OSTEOCHONDRAL IMPLANTS, ARTHROPLASTY METHODS, DEVICES, AND SYSTEMS
Implants for resurfacing or repairing one or more articular cartilage bearing surfaces of a biological organism include an engineered tissue and a biocompatible porous substrate secured to the engineered tissue for attaching the implant to a native bone of the biological organism. The engineered tissue includes a scaffold containing a biocompatible material, and a plurality of living chondrocytes supported by the scaffold. Methods for culturing chondrocytes for incorporation into a biocompatible implant are provided. A bioreactor for producing functional cartilaginous tissue from a cell-seeded scaffold and a system for producing functional cartilaginous tissue are also provided.
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This application is a divisional application claiming priority to U.S. application Ser. No. 12/498,358, which is a Non-Provisional Patent Application of U.S. Provisional Patent Application Ser. No. 61/078,424, filed Jul. 6, 2008, the entirety of which are each incorporated by reference.STATEMENT OF GOVERNMENT INTEREST
This invention was made with United States government support under AR46568 and AR53530 awarded by National Institute of Health. The United States government has certain rights in the invention.BACKGROUND
Articular cartilage is a specialized connective tissue that bears load and reduces friction across moving joints. It is composed of an extracellular matrix that contains no nerves or blood vessels and relatively few cells (5% volume). Damage can arise due to disease or trauma and is common, especially in the aging population. Cartilage can decrease in strength with age. When damaged, articular cartilage either does not heal or at best heals only very slowly. Instead of healing, damaged cartilage often degenerates further, leading to pain and loss of function. Due to the prevalence of osteoarthritis (OA) and damage to articular cartilage, coupled with this poor intrinsic healing response, there is a great demand for clinical intervention.
Treatment of damaged cartilage in living animals presents difficult challenges. Adult cartilage is difficult to repair. Joint repair is conventionally done by replacing the entire joint or joint surfaces without trying to repair cartilage, usually in the form of a highly-invasive non-biological prosthetic (such as total joint arthroplasty). However, metal/plastic orthopedic implants have a limited lifespan (e.g., about 20 years) and are ideally reserved for use in older patients. The onset of arthritis, however, can begin as early as the age of 40 with much younger patients suffering from the disease as a result of trauma. Thus, some patients face the prospect that an artificial joint implant may wear out and need to be replaced.
One common biological alternative to arthroplasty entails the transplantation of healthy osteochondral autografts (cartilage along with some of the underlying bone) from a non-load bearing region. Osteochondral implants are designed to be press-fit into pre-drilled cavities in the damaged joint, replacing the host cartilage above while anchoring to the bone below. Osteochondral grafts are better anchored than chondral-only grafts and are less likely to be displaced by shearing forces within the joint. While these autologous grafting procedures are promising, they are limited both by the amount of tissue available and donor-site morbidity associated with its harvest. The use of donor cartilage from tissue banks (allografts) or from animal origin (xenografts) addresses these limitations, but introduces the possibility of disease transmission.
Tissue engineering strategies, if successful, could alleviate these problems by creating replacement tissues of the proper size and shape without concurrent damage to other regions of the patient's body. There is a great variety of tissue engineering approaches to form osteochondral constructs. For example, techniques for repairing cartilage have been proposed using scaffolds implanted with progenitor cells such as chondrocytes, stromal cells, stem cells, and such. However, clinical outcomes with biologic replacement materials have not been satisfactory, particularly because of mechanical issues, morphology and durability of biologics-based replacements.SUMMARY
Briefly, some aspects of the inventions include a two part implant with a biologic part and an artificial (or non-living biologic material) part. The implant can be grown in vitro and implanted such that the biologic part forms an articular surface of a joint. The invention also includes devices, systems, and methods for making, implanting, and treating patients and associated articles of manufacture.
Hybrid Synthetic-Biologic Joint Arthroplasty Systems comprise a group of related implants and techniques that provide a variety of options for performing joint replacement and resurfacing surgeries. The components may be similar for all systems and include implants for replacement or resurfacing of joint cartilage and bone, and techniques for tissue harvest, processing, and implantation. The implants may be composed of a synthetic component (e.g., metal, polymer, biomaterial) and a biologic component (e.g., tissue, cells, matrix) combined together. The hybrid implants are preferably designed to optimize long term success in joint replacement and resurfacing surgery of all major joints (hip, knee, ankle, shoulder, elbow, and fingers) by combining the advantages of synthetic and biologic arthroplasty techniques while minimizing the disadvantages of each.
The basic components for each system are: prostheses designed for replacement or resurfacing of articular cartilage and bone, and techniques for tissue harvest, processing, and implantation. The prostheses are composed of a synthetic component (e.g., metal, polymer, biomaterial) and a biologic component (e.g., tissue, cells, matrix). These hybrid prostheses allow for creating joint specific partial or complete hemi or total arthroplasty. Some basic embodiments for the hybrid prostheses include a cylindrical synthetic base with tissue engineered chondral layer and an anatomic synthetic base with tissue engineered chondral layer.
An immediate application of an engineered articular cartilage bearing surface is focal defect repair or resurfacing of an entire articular surface. The treatments are used, for example, for focal cartilage defects of the knee, ankle, elbow, and shoulder, partial and complete hemi and total joint arthroplasty of the knee, shoulder, hip, ankle, elbow, wrist, temporomandibular joint (TMJ), fingers, and toes—potentially millions of procedures each year worldwide. A biologic articular surface (versus plastic or metal) anchored to joints via a metal component. In an entire system, the process of using allogeneic chondrocytes that are expanded in culture and then seeded into an appropriate hydrogel that is integrated with an appropriate underlying “bony” base may be used. Additionally, techniques and design elements that provide fixation of the engineered hybrid construct implants are included.
The hybrid implant systems and related methods described herein are designed to improve long term success in joint replacement and resurfacing surgery of the hip, knee, ankle, shoulder, elbow, wrist, TMJ, fingers, and toes by combining the advantages of synthetic and biologic arthroplasty systems while minimizing the disadvantages of each. Specifically, the advantages of synthetic arthroplasty that can be obtained from the hybrid implants include: (1) functional replacement of bone; (2) ability to size and shape implants appropriately; (3) excellent implantation and fixation techniques; (4) immediate biomechanical function. The advantages of biologic arthroplasty that can be obtained from the hybrid implants include: (1) creation of living, site appropriate tissue with implant-host integration; (2) minimizing amount of foreign material in the body; (3) potential for continued remodeling; (4) improvement in tissue/joint characteristics and function; and (5) public perception and interest.
The disadvantages of synthetic systems that can be minimized using hybrid implants are: (1) metal and polymer breakdown products and their effects; (2) lack of long term durability and function; and (3) loss of future arthroplasty options. The disadvantages of biologic systems that can be minimized using the hybrid implants include: (1) the large amount of tissue required; (2) problems associated with cartilage-cartilage and cartilage-bone integration; (3) requirements for immediate load bearing function; (4) devitalized trabecular bone may have an inhibitory effect on in vitro chondral tissue development when used as a base material for the tissue-engineering of osteochondral constructs for cartilage repair.
One aspect of the invention is an implant for resurfacing or repairing one or more articular cartilage bearing surfaces of a biological organism. The implant includes an engineered tissue and a biocompatible porous substrate secured to the engineered tissue for attaching the implant to a native bone of the biological organism. The engineered tissue includes a scaffold containing a biocompatible material, and a plurality of living chondrocytes supported by the scaffold. The porous base substrate is substantially free of trabecular bone. In some instances, the porous substrate includes a metal such as tantalum. In other instances, the porous substrate includes a synthetic polymer or biologic material. The synthetic polymer can be polycaprolactone, poly-l-lactic acid, or polyglycolic acid. In some cases, the biologic material is collagen or hydroxyapatite. The scaffold contains a hydrogel such as agarose or alginate in some embodiments. In some implants, the engineered tissue has a bearing surface that has substantially the same shape of at least a portion of one of the one or more articular cartilage bearing surfaces that is to be resurfaced or repaired. The engineered tissue can have a bearing surface that has substantially the same shape as one of the one or more articular cartilage bearing surfaces that is to be resurfaced. In some cases, the engineered tissue has a total surface area in the range of about 0.05 cm2 to about 50 cm2, or a volume in the range of about 0.005 ml to about 80 ml. In some embodiments, the engineered tissue contains Type II collagen in an amount in the range of about 2 percent (w/w) to about 8 percent (w/w) or about 4 percent (w/w) to about 8 percent (w/w), a glycosaminoglycan (GAG) content in the range of about 4 percent (w/w) to about 10 percent (w/w) or about 5 percent (w/w) to about 8 percent (w/w), or an equilibrium Young's modulus (EY) of at least about 150 kPa. In some embodiments, the engineered tissue has an equilibrium Young's modulus (EY) in the range of about 150 kPa to about 1500 kPa, about 185 kPa to about 1300 kPa, about 275 kPa to about 1300 kPa, or about 800 kPa to about 1300 kPa.
Another aspect of the invention is directed to an implant for resurfacing or repairing one or more articular cartilage bearing surfaces of a biological organism, in which the implant includes an engineered tissue. The engineered tissue includes a scaffold containing a biocompatible material, and a plurality of living chondrocytes supported by the scaffold. The engineered tissue has an equilibrium Young's modulus (EY) of at least about 150 kPa. In some instances, the engineered tissue has an equilibrium Young's modulus (EY) in the ranges as described above. In some embodiments, the engineered tissue contains Type II collagen in an amount as described above, or has glycosaminoglycan (GAG) content in the range described above. In some aspects of the invention, the implant also includes a porous substrate secured to the engineered tissue for attaching the implant to a native bone of theI.ological organism. The porous substrate can be substantially free of trabecular bone. In some embodiments, the scaffold contains a hydrogel as described above. In other embodiments, the engineered tissue has a bearing surface as described above or has a total surface area or volume as described above.
