osteopenic condition. Preferred embodiments where the present invention may prove particularly useful include treatment of metaphyseal bone, including proximal femur (hip), proximal humerus (upper arm), distal radius (wrist), and vertebral bodies (spine), particularly the vertebral body.
- The method comprises administering to a site of osteopenic or osteoporotic bone, or a site of low bone mass or density, an effective amount of a composition comprising at least one active agent which is capable of inducing growth of bone or increasing the formation of bone tissue or reducing bone loss at the site. Bone mass is commonly designated "bone mineral content" or BMC and is measured in grams. Bone density is commonly designated "bone mineral density" or BMD and is expressed as grams per unit area or grams per unit volume. In a preferred embodiment, the mode of administration is by intraosseous injection. In preferred embodiments, the active agent is one or more proteins selected from the group of proteins known as the Transforming Growth Factors-Beta (TGF-β) superfamily of proteins, preferably selected from the Bone Morphogenetic Proteins (BMPs), the Growth and Differentiation Factors (GDFs), as well as other proteins, as described more fully herein. The methods and compositions of the present invention are advantageous in that they provide a localized treatment for osteoporosis or osteopenic bone, rather than systemic treatment. The present invention is further advantageous in that it utilizes as active agents osteogenic proteins, which may be produced via recombinant DNA technology, and therefore are of potentially unlimited supply. The methods and compositions of the present invention are further advantageous in that regeneration of the bone tissue increases the bone mass/density, increase the bone strength, and thereby reduce the severity of osteoporosis or incidence of osteoporotic lesions, ultimately lessening the incidence of bone fractures. In a preferred embodiment of the present invention, the active agents are administered locally through injection using a suitable buffer and/or carrier. One suitable buffer comprises glycine, sucrose, and glutamic acid hydrochloride, at a pH of less than 6.0. In a preferred embodiment of the invention, this formulation comprises about 2.5% glycine (g/100 ml (w/v)), about 0.5% sucrose (w/v), about 5 mM glutamic acid hydrochloride (about 0.1% w/v), and about 0.01 % (w/v) polysorbate 80, at a pH of about 4.5. This buffer is referred to later in this application as "MFR 842." Further buffers suitable for use in the present invention are described in United State Patent 5,385,887, the disclosure of which is hereby incorporated by reference. Suitable carriers include collagen gels, hyaluronate, alginates and hyaluronic acids, injectable calcium phosphates, polyols, demineralized bone matrix and combinations of the above. Other carriers which may be useful for the present invention include blood as well as clotting proteins, such as fibrin or thrombin, and oils.
In other preferred embodiments, the active agent further comprises, in addition to one or more proteins selected from the TGF-β superfamily of proteins, one or more auxiliary proteins, such as Hedgehog, Noggin, Chordin, Frazzled, Cerberus and
Follistatin, soluble BMP receptors, or other protein or agent, as described further herein.
In addition to healing of osteoporotic bone, compositions of the present invention may be useful for injectable formulations of BMPs for uses such as injection into joints for treatment and repair of osseous defects, cartilage defects, inhibition of cartilage degradation and to promote cartilage repair. The formulations may also be injected into tendons, ligaments and/or their attachment sites to bone. Injectable formulations of BMPs may also find application to other bone sites such as bone cysts, implants into bones, closed fractures and distraction osteogenesis.