Yet another aspect of the invention is directed to a method for culturing chondrocytes for incorporation into a biocompatible implant. A plurality of adult living chondrocytes are passaged in the presence of one or more growth factors. The chondrocytes are suspended in a gelable scaffold material. The chondrocytes and the gelable scaffold material is cultured in a medium containing transforming growth factor-beta3 (TGF-beta3). In some instances, the suspension of chondrocytes and gelable scaffold material is casted into one or more slabs, and the one or more slabs are cored to create one or more disks. In some embodiments, the suspension of chondrocytes and gelable scaffold material are secured to a biocompatible porous substrate. The suspension of chondrocytes and gelable scaffold material can be transferred to a mold and the biocompatible porous substrate substantially free of trabecular bone can be immersed into the chondrocytes and gelable scaffold material. In some instances, the biocompatible porous substrate contains a metal, a synthetic polymer or a biologic material as described above. In further embodiments, chondrocytes obtained from an autologous donor are passaged, while in other instances, chondrocytes obtained from an allogeneic donor are passaged. In some cases, adult canine chondrocytes are passaged. In the method of the invention, the chondrocytes can be passaged in the continuous presence of one or more growth factors.
Another aspect of the invention is a bioreactor for producing functional cartilaginous tissue from a cell-seeded scaffold. The bioreactor includes a support for supporting the cell-seeded scaffold, a platen, and a drive system. The drive system is operable to move the platen relative to the support to compress the cell-seeded scaffold while it is supported by the support and slide the platen on a surface of the compressed cell-seeded scaffold. In some instances, the cell-seeded scaffold has a bearing surface and the drive system is operable to slide the platen on the bearing surface, the platen being configured so no more than about half of the bearing surface is covered by the platen at any time.
Yet another embodiment of the invention is a system for producing functional cartilaginous tissue. The system includes a cell-seeded scaffold, a support supporting the cell-seeded scaffold, a platen, and a drive system. The drive system is operable to move the platen relative to the cell-seeded scaffold to sequentially (a) compress a first portion of the cell-seeded scaffold while temporarily maintaining a second portion of the cell-seeded scaffold different from said first portion in a substantially uncompressed state; and (b) compress the second portion of the cell-seeded scaffold while temporarily maintaining the first portion in a substantially uncompressed state.
Still another aspect of the invention is a method for producing functional cartilaginous tissue from a cell-seeded scaffold. The cell-seeded scaffold is compressed with a platen and the platen is slid on a surface of the compressed cell-seeded scaffold. In some instances, the cell-seeded scaffold is made by a process in which a plurality of living chondrocytes is suspended in a gelable scaffold material, and the chondrocytes and the gelable scaffold material are cultured in a medium containing transforming growth factor-beta (TGF-beta). In some embodiments, the suspension of chondrocytes and gelable scaffold material is molded into one or more slabs. One or more bodies can be excised from the one or more slabs, the bodies each having an average thickness of about 1 mm to about 6 mm or about 1 mm to about 4 mm. In some cases, the suspension of chondrocytes and gelable scaffold material is secured to a biocompatible porous substrate. The suspension of chondrocytes and gelable scaffold material can be transferred to a mold, and the biocompatible porous substrate substantially free of trabecular bone can be immersed into the chondrocytes and gelable scaffold material. In some instances, the biocompatible porous substrate contains a metal, a synthetic polymer or a biologic material as described above. Chondrocytes obtained from an adult human or animal subject are used in some embodiments, and the chondrocytes are passaged in the presence of one or more growth factors, such as TGF-beta, fibroblast growth factor-2 (FGF-2), and platelet-derived growth factor-BB (PDGF-BB).
Yet another embodiment of the invention is directed to a method for producing functional cartilaginous tissue from a cell-seeded scaffold. A first portion of the cell-seeded scaffold is compressed while temporarily maintaining a second portion of the cell-seeded scaffold different from the first portion in a substantially uncompressed state. The second portion of the cell-seeded scaffold is compressed while temporarily maintaining the first portion in a substantially uncompressed state. In some instances, the cell-seeded scaffold is made by a process in which a plurality of living chondrocytes is suspended in a gelable scaffold material, and the chondrocytes and the gelable scaffold material are cultured in a medium containing transforming growth factor-beta (TGF-beta). In some embodiments, the suspension of chondrocytes and gelable scaffold material is molded into one or more slabs. One or more bodies can be excised from the one or more slabs, the bodies each having an average thickness of about 1 mm to about 6 mm or about 1 mm to about 4 mm. In some cases, the suspension of chondrocytes and gelable scaffold material is secured to a biocompatible porous substrate. The suspension of chondrocytes and gelable scaffold material can be transferred to a mold, and the biocompatible porous substrate substantially free of trabecular bone can be immersed into the chondrocytes and gelable scaffold material. In some instances, the biocompatible porous substrate contains a metal, a synthetic polymer or a biologic material as described above. Chondrocytes obtained from an adult human or animal subject are used in some embodiments, and the chondrocytes are passaged in the presence of one or more growth factors, such as TGF-beta, fibroblast growth factor-2 (FGF-2), and platelet-derived growth factor-BB (PDGF-BB).
Other objects and features will be in part apparent and in part pointed out hereinafter.
Corresponding reference characters indicate corresponding parts throughout the drawings.DETAILED DESCRIPTION
Referring now to the drawings, one embodiment of a chondral implant, generally designated 101, is illustrated in
The chondrocytes can be juvenile chondrocytes and/or adult chondrocytes. Juvenile chondrocytes are those obtained from an organism before ossification of the epiphyseal plates in the subchondral and metaphyseal bone. Conversely, adult chondrocytes are those obtained from an organism after ossification of the epiphyseal plates. The chondrocytes can be autologous, or allogeneic. The chondrocytes can also consist of or include chondrocytes derived from stromal cells and/or stem cells that have been induced to exhibit the chondrocyte phenotype (e.g., by being subjected to mechanical loading and/or chondrogenic media). Further, the chondrocytes can also be accompanied by other living cells supported by the scaffold, including stromal cells, stem cells, and the like.
In addition to the scaffold and chondrocytes, the engineered tissue 103 suitably also includes an extracellular matrix (ECM) secreted by the chondrocytes. The ECM suitably has characteristics that are similar to the ECM of native cartilage. For example, the ECM is suitably rich in type II collagen and proteoglycans, such as glycosaminoglycan (GAG). For example, the engineered tissue suitably has a Type II collagen content in the range of about 2 to about 8 percent (w/w), more suitably in the range of about 4 to about 8 percent (w/w). Further, the engineered tissue can suitably have a Type II collagen content of about 4 percent (w/w) or more. The engineered tissue suitably has a GAG content in the range of about 4 to about 10 percent (w/w) and more suitably in the range of about 5 to about 8 percent (w/w). The engineered tissue 103 is also suitably functional to maintain an interstitial hydrodynamic pressure. Water is attracted to the feather-like polyanionic chains on the proteoglycan molecules, which are present in the engineered tissue in sufficient amounts to cause an osmotic swelling pressure. The high-tensile strength type II collagen forms a tight network of fibers arranged in a zonal architecture in which a surface layer of the bearing surface has a relatively higher concentration of collagen and a zone of tissue under the surface layer has a relatively lower concentration of collagen. The collagen fibers in the surface layer (which is sometimes referred to as surface tangential layer) are suitably oriented so a majority of the fibers are generally parallel to the surface of the articular bearing surface. The collagen works in opposition to the proteoglycan chains, resisting the swelling pressure and producing the load-bearing characteristics unique to cartilaginous tissue.
The zonal architecture characteristics of the engineered tissue 103 also include more than one characteristic phenotype of chondrocytes in native cartilage including spindyloid, round, or hypertrophic cells with pericellular, territorial, and/or interterritorial ECM such that collagen is primarily concentrated on the periphery and proteoglycan is primarily concentrated deeper in the engineered tissue 103.
The cell-seeded scaffold optionally includes one or more diffusion channels to enhance diffusion of nutrients into the scaffold, e.g., in the early stages of maturation. As illustrated in
Various materials can be used to make the scaffold. For example, a suitable scaffold can be made of an agarose hydrogel. However, other materials, including but not limited to alginate, polyethylene glycol, and other hydrogels, can be used within the scope of the invention.
The scaffold suitably has initial mechanical properties, porosity, and biocompatibility that is suitable for seeding the scaffold with cells and producing the engineered tissue according to the methods described below. The scaffold suitably has a hydraulic permeability in the range of about 2.8×10−13 to about 3.2×10−13 m4/Ns. Preferably, the scaffold is able to bear and transfer loads to the surrounding tissue without being crushed. The scaffold preferably also has a porosity that allows for cell infiltration and nutrient transport. The scaffold is also preferably biocompatible to mitigate immunogenic issues while allowing engineered tissue to develop and maintain functional properties in vitro and in vivo.
As discussed in greater detail below, certain advantages can be obtained by applying mechanical loading to the cell-seeded scaffold/developing engineered tissue. Initially, it is the mechanical properties of the scaffold that dictate the nature of the mechanical loading that can be applied to the developing engineered tissue. In some cases it may be desirable to begin mechanical loading of the cell-seeded scaffold relatively early in the maturation process to expedite production of the ECM by the cells supported by the scaffold and reduce the amount of time needed to ready the developing engineered tissue for implantation. The scaffold suitably has the ability to withstand application of physiologic deformational loading (e.g., 10 percent peak-to-peak deformation from unconstrained compression at 1 Hz) without resulting in separation of the scaffold from a loading platen of a dynamic loading machine used to apply a load to the scaffold, without resulting in permanent deformation of the scaffold, and without requiring the cells seeded in the scaffold to first produce a matrix before the loading is applied. This allows the mechanical loading to begin shortly (e.g., substantially immediately) after the scaffold is seeded with cells. Further, the scaffold suitably exhibits a similar load-support mechanism as native articular cartilage. For example, the scaffold is suitably able to bear greater than 90% of an applied load via interstitial fluid pressurization. The scaffold also suitably promotes and/or maintains exhibition of the chondrocyte phenotypes by cells in the scaffold. The chondrocyte phenotypes are preferred because chondrocytes tend to produce more of the desirable type II collagen and cartilage specific proteoglycan, aggrecan, (which are desirable in the ECM of cartilaginous tissue for in vivo function) as opposed to other phenotypes such as fibroblasts which tend to produce other types of collagen and proteoglycan, which are less desirable than type II collagen in the ECM of cartilaginous tissue because they are associated with disease and/or dysfunction.
The gelable scaffold material is also suitably permeable to nutrients when in gel form. There are several measures of the permeability of a gelable scaffold material, including for example, the volume fraction of the pores (porosity), the hydraulic permeability to water based solutions, and the diffusion coefficient of solutes of various molecular weights. The gelable scaffold materials of the present invention suitably have an average porosity in the range of about 96 percent to about 99 percent and more suitably about 98 percent, when in gel form.
The hydraulic permeability of a gelable scaffold can be measured, for example, using a permeation device. In particular, the hydraulic permeability can be measured by perfusing a water-based electrolyte solution (such as physiological saline) through the scaffold and measuring the pressure difference across the scaffold at various perfusion flow rates. The gelable scaffold materials used herein suitably have a hydraulic permeability in the range of about 2.8×10−13 to about 3.2×10−13 m4/N·s
The diffusion coefficient of a gelable scaffold material can be measured, for example, by fluorescent recovery after photobleaching (FRAP). In particular, the diffusion coefficient can be measured by incubating the gelable scaffold material with fluorescein isothiocyanate (FITC)-conjugated dextran having a molecular weight representative of large growth factors or matrix products commonly used or produced during cell culture (e.g., about 70 kDa). The gelable scaffold material can then be exposed to a high intensity monochromatic laser to induce localized photobleaching, and the recovery of fluorophores can be monitored. The gelable scaffold materials used herein suitably have diffusion coefficients ranging from about 8 μm2/second to about 50 μm2/second, and more suitably in the range of about 19 μm2/second to about 25 μm2/second. The diffusion coefficient is a measure of how fast nutrients, growth factors, and other substances diffuse through the scaffold material.
One scaffold that includes all of the characteristics listed above can be made of a thermoreversible agarose hydrogel (e.g., a 2 percent agarose hydrogel). It is noted that the scaffold material is likely to degrade over time. However, in contrast to native cartilaginous tissue, there is at least some residual scaffold material present in the engineered tissue 103 produced and matured by the methods described below.
The scaffold can be shaped (e.g., molded as described below) so the engineered tissue has a bearing surface 105 that has substantially the same size and shape as at least a portion of the native articular bearing surface that is to be resurfaced, restored, or repaired by the implant 101. For example, the scaffold can be molded into a shape having a surface that replicates only a portion of an articular bearing surface for replacement of only a portion of the articular bearing surface (e.g., a circular disk or other plug used to repair focal defects in the articular bearing surface). As another example, the scaffold can be molded to produce a bearing surface that replicates an entire articular bearing surface for total resurfacing of the bearing surface. If desired, suitable molds can be produced in conjunction with magnetic resonance imaging (MRI) or other imaging technology in combination with CAD-based rapid prototyping technology to produce engineered tissue having a shape including a surface that replicates the bearing surface of a particular patient.
As illustrated in
The engineered tissue 103 has characteristics that are substantially similar to or which exceed those of native cartilage. For example, the equilibrium Young's modulus is suitably at least about 150 kPa, more suitably in the range of about 150 kPa to about 1500 kPa, more suitably in the range of about 185 kPa to about 1300 kPa, still more suitably in the range of about 275 kPa to about 1300 kPa, and more suitably in the range of about 800 kPa to about 1300 kPa. As those knowledgeable of the properties of cartilaginous tissue know, the strain in cartilaginous tissue in response to a compression load will vary over time as fluid moves through the tissue in response to the load. Equilibrium Young's modulus is based on the amount of strain after the strain produced by the load has become substantially constant. Engineered tissue having these characteristics can be produced according to methods described in greater detail below.
The size of the body of engineered tissue 103 can vary depending on the amount of articular cartilage that is to be replaced by the implant. Using the methods described below, it is possible to make a significant amount of engineered tissue 103 having the mechanical and chemical properties described herein in a relatively short period of time. For example, the engineered tissue suitably has a total surface area in the range of about 0.05 cm2 to about 50 cm2, more suitably in the range of about 0.5 cm2 to about 50 cm2, more suitably in the range of about 1 cm2 to about 50 cm2, more suitably in the range of about 1 cm2 to about 25 cm2, more suitably in the range of about 1 cm2 to about 12 cm2, and more suitably in the range of about 5 cm2 to about 12 cm2. The engineered tissue suitably has a volume in the range of about 0.005 ml to about 80 ml, more suitably in the range of about 1 ml to about 80 ml, more suitably in the range of about 1 ml to about 25 ml, and still more suitably in the range of about 1 ml to about 10 ml. In the case of a plug type implant, for example, the volume can be in the range of about 0.005 ml to about 1.15 ml. In the case of an anatomically shaped implant for resurfacing a joint, the volume can be in the range of about 0.005 ml to about 25 ml. The engineered tissue suitably has a thickness in the range of about 0.1 mm to about 25 mm, more suitably in the range of about 1 mm to about 20 mm, and more suitably in the range of about 1 mm to about 10 mm, and still more suitably in the range of about 4 mm to about 10 mm.
The implant can be combined with other implants (e.g., a bone graft to make an osteochondral implant) during or prior to surgical restoration of an articular joint to replace or augment native cartilage in the joint. However, it is also contemplated, that the implant can be affixed directly to a native biological structure associated with an articular joint (e.g., native bone and/or native cartilage) using any suitable surgical techniques and without using any other implants within the scope of the invention.Osteochondral Implants
Although the chondral implant 101 described above can be suitable for some applications, advantages can be obtained in some cases by making an osteochondral implant including the engineered tissue 103 described above as the chondral portion of the implant and, as the osteo portion of the implant, a biocompatible porous substrate secured to the engineered tissue and suitable for attaching the engineered tissue to native bone associated with the articular joint. As noted above, cartilage heals poorly. This presents a further challenge to cartilage repair as the absence of healing response between the engineered tissue 103 and the adjacent native cartilage can result in poor graft-host integration. To facilitate integration of the engineered tissue 103 with native tissue, transplantation of the engineered tissue can be performed with an underlying segment of bone or a suitable non-biological porous substrate that acts as an anchor and secures the implant to the underlying bone. Using an osteochondral implant capitalizes on the ability for bone to heal well. Additionally, injuries that penetrate the subchondral bone (as would be the case during surgical implantation of an osteochondral implant) illicit a temporary cartilage repair response that involves cell migration from the bone marrow, fibrin clot formation, and associated vascular ingrowth.
One embodiment of an osteochondral implant 201 is illustrated in
When the scaffold material saturating the pores of the interface layer sets up as a gel, the cell-seeded scaffold is secured to the porous substrate. The porous substrate 211 remains secured to the cell-seeded scaffold as it matures into the engineered tissue 203. It is understood, however, that the engineered tissue 203 can be secured to the porous substrate 211 in other ways (such as an adhesive, interdigitated design of components, and/or direct mechanical fixation) within the scope of the invention. Also, the porous substrate 211 can be secured to the engineered tissue 203 after it has been matured within the scope of the invention.
Various materials can be used as the porous substrate 211 for the osteochondral implant 201 within the scope of the invention. The porous substrate 211 is suitably made of a material having properties that do not change over time in culture. The porous substrate 211 suitably has an open porous structure that facilitates securing the bone to gelling chondrocyte-laden agarose or other hydrogels that may be used as the scaffold to produce the engineered tissue. The porous substrate is also suitably biocompatible. The porous substrate can be osteoinductive and/or osteoconducive. The porous substrate is also suitably made of a material that can be readily configured to have anatomic size, shape, and geometry such that the substrate can be implanted and secured to the recipient's bone using standard surgical techniques.
In the implant 201 illustrated in
The implant 201 illustrated in
The scaffold for the engineered tissue 103 for the implant 201 is suitably substantially identical to the scaffold described above for the chondral implant 101 above. For example, the scaffold can be made of the same agarose hydrogel described above. Other scaffold materials described above can also be used within the scope of the invention. In addition to the factors that impact selection of a scaffold material for the chondral only implant 101, the scaffold material should also be selected to provide a sufficient interface strength between the chondral and osteo portions of the implant 201 to withstand the shear forces that will be encountered at the articular joint.
As illustrated in
Another embodiment of an osteochondral implant 301 is illustrated in
The inventors have found that chondrocyte-seeded agarose hydrogel constructs cultured alone or attached to an underlying bony base in a chemically defined medium formulation yields engineered cartilaginous tissue with native Young's modulus (EY) and glycosaminoglycan (GAG) content. By day 42 in culture the incorporation of a bony base significantly reduced these properties (EY=87±12 kPa, GAG=1.9±0.8% w/w) compared to the gel-alone group (EY=642±97 kPa, GAG=4.6±1.4% w/w). The mechanical and biochemical properties of chondrocyte-seeded agarose constructs were inhibited when co-cultured adjacent to bone (unattached). It is believed that that soluble factors rather than direct cell-bone interactions mediate the chondro-inhibitory bone effects. Altering the method of bone preparation, including demineralization, or the timing of bone introduction in co-culture did not ameliorate the effects. In contrast, osteochondral constructs with native cartilage properties (EY=730±65 kPa, GAG=5.2±0.9% w/w) were achieved when a porous tantalum metal base material was adopted instead of bone. (Example 1 below).
In particular, the substrate 311 of the embodiment illustrated in
Another osteochondral implant 401 is illustrated in
Also within the scope of the present invention are methods for producing functional cartilaginous tissue, including methods for making the chondral and osteochondral implants described above. These methods generally include making a cell-seeded scaffold including a plurality of living chondrocytes and a gelable scaffold material, and culturing the cell-seeded scaffold (the gelable scaffold material and chondrocytes) in a medium comprising transforming growth factor-beta (TGF-beta). The culturing is suitably performed in a bioreactor, wherein mechanical loading is applied to the cell-seeded scaffold according to the methods described in detail below.Method of Making the Cell-Seeded Scaffold
Methods for making the cell-seeded scaffold are also included within the scope of the present invention. The methods for making the cell-seeded scaffolds of the present invention generally include suspending a plurality of living chondrocytes in a gelable scaffold material, and forming the cell-seeded scaffold by shaping the living chondrocytes and gelable scaffold material into a desired shape. In some embodiments, the cell-seeded scaffold is combined with a porous substrate as described above.