DETAILED DESCRIPTION OF THE INVENTION According to the present invention, methods and compositions are provided for treatment of patients who exhibit signs of osteoporosis, or osteopenic conditions, including osteoporotic bone lesions. The identification of such patients may be accomplished by procedures which are well known in the art. These procedures include measurement of bone mass/density using dual-energy X-ray absorptiometry (DEXA), Kilgus et al., J. Bone & Joint Surgery. 75-B:279-287 (1992); Markel et al., Acta Orthop Scand, 61:487-498 (1990); and quantitative computed tomography (QCT), Laval-Jeantet et al., J Comput Assist Tomogr. 17:915-921 (1993); Markel, Calcif Tissue Int. 49:427-432 (1991); single-photon absorptiometry, Markel et al. Calcif Tissue Int, 48 : 392-399 ( 1991 ) ; ultrasound transmission velocity (UTV) ; Heaney et al., JAMA, 261:2986-2990 (1989); Langton et al., Clin Phvs Phvsiol Meas, 11:243- 249 (1990); and radiographic assessment, Gluer et al., J Bone & Mineral Res, 9:671- 677 ( 1994) . Other methods of identification of patients at risk of bone fracture include assessment of age-related factors, such as cognisance, as well as prior occurrence of osteoporosis-related fractures. Porter et al., BMJ, 301: 638-641 (1990); Hui et al., J
Clin Invest, 81: 1804-1809 (1988). The above publications are hereby incorporated by reference herein.
The methods comprise applying to the osteoporotic or osteopenic site an amount of a composition comprising one or more purified osteogenic proteins which is effective to induce the formation and/or maintenance of bone.
ACTIVE AGENT
The active agent is preferably selected from the family of proteins known as the transforming growth factors-beta (TGF-β) superfamily of proteins, which includes the activins, inhibins and bone morphogenetic proteins (BMPs). Most preferably, the active agent includes at least one protein selected from the subclass of proteins known generally as BMPs, which have been disclosed to have osteogenic activity, and other growth and differentiation type activities. These BMPs include BMP proteins BMP-2, BMP-3, BMP-4, BMP-5, BMP-6 and BMP-7, disclosed for instance in United States Patents 5,108,922; 5,013,649; 5,116,738; 5,106,748; 5,187,076; and 5,141,905; BMP-
8, disclosed in PCT publication WO91/18098; and BMP-9, disclosed in PCT publication WO93/00432, BMP- 10, disclosed in PCT application WO94/26893; BMP-11, disclosed in PCT application' WO94/26892, or BMP-12 or BMP-13, disclosed in PCT application WO 95/16035; BMP-15,BMP-15, disclosed in United States Patent 5,635,372; or BMP- 16, disclosed in co-pending patent application, serial no. 08/715,202, filed on September 18, 1996. Other TGF-β proteins which may be useful as the active agent in the present invention include Vgr-2, Jones et al., Mol. Endocrinol., 6: 1961-1968 (1992), and any of the growth and differentiation factors [GDFs], including those described in PCT applications WO94/15965; WO94/15949; WO95/01801; WO95/01802; WO94/21681 ; WO94/15966; WO95/10539; WO96/01845; WO96/02559 and others. Also useful in the present invention may be
BIP, disclosed in WO94/01557; HP00269, disclosed in JP Publication number: 7-250688; and MP52, disclosed in PCT application WO93/16099. The disclosures of all of the above applications are hereby incorporated by reference. A subset of BMPs which are presently preferred for use in the present invention include BMP-2, BMP-4, BMP-5, BMP-6, BMP-7, BMP- 10, BMP-12 and BMP- 13. The active agent is most preferably BMP-2, the sequence of which is disclosed in United States Patent 5,013,649, the disclosure of which is hereby incorporated by reference. Other BMPs and TGF-β proteins known in the art can also be used.
The active agent may be recombinantly produced, or purified from a protein composition. The active agent, if a TGF-β such as a BMP, or other dimeric protein, may be homodimeric, or may be heterodimeric with other BMPs (e.g., a heterodimer composed of one monomer each of BMP-2 and BMP-6) or with other members of the TGF-β superfamily, such as activins, inhibins and TGF-β 1 (e.g., a heterodimer composed of one monomer each of a BMP and a related member of the TGF-β superfamily). Examples of such heterodimeric proteins are described for example in
Published PCT Patent Application WO 93/09229, the specification of which is hereby incorporated herein by reference.
The active agent may further comprise additional agents such as the Hedgehog, Frazzled, Chordin, Noggin, Cerberus and Follistatin proteins. These families of proteins are generally described in Sasai et al., Cell, 79:779-790 (1994) (Chordin);
PCT Patent Publication WO94/05800 (Noggin); and Fukui et al., Developmental Biology, 159: 131-139 (1993) (Follistatin). Hedgehog proteins are described in WO96/16668; WO96/17924; and WO95/18856. The Frazzled family of proteins is a recently discovered family of proteins with high homology to the extracellular binding domain of the receptor protein family known as Frizzled. The Frizzled family of genes and proteins is described in Wang et al., J. Biol. Chem., 271:4468-4476 (1996). The active agent may also include other soluble receptors, such as the truncated soluble receptors disclosed in PCT patent publication WO95/07982. From the teaching of WO95/07982, one skilled in the art will recognize that truncated soluble receptors can be prepared for numerous other receptor proteins. Such would also be encompassed within the present invention. The above publications are hereby incorporated by reference herein.
The amount of active agent useful herein is that amount effective to stimulate increased osteogenic activity of present or infiltrating progenitor or other cells, and will depend upon the size and nature of the defect being treated, as well as the carrier being employed. Generally, the amount of protein to be delivered is in a range of from about 0.1 to about 100 mg; preferably about 1 to about 100 mg; most preferably about 10 to about 80 mg.
CARRIER Materials which may be useful as the carrier in practicing the present invention include pharmaceutically acceptable materials having viscosity and polarity such that, when added to the bone morphogenetic protein, form a composition that possesses appropriate handling characteristics for injectable application to the site of osteoporotic or osteopenic bone. Adding the carrier to the bone morphogenetic protein allows the protein to remain in the diseased or lesioned site for a time sufficient to allow the protein to increase the otherwise natural rate of regenerative osteogenic activity of the infiltrating mammalian progenitor or other cells, and to form a space in which new tissue can grow and allow for ingrowth of cells. The carrier may also allow the bone morphogenetic protein to be released from the disease or lesion site over a time interval appropriate for optimally increasing the rate of regenerative osteogenic activity of the progenitor cells. The carrier may also supply a framework on which to induce new formation in severely osteoporotic bone.
The most preferred family of carriers comprises collagenous materials. These are preferably in a form suitable for injection, such as a gel. Such gels may be cross- linked or non-cross-linked. Other forms of collagen, such as dispersions or fibrillar collagen, may also be useful in the methods of the present invention. Another preferred family of carriers is cellulosic materials such as alkylcellulose, including hydroxyalkylcellulose, methylcellulose, ethylcellulose, hydroxyethylcellulose, hydroxypropylcellulose, hydroxypropylmethylcellulose, and carboxymethylcellulose, the most preferred being the cationic salts of carboxymethylcellulose (CMC). In the case of cellulosic carriers and collagen gels, it is preferred that the carrier be in the form of a hydrated cellulosic viscous gel. Viscosity may be increased through mechanical means, such as high agitation for a suitable period of time, followed by autoclaving, or chemically. The active agent and cellulosic carrier is preferably in a solution of suitable buffer. One preferred buffer solution is a composition comprising, in addition to the active agent, about 1.0 to about 10.0%
(w/v) glycine, about 0.1 to about 5.0% (w/v) of a sugar, preferably sucrose, about 1 to about 20 mM glutamic acid hydrochloride, and optionally about 0.01 to about 0.1% of a non-ionic surfactant, such as polysorbate 80. Preferred solutions are from about 1 % to about 20% w/v cellulosic carrier/buffer. If desired, a salt may be added. A preferred viscous gel carrier is described in Example 2 below. The amount of osteogenic protein useful with viscous gel carrier is generally in a range of from about 0.1 to about 100 mg, preferably about 1 to about 100 mg; most preferably about 10 to about 80 mg per cubic centimeter of implant material required.