As noted above, the living chondrocytes which are incorporated into the cell-seeded scaffolds of the present invention can be juvenile (i.e., immature) and/or adult (i.e., mature) chondrocytes. The chondrocytes are suitably primary chondrocytes or chondrocytes which have been subjected to limited expansion (passaging) in cell culture. Thus, to obtain the chondrocytes, cartilage is suitably harvested from a joint of a human or animal subject and the chondrocytes are isolated from the surrounding extracellular matrix (ECM). The chondrocytes can be chondrocytes from an autologous donor or an allogeneic donor.
In one embodiment, the chondrocytes may suitably be isolated from the surrounding ECM by digesting away the collagen with a collagenase (e.g., collagenase type VI) and separating the chondrocytes from the digested collagen, e.g. by filtering the suspension of digested collagen and chondrocytes. The chondrocytes may then suitably be concentrated (for example by centrifugation), counted (for example, using a hemocytometer), and resuspended in a physiologically compatible buffer to create a cell suspension having a suitable concentration of chondrocytes. In some embodiments, other types of living cells may also be added to the cell suspension, for example, stromal cells, stem cells, and the like. Suitable concentrations of chondrocytes in the cell suspension range from about 20 million cells/ml to about 400 million cells/ml. In some embodiments, the concentration of chondrocytes in the cell suspension is suitably about 30 million cells/ml to about 200 million cells/ml. In other embodiments, the concentration of chondrocytes in the cell suspension is about 60 million cells/ml.
If primary chondrocytes are to be used to make the implant, the isolated primary chondrocytes (with or without additional types of living cells) are suitably suspended in a gelable scaffold material. In one embodiment, a volume of the cell suspension is suitably mixed with a gelable scaffold material.
In some embodiments, in order to increase the number of chondrocytes available for incorporation into the cell-seeded scaffold, the primary chondrocytes can be subjected to limited expansion (passaging) in cell culture prior to being mixed with the gelable scaffold material. Passaging the chondrocytes is advantageous where the amount of cartilage which can be obtained is limited, for example where the cartilage is obtained from a living human subject. Furthermore, passaging has been found to be particularly suitable when the chondrocytes are adult chondrocytes. Following isolation of the chondrocytes from the cartilage of a human or animal subject, the chondrocytes are suitably plated in tissue culture dishes, tissue culture flasks, or the like, and grown at 37° C., 5% CO2 until substantially confluent. The chondrocytes are suitably cultured in Dulbecco's Modified Eagle Medium (DMEM) in the presence of serum and one or more growth factors, for example, TGF-beta, fibroblast growth factor (FGF), and platelet-derived growth factor (PDGF). The serum is suitably FBS, the TGF-beta is suitably TGF-beta1 or TGF-beta3, the FGF is suitably FGF-2 and the PDGF is suitably PDGF-BB. In one embodiment, the chondrocytes are suitably cultured in DMEM containing fetal bovine serum (FBS), about 0.1 ng/ml to about 10 ng/ml TGF-beta1 or TGF-beta3, about 0.5 ng/ml to about 50 ng/ml FGF-2 and about 1 ng/ml to about 100 ng/ml PDGF-BB. In another embodiment, the chondrocytes are suitably cultured in DMEM containing FBS, about 1 ng/ml TGF-beta, about 5 ng/ml FGF-2, and about 10 ng/ml PDGF-BB. Once the chondrocytes are substantially confluent, they are removed from the tissue culture plate (e.g., using trypsin or the like) and replated into two or more tissue culture dishes, flasks, or the like. The chondrocytes are again cultured in DMEM containing serum and growth factors described as described above until the chondrocytes reach substantial confluency. The replating can be repeated, and replating counts as one passage.
Persons having ordinary skill in the art will recognize that the number of passages to which the chondrocytes can be subjected will be limited by the tendency of the chondrocytes to become undifferentiated during passaging. The skilled artisan will also recognize that some level of de-differentiation during passaging is acceptable within the scope of the present invention, so long as the chondrocytes are capable of returning to a substantially differentiated state once incorporated into the cell-seeded scaffold and cultured in the presence of TGF-beta. The number of passages will therefore suitably be limited to a number of passages where although some de-differentiation may occur, the chondrocytes substantially return to their differentiated state once incorporated into the cell-seeded scaffold and cultured in the presence of TGF-beta, suitably in a bioreactor wherein mechanical loading is applied to the cell-seeded scaffold according to the methods described below. For example, the chondrocytes are suitably passaged for fewer than about five passages, and more suitably for fewer than about three passages. Following passaging, the chondrocytes are suitably removed from the tissue culture plate and suspended in a physiologically compatible buffer to create a cell suspension having a suitable concentration of chondrocytes, as described above, and the cell suspension is suitably mixed with a gelable scaffold material.
The gelable scaffold material is suitably an agarose hydrogel material. However, as noted above, other materials, including but not limited to alginate and various synthetic and natural (e.g., collagen, hyaluronan) hydrogels, can be used within the scope of the invention. When the gelable scaffold material is a thermoreversible gelable scaffold material, the gelable scaffold material suitably gels at a temperature at which the viability and health of the cells will not be substantially detrimentally affected during the time it takes the gelable scaffold material to gel. For example, the gelable scaffold material suitably has a gel point of about 4° C. to about 38° C. When the gelable scaffold material is thermoreversible gelable scaffold material, the gelable scaffold material also suitably has a low melting point. For example, when the gelable scaffold material is agarose, the agarose is suitably a low melt agarose, for example Sigma agarose Type VII (having a gel point of 26° C.±2.0° C. at 1.5% and a melting temperature of ≦65° C.) or Sigma agarose Type IX (having a gel point of 8-17° C. at 0.8% and a melting temperature of ≦50° C.).
In one embodiment of the method of making the cell-seeded scaffold, a volume of the cell suspension is mixed with an approximately equal volume of about 2% to about 6% agarose, to yield a final agarose concentration of about 1% to about 3%. In addition, mixing the volume of the cell suspension with the gelable scaffold material will suitably yield a chondrocyte concentration in the cell suspension/gelable scaffold material suspension of about 10 million cells/ml to about 200 million cells/ml. More suitably, the mixing will yield a chondrocyte concentration of about 10 million cells/ml to about 60 million cells/ml. For example, in some embodiments, a volume of a cell suspension having a chondrocyte concentration of 60 million cells/ml is mixed with an approximately equal volume of 4% low-melt agarose at 37° C. to yield a chondrocyte concentration of 30 million cells/ml and an agarose concentration of 2%.Casting/Molding the Cell-Seeded Scaffold
Once the plurality of living chondrocytes have been suspended in the gelable scaffold material, the cell-seeded scaffold can be formed by shaping the suspension of living chondrocytes and gelable scaffold material into a desired shape.
In one embodiment of a method for shaping the living chondrocytes and gelable scaffold material into a desired shape, the suspension of chondrocytes and gelable scaffold material is suitably casted or molded into one or more slabs. One or more bodies can then suitably be excised from the one of more slabs. The bodies suitably each have an average thickness of about 0.1 mm to about 10 mm (e.g., about 0.5 mm to about 6 mm). In some embodiments, the bodies are disks having substantially circular cross-sections and have average diameters in the range of about 3 mm to about 20 mm (e.g., about 4 mm to about 10 mm). For example, a chondrocyte/agarose suspension can be cast into slabs and cored using a sterile disposable punch to final dimensions of about 3 mm to about 4 mm (diameter) by about 2.3 mm (thickness).
Another embodiment of a method for shaping the scaffold/engineered tissue 103, 203, 303, 403 into a desired shape and combining the scaffold/engineered tissue with a porous substrate 211, 311, 411 is illustrated in
One embodiment of a molding system uses a mold 801 (
The mold base 803 suitably includes a plate 807 and a projection 809 extending from the plate. The projection 809 suitably extends up from a central portion of the plate 807 so the plate forms a shoulder extending circumferentially around the projection. The retainer 805 includes a circumferential sidewall 821 having an inner surface 825 that forms an opening 831 extending through the retainer from the top to the bottom. The opening 831 is sized and shaped to receive the projection 809 when the bottom 823 of the retainer is placed on the shoulder 807 of the mold base 803. The projection 809 suitably has a side surface 827 sized and shaped to conform to the inner surface 825 of the retainer sidewall 821. If desired, a gasket or other seal (not shown) can be positioned between the inner surface 825 of the retainer sidewall 821 and the side surface 827 of the projection and/or between the bottom 823 of the retainer 805 and the shoulder 807 of the mold base to form a fluid-tight seal between the mold base and the retainer.
When the mold base 803 and retainer 805 are secured together with the bottom 823 of the retainer on the shoulder 807 of the mold base as illustrated in
The upper surface 811 of the projection 809 suitably has a shape designed to produce the articular bearing surface of the cell-seeded scaffold/engineered tissue. For example, the shape of the projection 809 at its upper surface 811 is suitably a negative of the articular bearing surface. The shape of the projection 809 at the upper surface 811 can be customized for a particular recipient. For example, digitized anatomical data from an MRI or other imaging system can be used in combination with a CAD-based rapid prototype system to create a mold base 803 in which the projection 809 (including the shape of the upper surface 811) is customized to account for the recipient's anatomy and thereby facilitate implantation of the resulting implant in the recipient. Alternatively, the mold base 803 can be selected from a set of standardized mold bases designed to produce implants having various standardized sizes and shapes that are suitable for commonly performed procedures. Because the mold base 803 and retainer 805 illustrated in
To use the mold 801, the retainer 805 is secured to a mold base 803 having a projection 809 defining an appropriately shaped upper surface 811 to form a mold cavity 841 that is shaped to produce the desired implant. Then a mixture 851 of cells and gelable scaffold material (e.g., produced as described above) is dispensed into the mold cavity 841. For example, the mixture 851 can be dispensed in the mold 841 cavity using a pipette 853 or other suitable device, as illustrated in
As illustrated in
For example, if the porous substrate 871 is made of tantalum, computer controlled wire electrical discharge machining can be used to shape the porous tantalum substrate while maintaining the porous structure of the tantalum. Virtually any shape that would be needed for a tantalum porous substrate of an osteochondral implant can be obtained from Zimmer, Inc. of Warsaw, Ind., which sells a suitable tantalum substrate as Trabecular Metal™.
The gelable mixture 851 penetrates a portion of the porous substrate 871 creating a layer 891 of substrate that is saturated with the gelable mixture. The gelable material is allowed to set up in the mold 801. The result is a multilayer construct 887 including a cell-seeded scaffold only layer 893, a scaffold-porous substrate interface layer 895, and a substrate only layer 897. The shape of the mold cavity 841, the shaped portion 873 of the porous substrate 871, and the temporary retaining portion 875 of the porous substrate are suitably selected so the cell-seeded scaffold layer 993 has a thickness in the range of about 0.1 mm to about 10 mm (e.g., about 2 mm), the interface layer 995 has a thickness in the range of about 0.1 mm to about 10 mm (e.g., about 2 mm), and the porous substrate layer has a thickness in the range of about 0.2 mm to about 40 mm (e.g., about 2 mm).
Then the construct 887 is placed in a bioreactor to allow the cell-seeded scaffold to develop into the engineered tissue through maturation, as described in more detail below.Method of Culturing the Cell-Seeded Scaffold in a Bioreactor
The cell-seeded scaffold (the gelable scaffold material and living chondrocytes) is suitably cultured in a medium which includes TGF-beta. The medium can also suitably include ascorbate and/or dexamethasone. The culturing is suitably carried out in a bioreactor which can also be configured for applying mechanical loading to the developing engineered tissue, as described in detail below.
The cell-seeded scaffold is suitably cultured in the bioreactor for a period of about 28 days to about 70 days, and more suitably for a period of about 28 days to about 56 days. It has been discovered that by using the methods of the present invention, engineered cartilaginous tissue having properties similar to those of native cartilage can be grown in the bioreactor in less than about 4, 5, 6, 7, or 8 weeks.
The medium in which the cell-seeded scaffold is incubated is suitably substantially serum-free. The use of tissue culture supplements such as serum is undesirable because such supplements are not chemically well-defined and can possess batch-to-batch compositional variations, raising quality control concerns for clinical applications of engineered tissue grown in the presence of serum.
In embodiments wherein the chondrocytes are chondrocytes derived from the cartilage of an adult human or animal subject, the TGF-beta is suitably present in the medium for substantially the entire period during which the cell-seeded scaffold is cultured in the bioreactor. For example, in one embodiment, the cell-seeded scaffold is cultured for 60 days with continuous growth factor (TGF-beta3) supplementation.
In embodiments wherein the chondrocytes are chondrocytes derived from the cartilage of an immature human or animal subject, it is advantageous to culture the cell-seeded scaffold in a medium in which TGF-beta is transiently present. For example, cell-seeded scaffolds containing immature chondrocytes can suitably be cultured in a medium supplemented with TGF-beta for about the first 14 days of the culture period, and subsequent culturing can be carried out in a medium which is substantially free of TGF-beta. When immature chondrocytes are used, these culture conditions lead to dramatic increases in the Young's modulus and the GAG content
The TGF-beta is suitably present in the medium at a concentration of about 1 ng/ml to about 100 ng/ml. For example, the TGF-beta can be suitably present in the medium at a concentration of 10 ng/ml. The TGF-beta can suitably be TGF-beta1 or TGF-beta3. Furthermore, in addition to the TGF-beta, one or more other growth factors may also be included in the medium. In particular, it has been found that the addition of insulin-like growth factor-1 (IGF-1) to the medium results in a high compressive Young's modulus and a high GAG content in the engineered cartilage.Dynamic Loading
The maturation process suitably includes periodic mechanical loading of the cell-seeded scaffold/developing engineered tissue to facilitate development of cartilaginous tissue having the desirable characteristics described above. The mechanical loading subjects the chondrocytes to conditions that are similar to what they would encounter in vivo in an articular joint. The chondrocytes respond to the loading by producing an ECM that is more similar in composition and arrangement to the ECM of native articular cartilage than would be produced in the same amount of time by chondrocytes that are not subjected to mechanical loading.
When mechanical loading is used, the maturation process suitably includes an exercise period in which the constructs are subjected to dynamic loading (meaning the load is repeatedly applied and removed) for a period of time followed by a rest period in which the constructs are not subjected to any significant mechanical loading. For example, the exercise period may include one or more exercise periods per day that are about 3 hours in total length and rest periods can include one or more rest periods totaling about 21 hours in length. The mechanical loading does not need to be applied every day. Good results have been obtained by exercising the constructs for about 3 hours daily for five days a week followed by two days without mechanical loading.
Various types of dynamic loading can be applied to the developing engineered tissue within the scope of the invention. One type of dynamic loading is unconstrained compression loading. Unconstrained compression loading can be applied by compressing the cell-seeded scaffold/developing engineered tissue axially (e.g., between two platens) while movement in the radial direction is unconstrained. See U.S. Pub. Pat. App. No. 20020106625, the contents of which are hereby incorporated by reference, for an example of a bioreactor operable to apply unconstrained compression loading. The axial load is suitably sufficient to produce deformation that reduces the thickness of the developing engineered tissue by up to about 50 percent, more suitably in the range of about 10 percent to about 30 percent, and still more suitably about 20 percent. The axial load is suitably applied with a frequency in the range of about 0.1 Hz to about 5 Hz.
Another type of dynamic loading that can be applied is a combination of compression loading and sliding/friction loading. This type of loading can be achieved by compressing a portion or all of the cell-seeded scaffold/developing engineered tissue with a platen and sliding the platen across a surface thereof. For example, as illustrated in
While not being bound by any particular theory, it is believed the sliding regime can provide improved results in some cases because the smaller contact area between the platen 901 and the scaffold 903 provides the scaffold with improved access to culture media during the exercise period, particularly when compared to a compression loading regime in which the upper and lower surfaces of the scaffold 903 are completely covered by the platens and the most significant pathway available for diffusion of nutrients into the scaffold radially inward from unconstrained edge margins of the scaffold.
In contrast, in the sliding/friction loading regime illustrated in
The axial deformation load applied by the sliding platen 901 to the scaffold 903 can vary within the scope of the invention. The axial load is suitably sufficient to compress the tissue thickness in the range of about 0.1 mm to about 5 mm. The amount of compression can vary according to the thickness of the cell seeded scaffold. In general, it is best to avoid compressing the tissue more than about 20 percent because this can lead to chondrocyte deactivation and other undesirable outcomes. For example, the axial load applied by the sliding platen 901 to the scaffold is suitably sufficient to reduce the thickness of the compressed tissue in the range of about 10 percent to about 20 percent.
Dynamic mechanical loading as described above, can be applied to the cell-seeded scaffold/developing engineered tissue 903 using the bioreactor described below and illustrated in
The bottom of the container 1005 is suitably filled with a layer of gel 1010 (e.g., agarose). A plurality of wells 1012 are cut or otherwise formed in the gel for holding a developing engineered tissue construct, which in
A pulley 1017 mounted on the lead screw can is suitably connected to a motor by a belt (motor and belt not shown) to drive rotation of the lead screw. The motor is suitably operable to drive cyclical rotation of the lead screw 1015 back and forth in opposite directions (e.g., at a frequency of about 1 Hz). As the lead screw 1015 rotates back and forth, e.g., over a range of about 360 degrees, the container 1005, which is rotatably fixed to the lead screw by the set screws 1021, rotates along with the lead screw relative to the cover 1003 and top assembly 1007.
As illustrated in
A load cell 1041 is supported on the top plate assembly 1007 by a bracket 1043 (
The bioreactor 1001 can readily be converted for application of unconstrained dynamic compression loads by replacing the top plate assembly 1007 with the top assembly 1107 illustrated in
Example 1 illustrates the effects two different materials (devitalized trabecular bone and tantalum) have on chondral development when used as the material for the porous substrate for an osteochondral implant.Experimental Design of Example 1
In Study 1 of Example 1, the development of chondrocyte-seeded agarose hydrogel constructs and osteochondral constructs were directly compared using the same tissue-engineering protocol. To assess the effects of soluble factors released by bone, chondral only constructs were also co-cultured adjacent (but unattached) to devitalized bone. To exclude the effect of soluble minerals, chondral only constructs were also cultured adjacent to demineralized bone. Finally, to test for the possibility that the inhibitory effect of bone is not related to soluble factors, but rather due to a decrease in the availability of growth factors through the absorption into bone, chondral only constructs were cultured in medium without TGF-β3.
In Study 2 of Example 1, the formation of functional osteochondral implants after separate cultivation of the chondral region was examined by delaying the introduction of bone to day 14 of culture or on day 28. Chondral only constructs were also cultured without any bone to serve as controls.
In Study 3 of Example 1, osteochondral constructs were formed with a porous tantalum metal substrate and compared to osteochondral constructs that included trabecular bone and chondral only constructs that did not include any bone.
Each study was carried out separately and all groups were cultured for 42 days.Materials and Methods for Example 1
Cell Isolation. Articular cartilage was harvested from bovine carpo-metacarpal (CMC) joints of freshly slaughtered 1-3 weeks old calves. Three to five joints were used for each study and cells were pooled from all joints. Cartilage chunks were digested in DMEM with 390 U/ml collagenase type VI (Sigma Chemicals, St. Louis, Mo.) for 11 hours at 37 C with stirring. The resulting cell suspension was then filtered through a 70 μm pore-size mesh and sedimented in a bench top centrifuge for 10 minutes at 1000 g. Viable cells were counted using a hemocytometer and trypan blue.
Osteochondral Substrate preparation. To prepare devitalized bone, cylindrical cores (about 15 mm long) of trabecular bone were isolated from the subchondral region of bovine tibia using a diamond-tipped, hollow drill (Starlite, Rosemont, Pa.). Cores were rough cut to about 6 mm in length and centered in a custom 4 mm thick stainless steel mold such that there were overhanging surfaces on both sides of the mold. These surfaces were then sanded flat with a hand-held device to ensure that the final bone cores had uniform dimensions (4 mm diameter×4 mm±50 μm length) with parallel faces cut normal to the axis of symmetry. The bone cores were then cleaned of marrow in one of three ways: 1) with a water pick and subsequently sterilized in 70% ethanol for four hours, 2) by washing in hypotonic buffer with detergent and DNAse and RNAse solutions, or 3) as provided by a commercial vendor through their FDA approved BioCleanse processes (RTI Biologics). To keep the quantity of bone consistent between experiments, cleansed bone was sorted to within a 10% deviation in mass and volume. The experiments presented in Study 1 of Example 1 and Study 2 of Example 1 were repeated with each of these cleaning methods with no significant differences in results. The data presented here are averaged across all experiments.