Another class of materials of particular interest for injectable carriers are resorbable hydroxyapatites as well as minerals, ceramics and phosphates. Resorbable hydroxyapatites, for example, can be formulated at various porosities with varying resorption rates; their handling characteristics vary from hard implantable types, to gel-like consistency, to those that are injectable but harden at body temperature. Suitable hydroxyapatite and ceramic carriers are described, for example in WO96/36562; and United States Patents 5,543,019; 5,306,305; 5,258,044; 5,496,399;
5,455,231; 5,336,264; 5,178,845; 5,053,212; 5,047,031; 5,129,905; 5,034,059; 4,880,610; 5,290,763; and 5,563,124; the disclosures of which are incorporated herein by reference.
Another preferred family of carriers for administration of the active agent of the present invention are injectable polymers, which may be viscous and which may optionally include a sequestering agent as well. Suitable polymers and sequestering agents include those described in United States Patent 5,171,579, the entire disclosure of which is incorporated herein by reference. Other polymers include the pluronics, such as Poloxamer 407 gel. Pluronics are a class of water soluble ABA type block surfactant copolymers which exhibit the unique property of reverse thermal gelation. They are liquid (and hence syringeable) at 4°C and gel at body temperature.
Poloxamer 407, MW 12,500, is excreted unchanged in the urine after systemic absorption and has supposedly been shown to be non-toxic in animals. Polylactides and/or polyethylene glycols, including poly(lactide)/poly(ethylene glycol) gels. Polylactides may be dissolved in polyethylene glycols, such as low molecular weight (2000) PLA dissolved in PEG to produce a syringeable solution that precipitates PLA upon injection into an aqueous environment, resulting in a relatively firm gel. In addition, the literature cites conjugates, such as Poly(lactic acid)-poly(ethylene glycol) conjugates, as appropriate carriers for BMPs (Miyamoto et al., Clin. Orthop. Rel. Res. 294:333 (1993)). Also useful as the carriers are fibrin-based polymers, in liquid or gel form. Among the materials useful as sequestering agents are hyaluronic acid, sodium alginate, poly(ethylene glycol), polyoxyethylene oxide, carboxyvinyl polymer and poly( vinyl alcohol), and cellulosic materials, such as hydroxycelluloses. One such preferred agent is carboxymethylcellulose.
The above materials disclosed to be useful as sequestering agents may themselves be useful as carriers for injection. In addition, combinations of the above described materials may be used.
It is also possible to use as injectable carriers solid materials which are narrow enough to be administered through injection. In such cases, the solid material may be combined with a viscous liquid carrier for ease and uniformity of administration. In cases where the carrier may be of higher viscosity than optimal, the carrier may optionally be combined with a diluent, such as aqueous glycerol, preferably the carrier diluent would be present in concentrations of about 10 to about 80% (v/v). Also, the above materials may be combined in particular embodiments of the present invention. For example, polymers, such as porous particulate polymers, may be dissolved or suspended in cellulosic or gel carriers to increase viscosity.
In a preferred embodiment of the present invention, the active agents are administered locally through injection using only a suitable buffer as carrier. One suitable buffer comprises glycine, sucrose, and glutamic acid hydrochloride, at a pH of less than 6.0. Preferred compositions of buffer solutions comprise about 1.0 to about 10.0% (w/v) glycine, about 0.1 to about 5.0% (w/v) of a sugar, preferably sucrose, about 1 to about 20 mM glutamine, glutamic acid, or glutamic acid hydrochloride, and optionally about 0.01 to about 0.1 % of a non-ionic surfactant, such as polysorbate 80. In a preferred embodiment of the invention, this formulation comprises about 2.5% glycine (g/100 ml (w/v)), about 0.5% sucrose (w/v), about 5 mM glutamic acid hydrochloride (about 0.1% w/v), and about 0.01% (w/v) polysorbate 80, at a pH of about 4.5. This buffer has been described as MFR 842.
Further buffers suitable for use in the present invention are described in United State Patent 5,385,887, the disclosure of which is hereby incorporated by reference. Preferred solutions may also include combinations of buffer and other carrier, such as a combination of buffer and cellulosic carrier. Preferred ranges for this combination are from about 1% to about 20% w/v cellulosic carrier/buffer. If desired, a salt may be added.