Demineralized bone. For the co-culture (Demin) group in Study 1 bone was demineralized in 6 NHC 1 for 12 hours.
Tantalum metal. Porous tantalum metal substrates (Zimmer) were prepared using wire cut electron discharge machining (to maintain the scaffold porosity) to final construct dimensions of 4 mm diameter×4 mm length.
Growth medium. The growth medium was changed every other day and consisted of high glucose Dulbecco's Modified Eagle's Medium supplemented with 1×PSF (100 units/ml Penicillin, 100 μg/ml Streptomycin, 0.25 μg/mlFungizone), 0.1 μM dexamethasone, 50 μg/mL ascorbate 2-phosphate, 40 μg/mL L-proline, 100 μg/mL sodium pyruvate, and 1× ITS+ premix (insulin, human transferrin, and selenous acid, Becton Dickinson, Franklin Lakes, N.J.). The ITS+ premix is a 100× aqueous solution containing 12.5 mg human recombinant insulin, 12.5 mg human transferring, 12.5 μg selenous acid, 2.5 g BSA, and 10.7 mg linoleic acid. Chemically defined medium was further supplemented with 10 ng/mL of TGF-β3 (R&D Systems, Minneapolis, Minn.) for the first 14 days of culture.
Material Testing. The equilibrium Young's modulus (EY) is commonly used as a measure of the behavior of cartilage that has been allowed to reach equilibrium after a known load or displacement has been applied. Constructs were tested for Young's modulus in unconfined compression using a custom computer-controlled testing system. An initial 0.02 N tare load was applied, followed by a compression to 10% strain (of the chondral region), at a strain rate of O.O5%/sec. Young's modulus was calculated from the equilibrium stress at 10% strain. Previous studies have shown Young's modulus to remain invariant across strain magnitudes ranging from 0% to 20%.
To determine the shear strength at the interface, the chondral region of osteochondral constructs were cut in half (
Biochemical Content. The biochemical content of each sample was assessed by first measuring sample wet weight, lyophilizing for 24 hours, and then measuring the sample dry weight. Once dry, the samples were digested in proteinase-K overnight at 56 C. Aliquots of digest were analyzed for glycosaminoglycan (GAG) content using the 1,9-dimethylmethylene blue dye-binding assay. A further aliquot was acid hydrolyzed in 12 N HCl at 110° C. for 16 hours, dried over NaOH, and resuspended in assay buffer. Orthohydroxyproline (OHP) content was then determined via a colorimetric assay by reaction with chloramine T and dimethylaminobenzaldehyde. OHP content was converted to total collagen content using the conversion of 1:10 ratio of OHP:collagen. Each biochemical constituent (GAG and collagen) was normalized to tissue wet weight.
Histological Analysis. Chondral samples were fixed in acid formalin ethanol, paraffin embedded, sectioned (8 μm thick), and stained to view proteoglycan or total collagen or type II collagen distribution. For osteochondral constructs histological specimens were prepared and stained at the Department of Surgical Sciences, University of Wisconsin. Live/dead assays were carried out using manufacture's protocol (Molecular Probes).
Statistics. Statistics were performed with the Statistica (Statsoft, Tulsa, Okla.) software package. Each data point represents the mean and standard deviation. Groups were examined for significant differences by analysis of variance (a=0.05), with EY, GAG, or OHP as the dependent variable using the Tukey's Honest Significant Difference Test (HSD).Results of Study 1 of Example 1
Study 1 showed both osteochondral (OC(bone)) and chondral (Gel) constructs developed significantly better mechanical and biochemical properties over time, as illustrated in
However the chondral constructs consistently performed better than the osteochondral constructs and the chondral constructs that were co-cultured with bone or demineralized bone. For example, the day 42 values for the osteochondral group were EY=87±12 kPa and GAG=1.9±0.8% w/w. In comparison, the values for the chondral only group were EY=642±97 and GAG=4.6±1.4% w/w.
Collagen values were not significantly different between the two groups. DNA quantification indicated a 30% increase in cell number over the culture period with no significant differences between the two groups. Live/dead staining revealed the presence of vital cells in all three regions of the osteochondral constructs, including the bone-only region where no cells were initially seeded. These cells appeared elongated and seemed to have attached to the underlying bony substrate. Immunohistological staining indicated the continued deposition of type I1 collagen in all three regions (
The presence of separate bone plugs in the co-culture experiments (co-culture(bone)) resulted in significantly lower EY and GAG by day 42 than the chondral only groups and no statistical differences from the osteochondral group (
Constructs cultured without TGF-3 (noTGF) resulted in significantly lower EY and GAG when compared to the chondral only groups, but higher EY than the osteochondral group (
Study 2 showed the addition of bone to the culture medium resulted in lower EY values regardless of whether the bone was added later in culture (
Study 3 showed that by day 42, osteochondral groups formed with bone substrate (OC(Bone)) developed significantly lower EY and GAG than chondral only (Gel) groups (
Taken together the Studies in Example 1 demonstrate that devitalized trabecular bone has in at least some cases an inhibitory effect on in vitro chondral tissue development when used as a base material for the tissue-engineering of osteochondral constructs for cartilage repair. Although not bound by any particular theory, it appears likely the bone was adversely affecting tissue development because soluble chemical mediators were inhibiting the observed chondral tissue development. It may be that osteoinductive factors released by bone may contribute to suppression of the chondrogenic phenotype. Bone matrix is known to contain intrinsic cytokines and growth factors that have a wide and largely unknown range of effects on cell development. The type and concentration of these factors vary even between the bones of the same animal.
The generation of osteochondral constructs was most successful when bone was substituted with a non-biological alternative. Using porous tantalum metal, native Young's modulus values and GAG and collagen content similar to chondral-only constructs were achieved. The integration strength (between the layers) of tantalum/agarose scaffolds were on par with, or exceeded, values reported in the literature, but remained below native levels.Example 2 Cell Isolation and Culture: Immature Chondrocytes
Articular cartilage was harvested from bovine carpo-metacarpal (CMC) joints of freshly slaughtered 1-3 week old calves. Three to five joints were used for each study and cells were pooled from all joints. Cartilage chunks were digested in DMEM with 390 U/ml collagenase type VI for 11 hours at 37° C. with stirring. The resulting cell suspension was then filtered through a 70 μm pore-size mesh and sedimented in a bench top centrifuge for 10 minutes at 1000×g. Viable cells were counted using a hemocytometer and trypan blue.
One volume of chondrocyte suspension (at 60×106 cells/ml) was then mixed with an equal volume of 4% low-melt agarose (Type VII, Sigma) at 37° C. to yield a final cell concentration of 30×106 cells/mL in 2% agarose. To create cell-seeded scaffolds for chondral implants (containing chondrocytes and gelable scaffold material, without any attached porous substrate), the suspension of chondrocytes and agarose was cast into slabs and cored using a sterile disposable punch to final dimensions of about 4 mm diameter and about 2.3 mm thickness. To create cell-seeded scaffolds for osteochondral implants (containing the chondrocytes and gelable scaffold material secured to a biocompatible substrate), 60 μL of the chondrocyte/agarose suspension was poured into the cylindrical wells of a custom mold. Biocompatible porous osteochondral substrates immersed in the chondrocyte/agarose suspension from above to the desired depth (adjusted using a temporary retaining ring). With this technique a multi-layered construct was formed with the following dimensions: a 2 mm agarose-only top region, a 2 mm agarose plus substrate interface region, and a 2 mm substrate-only region.
The cell-seeded scaffolds were cultured in chemically-defined medium containing high-glucose DMEM Dulbecco's Modified Eagle's Medium supplemented with 1×PSF (100 units/ml penicillin, 100 μg/ml Streptomycin, 0.25 μg/ml Fungizone (Amphotericin B)), 0.1 μM dexamethasone, 50 μg/mL ascorbate 2-phosphate, 40 g/mL L-proline, 100 μg/mL sodium pyruvate, and 1×ITS+ premix (insulin, human transferrin, and selenous acid). The chemically defined medium was further supplemented with 10 ng/mL of TGF-β3 for the first 14 days of culture. The growth medium was changed every other day.Example 3 The Beneficial Effect of Delayed Compressive Loading on Tissue-Engineered Cartilage Constructs Cultured with TGF-Beta3
The objective of these studies was to determine whether the functional properties of tissue-engineered cartilage constructs cultured in a chemically-defined medium supplemented briefly with TGF-β3 could be enhanced with the application of dynamic deformational loading. The application of dynamic compressive loading (DL) within appropriate ranges of magnitude and frequency can be a beneficial tool for the functional tissue engineering of articular cartilage. It has been shown to increase synthesis of cartilage ECM components such as proteoglycans, collagens, and other matrix elements using a variety of loading apparatuses and culture systems when compared to control constructs maintained in free-swelling (FS) culture. The effect of dynamic loading is influenced by other factors in the tissue-engineering system such as the choice of scaffold, the formulation of feed media, and cellular factors such as species, age, and seeding density, and therefore protocols must be developed for a given set of experimental conditions.
It has been shown that temporal supplementation with transforming growth factor β3 (TGF-β3) (a 2-week exposure to TGF-β3 followed by 6 additional weeks of culture in medium substantially free of TGF-β3) in free-swelling, serum-free cultures of chondrocyte-laden agarose hydrogel constructs resulted in the development of constructs possessing cartilage-like compressive mechanical properties (EY>800 kPa). These values are significantly higher than modulus values obtained for engineered cartilage using any other culture system over the same culture duration; the only comparable outcome previously required over 7 months of continuous cultivation to develop similar properties. Prior to the current study, however, there was no data showing how chondrocyte-seeded constructs would respond to the application of dynamic loading under these media conditions.
In the present study, dynamic deformational loading applied concurrently with TGF-β3 supplementation yielded significantly lower (−90%) overall mechanical properties when compared to free-swelling controls. In contrast, the same loading protocol applied after discontinuation of the TGF-β3 supplementation resulted in significantly increased (+10%) overall mechanical properties relative to free-swelling controls. Equilibrium modulus values reached 1,306±79 kPa and glycosaminoglycan (GAG) levels reached 8.7±1.6% w/w during a 8 week culture period and are similar to host cartilage properties (994±280 kPa, 6.3±0.9% w/w). Thus, one strategy for the functional tissue engineering of articular cartilage, particularly to accelerate construct development, may incorporate sequential application of different growth factors and applied deformational loading.Materials and Methods A. Experimental Design.
Three studies are discussed in this example (see
The timeline of the studies are detailed in
In Study 1 (n=4 per group), TGF-β3 was supplemented to the media either for the first 14 days only (discontinuous) or it was supplemented throughout the duration of the study (continuous). There was no loading introduced to these developing constructs at any time. Based on the results of Study 1, a protocol of discontinuous TGF-β3 supplementation was adopted for both Study 2 and Study 3.
In Study 2 (n=5 per group), dynamic deformational loading was initiated on day 0 and was continued throughout the culture period.
In Study 3 (n=8 per group), dynamic deformational loading was initiated on day 14 (delayed until the day TGF-β3 was discontinued). In all studies, dynamic deformational loading is abbreviated CDL when initiated at day 0, and DDL when delayed until after the discontinuation of TGF-β3. A follow up study (n=5 per group) was also performed with loading initiated on day 0 on the basal media without TGF-β3.B. Cell Isolation.
Articular cartilage was harvested from bovine carpo-metacarpal (CMC) joints of freshly slaughtered 2-3 month old calves. Three to five joints were used for each study and cells were pooled from all joints. Cartilage was rinsed in high-glucose Dulbecco's Modified Essential Medium (hgDMEM) supplemented with 5% fetal bovine serum (FBS), amino acids (0.5× minimal essential amino acids, 1× nonessential amino acids), buffering agents (10 mM HEPES, 10 mM sodium bicarbonate, 10 mM TES, 10 mM BES), and antibiotics (100 U/ml penicillin, 100 μg/ml streptomycin). The cartilage chunks were then combined and digested in DMEM with 390 U/ml collagenase type VI for 11 hours at 37° C. with stirring. The resulting cell suspension was then filtered through a 70 μm pore size mesh and sedimented in a bench top centrifuge for 10 minutes at 1000×g. Viable cells were counted using a hemocytometer and trypan blue.
One volume of a chondrocyte suspension (at 60×106 cells/ml) was then mixed with an equal volume of 4% low-melt agarose (Type VII, Sigma) at 37° C. to yield a final cell concentration of 30×106 cells/ml in 2% agarose. The chondrocyte/agarose mixture was cast into slabs and cored using a sterile disposable punch to final dimensions of 0.3 cm diameter and 0.23 cm thickness (0.016 cm3). Constructs were maintained in culture in a chemically-defined serum-free growth medium for 42 days or up to 56 days depending on the study (See
The prescribed loading protocol consisted of a nominal 5% dynamic strain (10% peak-to-peak deformation) above a 10% tare strain in unconfined compression with impermeable platens loading at 1 Hz frequency, for 3 hrs/day, 5 days/week (as had been previously found to be optimal for media formulations containing FBS). The duty cycle consisted of 3 hrs of continuous loading followed by 21 hrs of rest. Deformational loading was carried out at 37° C. and 5% CO2 in a humidified incubator. FS controls were positioned adjacent to the loading device.
The load and displacement profiles delivered by the bioreactor were analyzed in a small sample of specimens at the completion of all the experiments. In practice, the applied sinusoidal displacement had a consistent frequency of 1.05 Hz, with a total harmonic distortion of 6.03±0.95%. Due to inherent compliance of the loading bioreactors, the applied strain amplitude decreased over the culture period, as tissue elaboration produced specimens with increasing stiffness; the dynamic strain amplitude started at 5% and tapered to 2% by day 42 in culture (4% peak-to-peak). This compliance, coupled with the increasing tare strain resulting from growing construct thickness, had the beneficial effect of compensating passively for the increasing construct stiffness to prevent any loading platen lift-off through the entire culture period (see
Cylindrical constructs were tested in unconstrained compression using a custom computer-controlled testing system. Initially, a series of stress-relaxation tests were conducted for each sample to 5%, 10%, 15%, and 20% strain and the Young's modulus (EY) of the construct was calculated from the equilibrium stress at each strain value and from the initial cross-sectional area. Since the resulting EY was found to remain invariant across the strain amplitudes tested, the remaining samples were tested at 10% strain only and at a strain rate of 0.05% strain/sec after an initial 0.02 N tare load. The unconstrained dynamic modulus was also measured, after reaching stress-relaxation equilibrium to 10% strain, by superimposing 2% strain at 1 Hz. Tests of static and dynamic compressive properties were selected since the normal physiological loading mode of cartilage is compressive. More specifically, the most functionally relevant mechanical property is the dynamic modulus in compression, since joint loading is typically intermittent.E. Biochemical Content.
The biochemical content of each sample was assessed by first measuring sample wet weight, lyophilizing for 72 hours, and then measuring the sample dry weight. Gross water content was determined from the difference. Once dry, the samples were digested in proteinase-K overnight at 56° C. Aliquots of digest were analyzed for GAG content using the 1,9-dimethylmethylene blue dye-binding assay. A further aliquot was acid hydrolyzed in 12 N HCl at 110° C. for 16 hours, dried over NaOH, and resuspended in assay buffer. Ortho-hydroxyproline (OHP) content was then determined via a colorimetric assay by reaction with chloramine T and dimethylaminobenzaldehyde, scaled for microplates. OHP content was converted to total collagen content using the conversion of 1:7.64 ratio of OHP:Collagen. DNA content was determined using the PicoGreen (Molecular Probes) assay following the manufacturer's standard protocols. Each biochemical constituent (GAG and collagen) was normalized to tissue wet weight.F. Histological Analysis.
Samples were fixed in acid formalin ethanol, paraffin embedded, sectioned (8 μm thick), and stained with either Safranin O (1% in dH20, pH 6.7) to view proteoglycan distribution, Picrosirius Red to view collagen distribution, or hematoxylin and eosin to view cell and tissue morphology. Samples were also stained for Type II collagen as follows: sections were digested in 0.5 mg/ml of testicular hyaluronidase, swollen in 0.5 M of acetic acid, blocked in 10% normal goat serum (NGS) and labeled with 10% NGS containing monoclonal primary antibody for types I and II collagens (Developmental Studies Hybridoma Bank). Non-immune controls were incubated in 10% NGS alone. Alexa 488-conjugated goat anti-mouse secondary antibody labeling and propidium iodide nuclear counterstaining were performed to visualize the ECM and cells, respectively. After staining, the slides were coverslipped and sections were analyzed using an inverted microscope with an Olympus Fluoview confocal system with dual wavelengths excitation at 488 and 568 nm (20× to 100×-oil objective lens).G. Statistics.
Statistics were performed with the Statistica (Statsoft) software package. Each data point represents the mean and standard deviation of four or five samples. Groups were examined for significant differences by two-way analysis of variance (ANOVA), with EY, G* (dynamic modulus), GAG, DNA, or OHP as the dependent variable, and time in culture and loading condition as the independent variables. Tukey's Honest Significant Difference Test (HSD) post-hoc tests were carried out with a statistical significance set at α=0.05.III. Results A. Study 1: The Effect of Transient TGF-β3 Exposure on Free Swelling Constructs
Constructs developed significantly different mechanical properties and biochemical composition depending on culture condition and time. In Study 1, performed in free-swelling cultures, constructs that were transiently exposed to TGF-β3 elaborated significantly stiffer tissue (EY=528±122 kPa, G*=2.9±0.3 MPa) than constructs that were exposed to TGF-β3 continuously (EY=165±42 kPa, G*=2.2±0.1 MPa) (
The results of Study 2 demonstrate the detrimental effects of dynamic deformational loading in the concurrent presence of TGF-β3 (
The results of Study 3 show that when loading was applied after the discontinuation of TGF-β3, the DDL group achieved mechanical properties (EY=1,306±79 kPa, G*=4.1±0.1 MPa) significantly higher than FS (EY=1,178±40 kPa, G*=3.5±0.2 MPa) (
Histological analysis confirmed abundant deposition of GAG throughout the constructs and a uniform distribution of type II collagen (FIGS. 24(1) and (2)) with little or no staining for type I collagen (not shown). Staining indicated that cells multiplied in localized pockets throughout the constructs (FIG. 24(3)). Cells proliferated with time, increasing on average 3-fold from day 0 concentrations, but did not differ significantly between any groups reported here. In
For comparison, the mechanical and biochemical properties of juvenile CMC articular cartilage were also measured (n=5) and were found to be EY=994±280 kPa, G* (at 1 Hz)=13±2.5 MPa, GAG=6.3±0.9 (% w/w), 24±3.5 (% d.w.), collagen=16±0.5 (% w/w), 66±5.5 (% d.w.). While EY for DDL and FS for Study 3 equaled or exceeded that of native cartilage by day 28 (
In this investigation a protocol of transient supplementation of serum-free media with TGF-β3 was adopted and a regimen of dynamic deformational loading was applied, the timing of which was adjusted towards achieving the most robust mechanical properties. The findings of this study indicate that coordination of the timing (introduction and duration) of the application of an appropriate chemical stimulus as well as the timing of the introduction of mechanical stimuli represents a strategy to optimize engineered tissue growth (i.e., a sequential loading protocol).
In Study 1, earlier results finding that discontinuation of TGF-β3 supplementation after two weeks in culture yields much better material properties than continuous supplementation were confirmed (
Related to this observation, collagen levels for constructs in all the studies presented here remained relatively low (
The results of this study address a number of important issues related to functional tissue engineering of articular cartilage. The most positive outcome is the finding that temporary supplementation of TGF-β3 followed by dynamic loading can produce an equilibrium modulus and GAG content which match those of native tissue over a culture period of 4 to 6 weeks only; the dynamic modulus and collagen content remain lower than in native tissue, but are as good as, or better than reported in previous studies.Example 4 Primed Mature Chondrocytes can Develop an Engineered Cartilage Tissue with Physiologic Properties
In previous studies, mature chondrocytes exhibited diminished proliferative and synthetic ability compared to younger cells. In this example, it is shown that growth factor treatment during passaging of adult cells leads to an engineered cartilage tissue with physiologic compressive stiffness.Materials and Methods A. Cell Culture.