MODE OF ADMINISTRATION The injectable compositions of the present invention may be administered in any clinically acceptable manner of injection. A number of commercially available syringes may be suitable for use in the present invention, and for administration of the compositions of the present invention. For example, suitable syringes are available the CalaseptR syringe [JS Dental Manufacturing, Ridgefield CT] comprises sterile calcium hydroxide paste in isotonic saline solution, in a non-aspirating or modified aspirating cartridge syringe; Henke-Ject Aspirating Syringe and Hypo Brand Dental Syringes/Needles [Smith & Nephew MPL, Franklin Park, LL]; intraosseous needles from MPL, Inc., Chicago LL; and Luer-LokR Syringes [Becton Dickinson, Franklin Lakes, NJ], may all be appropriate syringes for use in the present invention.
In another embodiment of the present invention, bone morphogenetic proteins are used as an osteoinductive agent in the process known as distraction osteogensis. This process is an alternative to segmental bone regeneration in response to implanted osteoinductive agents. In traditional segmental bone repair, the osteoinductive agent and carrier are placed in the defect created between the parent bone ends. For bone formation to occur, the osteoinductive agent has to have sufficient residence time in the defect to stimulate differentiation of sufficient numbers of bone forming cells to support new bone formation. The carrier also has to have sufficient residence time to serve as a scaffold for bone forming cells to attach (osteoconduction). In addition, the carrier also has to have sufficient porosity to allow cells and blood vessels to penetrate into the defect for bone formation to occur. In contrast, the process of distraction osteogenesis creates a regenerate construct between the distracted parent bone ends that is highly vascular and contains a large population of mesenchymal stem cells destined to become bone forming cells. As a result, the regenerate construct represents a much more ideal environment for cell differentiation growth factors such rhBMP-2 to stimulate rapid bone induction relative to induction of bone within a segmental defect.
The process of distraction osteogenesis begins with an initial latency period allowing a fibrous connection to form between the bone ends to be distracted.
Following this latency period, the bone ends are slowly distracted at a controlled rate of up to 1 mm per day in human clinical cases. Once the regenerate forms and the bone ends are distracted to the appropriate length, a prolonged consolidation period is required to allow the regenerate to form bone. This prolonged consolidation period which can be on the order 4 to 6 months is associated with considerable morbidity.
A frequent complication is the occurrence of pin track infections resulting from the extended length of time the external fixator used to generate the distraction must remain in place. In addition, there are considerable psychological effects and life style alterations associated with wearing the external fixator for prolonged periods of time. In addition to complications associated with the external fixator, there are a number of patients where the regenerate does not form properly and a delayed union or non-union occurs. Since the regenerate contains a responsive cell population and is already highly vascularized following the initial distraction phase, the use of bone morphogenetic proteins may rapidly accelerate the rate of bone formation during the normally prolonged consolidation phase of distraction osteogenesis. Acceleration of the distraction phase is limited by stretching of the soft tissues associated with bone. The cells created using distraction osteogenesis may also be harvested in order to provide a source of cells which are primed for osteogenesis. These cells can be cultured to prepare immortalized cell lines. If desired, these cells can also be immunotolerized using agents such as CTLA4 receptors [U.S. Patent 5,434,131] or CTLA4 ligands or B7 monoclonal antibodies [WO 96/40915]. Methods and materials for such immunotolerization are disclosed in the above references, and include co- transfection or treatment with these factors. The disclosure of these references is hereby incorporated herein by reference.
The following examples further describe the practice of embodiments of the invention with rhBMP-2 in a buffer carrier. The examples are not limiting, and as will be appreciated by those skilled in the art, can be varied in accordance with the above specification.
EXAMPLES Example 1: Oophorectomized Rat Model:
The oophorectomized rat is a well-established model of osteoporosis and its use is recommended by the FDA as one of the animal models to be employed in demonstrating efficacy of potential therapeutic agents for osteoporosis. Preclinical studies testing the efficacy of rhBMP-2 in the oophorectomized rat model of osteoporosis demonstrated that 100 Mg rhBMP-2 in MFR 842 buffer, injected into the intramedullary space of the tibial shaft, was associated with extensive bone formation. Further evaluation with this model is conducted at lower doses.
In a similar study, five orariectomized rats were injected with 40 ug of rhBMP- 2 in MFR 842 buffer solution into one side of the femoral neck, and MFR 842 buffer alone on the other side. After six weeks, the femora are harvested, analyzed by DEXA for bone density and by histology.
In a larger study, six weeks after ovariectomy, rat tibiae are injected with 0, 10, or 50 Mg of rhBMP-2 in 20 ML MFR 842 buffer. Controls include sham ovariectomized animals [surgery performed, but ovaries are not removed], buffer injections and sham surgeries. After six weeks, the femora are harvested and groups analyzed by DEXA, biomechanics, and histornorphometry.
Example 2. Sheep Core Decompression Model
Preclinical studies in support of the application of rhBMP-2 to the treatment of osteonecrosis of the hip at the time of core decompression demonstrated that rhBMP-2 stimulates bone formation in the core decompression track within the femoral neck of normal (non-osteoporotic) sheep. In this study, defects in both the femoral head/neck and distal femur were created, the latter to facilitate DEXA imaging. rhBMP-2 in various formulations, including buffer, blood, blood clot and collagen dispersions was placed at the site of defect. Example 3. Human Core Decompression Study.
Patients with osteonecrosis of the femoral head were treated by core decompression with or without implantation of blood clot containing rhBMP-2 into the core track. Patients who received rhBMP-2 experienced a reduction in the volume of necrotic bone compared to patients treated by core decompression alone. The treatment was well tolerated with complications limited to some bone formation adjacent to the cortical entry site. Example 4. Biodistribution of rhBMP-2.
Four aged ewes underwent surgical placement of a cannulated needle into the femoral neck using uniplanar fluoroscopic guidance. A bolus injection of radiolabelled rhBMP-2 in buffer solution was delivered through the needle into the proximal femur. Local (bone) distribution of rhBMP-2 was monitored by gamma camera. Systemic distribution was assessed by periodic serum sampling. In vivo gamma camera images of the femur indicate that the injected rhBMP-2 enters the femoral head and neck and that part of the injected material is retained at these sites for at least 72 hours. Serum analysis of radiolabelled rhBMP-2 indicates that the majority (-85%) of the rhBMP-2 enters the systemic circulation within five minutes of administration. Example 5. Intra-Femoral Injections.
Patients with osteoporosis who have sustained a fracture of the proximal femur are identified. Intraosseous administration of injectable rhBMP-2 is accomplished in the non-fractured (contralateral) femur using an operating room, biplanar fluoroscopy, and patient positioning on a fracture table. Each patient undergoes the necessary surgical treatment of the fractured femur. At the completion of surgical procedure, but before termination of the anesthesia, the lower extremities are repositioned on the fracture table to gain access to the uninjured contralateral hip. Under sterile conditions and biplanar image intensifier visualization, the designated dose of rhBMP-
2 is delivered by percutaneous, intraosseous route into the proximal femur. Follow-up evaluations include radiographic assessment, clinical evaluation of infection and fracture, and DEXA evidence of bone formation. Example 6: Rabbit Ulnar Osteotomy and Fracture Models. In the osteotomy model, the ulna is simply exposed, the periosteum is stripped, and a 2 to 5 mm osteotomy created using an oscillating saw. The incision is then closed, and the appendage bandaged to provide additional stability. Bilateral surgeries may be used in order to compare active agent against untreated or control substances.
The rabbit ulnar fracture model is similar to the rat femoral fracture model. The rabbit ulnar fracture model relies on a weight-driven blunt instrument to create the fracture essentially using incident three-point bending. The fracture is created by fully extending and clamping the forelimb to an aluminum rod containing two vertical bars. In a modification from the rat apparatus, a 23G needle is placed in between the radius and ulna to serve as a guide pin. The blunt guillotine is then positioned, and a 850 gm weight raised to 45 cm and allowed to fall to create the fracture.
Assessment of efficacy in both the rat femoral and rabbit ulnar fracture models can be accomplished primarily using biomechanics. Qualitative measures of fracture repair, such as radiology, can be obtained, but it is difficult to see subtle differences over normal fracture repair, and will not give a convincing demonstration that the injection is translating to accelerated fracture repair.
Example 7: Rat Ectopic Implant Models
In one experiment, several non-collagenous materials were tested in the rat ectopic implant model. The materials included in this study were: 1. MFR 842 buffer; 2. Poloxamer 407 gel.
3. Poly(lactide)/poly(ethylene glycol) gels. Low molecular weight (2000) PLA dissolved in PEG produces a syringeable solution that precipitates PLA upon injection into an aqueous environment, resulting in a relatively firm gel. Two different percentages were tested. 4. Poly(lactic acid)-poly(ethylene glycol) conjugates. Each material was implanted with 0, 10, and 80 μg rhBMP-2. Lyophilized rhBMP-2 was mixed with the gels using a mortar and pestle. The buffer, Pluronic gels, and PEG/PLA gels were first injected into blood clots. The PLA-PEG conjugates were implanted directly into the subcutaneous space. Six implants (three animals) were used per group. In addition, the intramuscular injection technique was investigated using the PLA/PEG gel and one Pluronic gel (both at the high dose only).
The above were scored for bone formation. Bone score is a semi-quantitative measurement of the area of bone present in representative histological sections; the score ranges from 0 for no bone present, to 5 when the entire section consists of bone.
Coupled with the wet weights and qualitative histological assessment of the sections, the following conclusions can be made. The Pluronics produced relatively little bone at the lower dose of rhBMP-2, and induced none when placed intramuscularly. Presumably the material does not have a long enough residence time, or does not sequester rhBMP-2 sufficiently. In addition, a significant inflammatory response was noted. The PLA/PEG gels produced reasonable quantities of bone, with some residual matrix observed (presumably the precipitated PLA) along with a foreign body giant cell response. The PLA-PEG conjugates produced well-defined ossicles of bone with bone marrow. Of the gels tested, this material performed best. Based on the samples tested, the intramuscular implantation appeared to be a more rigorous test of materials. In this experiment, rhBMP-2 in buffer simply injected into blood clot performed the best overall; presumably the rhBMP-2 is able to rapidly distribute and bind to the blood clot.
In another rat ectopic study, several cross-linked and non-cross-linked collagen materials were tested. In addition, porosity was introduced into the PLA/PEG gels by the addition of MFR 842 buffer as an excipient, and a lower percentage of PLA was tested. Some of the collagen materials were tested in an aqueous (MFR 842) or non- aqueous (PLA/PEG gel) environment. The collagen materials tested included:
1. Homogenized Helistat® bovine type I collagen cross-linked hemostatic sponge (currently in use with rhBMP-2 clinically) made into a suspension;
2. Homogenized Helitene™ (fibrillar form). Only tested with PLA/PEG in this experiment; 3. Collagen dispersion (Integra LifeSciences, Plainsboro, NJ). The non-cross- linked parent material of Helistat©. At the concentration tested (0.78%, as provided), it is not viscous at all.
4. Zimmer collagen gel. The collagen component of the Collagraft® kit. All materials were tested with 10 μg rhBMP-2 using the blood clot injection method. The samples were scored for histologic bone formation. The materials which performed best in this study were the Helistat® dispersion and the collagen gel, yielding bone scores of 3 to 4, and no adverse tissue reaction. All PLA/PEG containing materials showed much smaller amounts of bone, and significant inflammatory response (non-specific foreign body type). Addition of PLA/PEG to the collagen material descreased the bone formation observed. In this experiment, the rhBMP-2 in buffer placed in blood clot perform poorly; this may be because a larger gauge needle was used to place the material, and it flowed back along the needle track before it could distribute in the blood clot. Likewise, the ILS dispersion performed poorly, perhaps due to low viscosity. These results indicate relatively little promise for the PLA/PEG gels, unless use of very low molecular weight PLA accelerates its resorption time. The collagen materials stand out above the other materials tested to date using this rat ectopic assay system.
Various collagen materials tested include 2% LLS dispersion, 2% Helitene™ dispersion, 2% Helistat® dispersion, the Zimmer collagen gel, and another collagen gel (6.5%) from Matrix Pharmaceuticals. All have been placed at 0, 20, and 80 μg rhBMP-2 and analyzed histologically.
Example 8: Distraction Osteogenesis
BMP-2 may accelerate the consolidation (bone formation or mineralization) phase in a rabbit model of limb lengthening. Osteotomies are created in rabbit tibia.
The tibia are then be distracted 2 cm over a period of approximately ten days. Following the distraction phase, rhBMP-2 is administered. Two modes of application are tested. One set of animals has rhBMP-2/ACS (1.5 mg/mL; 0.075 mg/tibia) surgically placed within the regenerate. The second group of animals has rhBMP-2/MFR842 buffer (0.75 mg/mL; 0.075 mg/tibia) percutaneously injected into three sites within the regenerate. A third group of control animals has surgical intervention similar to the rhBMP-2/ACS-treated animals, with placement of ACS/buffer within the regenerate. Additional sets of animals have distraction performed, with no surgical intervention. Groups of animals are sacrificed at 5, 14 and 24 days. Radiographs are taken following the distraction phase and at sacrifice and are used to evaluate new bone formation in response to treatment and control.
Bone density within the defect is determined with Dual Energy X-Ray Absorptiometry and Peripheral Quantitative Computed Tomography (pQCT). The three dimensional distribution of bone within the defect is evaluated with pQCT. Histological evaluation of non-decalcified specimens is used to quantify histomorphometric parameters. Results to date indicate a visually detectable acceleration of bone induction in rhBMP-2/ ACS treated animals compared to untreated surgical controls at 5 days and 14 days based on radiographic evaluation. The DXA and pQCT images confirm these findings. In addition the pQCT images indicate greater three-dimensional distribution of bone within the regenerate and evidence of early stages of corticalization in the rhBMP-2/ACS treated animals at 14 days. Further results may support the rhBMP-2/ ACS treatment effect of significant acceleration of the consolidation phase of distraction osteogenesis. Formation of an intact cortex is the primary indicator for removal of the external fixator and associated return to unprotected full weight bearing. The rhBMP-2/MFR842 injection buffer treatment is the preferred route of administration having more wide spread application in primary distraction osteogenesis.

Claims

CLAIMSWe claim:
1. A method for reducing the severity and/or incidence of fractures comprising administering to a site of osteoporotic or osteopenic bone tissue an injectable composition comprising an effective amount of an active agent in a suitable carrier.
2. The method of claim 1 , wherein the active agent is a member of the TGF-╬▓ superfamily of proteins.
3. The method of claim 1, wherein the active agent is a member of the bone morphogenetic protein family of proteins.
4. The method of claim 1, wherein the active agent is selected from the group consisting of BMP-2, BMP-4, BMP-5, BMP-6, BMP-7, BMP- 10, BMP-12 and BMP-
13.
5. The method of claim 1, wherein the active agent is BMP-2.
6. The method of claim 1, wherein the carrier is selected from the group consisting of a suitable buffer, blood, collagen gel and injectable calcium phosphates.
7. A method for healing bone fractures comprising implanting BMP into the region between ends of the bone fracture and allowing such rhBMP-2 to stimulate bone induction.
8. A cell produced by the method of claim 7 and harvested from the region between bone ends.
PCT/US1998/001143 1997-01-21 1998-01-21 Injectable formulations for treatment of osteoporotic bone WO1998031788A1 (en)

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