Canine chondrocytes were isolated from shoulder and knee cartilage of adult mongrel dogs (2-5 years old, 90+ lbs.) according to the method described above. Cells were either used immediately after isolation or passaged in DMEM with 10% FBS, 1 ng/mL TGF-β1, 5 ng/mL FGF-2, and 10 ng/mL PDGF-BB. Primary (unpassaged) or passaged chondrocytes were suspended in 2% agarose at 30×106 cells/mL. Disks created as described above and having diameters of 0.4 mm and thicknesses of 1.5 mm (Ø4.0×1.5 mm) were cultured in 35 mL of chondrogenic media and ascorbate at 37° C. and 5% CO2. More specifically, the media consisted of hgDMEM supplemented with 1×PSF (100 units/ml penicillin, 100 μg/ml Streptomycin, 0.25 μg/mlFungizone (Amphotericin B)), 0.1 μM dexamethasone, 50 μg/ml ascorbate 2-phosphate, 40 μg/mL-proline, 100 μg/ml sodium pyruvate, and 1×ITS+(insulin, human transferrin, and selenous acid).
Primary chondrocyte-seeded hydrogels were cultured with 10 ng/mL TGF-β3 throughout the culture period (“P0 Continuous”). Passaged chondrocyte constructs were exposed to TGF-β3 either continuously (“P1 Continuous”) or only for the first 2 weeks in culture (“P1 2 W”). Media was changed every 48 h. A schematic of the experimental design is shown in 25.B. Mechanical Testing.
Young's modulus (EY) and dynamic modulus (G*) of samples (n=4-5 per group) were calculated from static and 0.1 Hz unconfined compression testing on day 0, 14, and 28. Following testing, constructs were weighed wet and frozen for biochemical analysis.C. Biochemical Analysis.
GAG and collagen contents were measured for each sample and normalized to construct wet weight (% w/w) according to the methods described above.D. Statistics.
Data were analyzed using 2-way ANOVA, with time and growth factor treatment as factors. Fisher LSD post-hoc test was used to determine significant differences (α=0.05).Results
Canine chondrocytes grown in monolayer culture with the growth factor cocktail reached confluence in 11 days, with an ˜8× increase in cell number. P0 Continuous constructs showed no changes in measured tissue properties over time in culture, with only an increasing trend in GAG content (d28: 1.0±0.6% w/w vs. d0: 0.2±0.1% w/w, p=0.583) (
The protocol used resulted in the successful expansion of mature chondrocytes that could form an engineered cartilage tissue with a Young's modulus in the physiologic range for native canine cartilage (˜200-500 kPa). The measured compressive stiffness and GAG content represent the highest reported values for engineered cartilage formed from mature chondrocytes. Canine chondrocytes have been shown to rapidly dedifferentiate during passaging without growth factor treatments and were therefore not included as a group in this study. The best results were achieved with continuous TGF-β3 treatment, consistent with mature bovine cells. This indicates that the use of TGF-β3 during 3D culture is translatable between adult cells of different species.Example 5 In Vivo Implantation of Chondral and Osteochondral Tissue-Engineered Constructs in a Canine Model
With focus on development of constructs suitable for repair of focal defects in the joint, cylindrical engineered osteochondral constructs resembling native osteochondral grafts of cartilage and underlying bone were developed. The advances in culture media formulation and development of the applied deformational loading protocol that are encompassed within the present invention have led to a robust culture protocol for cultivation of engineered tissue constructs with native properties of articular cartilage in less than 8 weeks. Together with an appropriate underlying substrate material, osteochondral constructs (stiffer than most described in the literature) with native chondral properties can be cultivated.
This example describes in vivo studies designed to assess the efficacy of the engineered tissues in a clinically-relevant large animal model. Chondral, osteochondral, and anatomically-shaped osteochondral constructs were developed. The engineered constructs used in these studies were produced using passaged, adult canine cells as described in the previous example and had native canine EY and GAG levels.Response of Canine Chondrocytes to Dynamic Deformational Loading
II. In Vivo Implantation
Either chondral (Study A) or osteochondral (gel-tantalum, Study B) constructs were implanted in the femur of adult mongrel dogs. In all studies, arthroscopic assessment and synovial fluid arthrocentesis were performed at 6 weeks with digital radiography, MRI, synovial fluid arthrocentesis, and arthroscopy performed at the time of sacrifice. Tissue was harvested and samples separated for material testing and subsequent biochemical composition analyses or histology.A. Study A: Chondral Implants.
In these in vivo studies, three full-thickness 4 mm defects were aseptically drilled through the cartilage and subchondral bone plate in the trochlear groove or lateral aspect of the lateral trochlear ridge of the femur of adult mongrel dogs (˜25 kg) to assess tissue repair with allogeneic chondrocyte-seeded engineered constructs possessing Young's moduli similar to native canine cartilage (
Chondral constructs in weight-bearing regions remained in place and appeared more hyaline-like. In contrast, constructs implanted in non-weight bearing regions exhibited some migration, exhibited significant subsidence and were weak in modulus (
These findings suggest that in vivo joint loading is important for engineered construct maintenance and remodeling in situ, and that collagen content of constructs can increase above those achievable in culture after implantation. From gross appearance and histology of unstained and H&E stained sections there is evidence of construct stability and early integration as suggested by the notable articular surface continuity associated with the entire perimeter of the construct.B. Study B: Osteochondral Implants.
For osteochondral constructs (
C. Synovium and Synovial Fluid Analyses.
In histological sections of harvested synovium (
Thus, using agarose as the gelable scaffold material yielded high mechanical and biochemical values and there was no evidence of an inflammatory response to agarose in vivo.D. Animal Lameness and Gross Appearance of Implant Sites of Chondral and Osteochondral Studies.
Animal lameness was scored on a scale from 0 to 5, with 5 being severe. For chondral and osteochondral constructs (n=5 animals), all had normal gait at 12 weeks except one dog that had very mild grade 1 of 5 intermittent lameness. The single animal with empty control defects showed grade 2 of 5 lameness at 12 weeks. No animals had palpable joint effusion and synovial fluid was clear and viscous upon examination after arthrocentesis. Additionally, some construct migration was noted for non-load-bearing sites whereas load-bearing samples showed excellent integration with surrounding cartilage and underlying bone. More subsidence was observed for chondral constructs, further motivating the use of chondral constructs supported by a bone or bone-substitute base for optimal cartilage resurfacing. Based on subjective arthroscopic assessment and India ink staining, the opposing surface of the patella was normal in all cases with no evidence for cartilage “kiss” lesions (e.g., fibrillation or erosion). No constructs were observed to fail under in vivo loading.Example 6 Measuring the Diffusion Coefficient of a Gelable Scaffold Material Materials and Methods A. Hydrogel Fabrication.
Sigma 2% type VII (VII) and 2% type IX (IX) agarose discs containing immature bovine chondrocytes at a final concentration of 30 million cells/ml were fabricated as described above and gelled at 25° C. and 4° C., respectively. Discs were cultured in serum-free, chemically-defined media, and TGF-β3 (10 ng/mL for the first 14 days of culture).B. Diffusivity Measurement.
Diffusion coefficients were measured by fluorescent recovery after photobleaching (FRAP). Constructs were incubated overnight in phenol red-free medium containing 0.5 mg/ml fluorescein isothiocynate (FITC)-conjugated 70 kDa dextran. This molecular weight is representative of large growth factors or matrix products commonly used or produced during culture. Each sample was then exposed to a high intensity monochromatic laser to induce localized photobleaching, and the recovery of fluorophores was modeled using Fick's law for one-dimensional diffusion with an initial Gaussian solute distribution to extract diffusion coefficients.C. Mechanical Testing.
Constructs were tested in unconfined compression with samples being loaded to 10% strain at a strain rate of 0.05% strain/sec, after an initial 0.02N tare load (EY). Dynamic modulus (G*) was measured by superimposing 2% peak-to-peak sinusoidal strain at 0.1 Hz.D. Biochemistry.
Constructs were proteinase K-digested, and glycosaminoglycan (GAG), collagen, and DNA content were determined using the DMMB dye-binding assay, orthohydroxyproline (OHP) assay, and Picogreen dsDNA assay, respectively.E. Histology.
Samples were fixed in acid formalin ethanol and paraffin embedded. 8 μm thick sections were stained with Alcian Blue and Picrosirius Red for proteoglycan and collagen distribution.F. Statistics.
A one-way ANOVA (α=0.05) with Tukey's HSD post-hoc tests was used to compare groups.II. Results
Hydrogel compositions were selected to provide similar initial diffusion coefficients for the two different agarose types (˜22 μm2/sec). Type VII agarose was significantly greater in initial modulus (Table 1).
With identical conditions and culture duration, however, type IX gels exhibited significantly higher mechanical properties and biochemical content (
Scaffolds have been fabricated with similar initial diffusion coefficients to control one parameter governing tissue development. In this study, both types of agarose constructs preserved the chondrocyte phenotype and promoted extracellular matrix development. However, over time, type IX gels exhibited increased properties over type VII constructs even though initial transport properties for dextran were similar. The EY and GAG content achieved for both gels in 6 weeks are comparable to that for wrist (carpo-metacarpal) bovine cartilage (EY: 994±280 kPa, GAG: 6.3±0.9% w/w).Example 7
This Example evaluates whether stiffer engineered cartilage constructs can be achieved by fostering development of tissues that possess central regions with properties more similar to the outer regions. In particular this Example examined the effects of (1) decreasing the initial thickness of the engineered constructs or (2) creating nutrient channels in the constructs, thereby shortening the effective diffusion distance for tissue development.
Example 7 includes three related studies examining matrix content and mechanical properties of chondral constructs produced according to varying methods. In Study 1 of Example 7, constructs of two different thicknesses (thick vs. thin) were compared. In Study 2 of Example 7, the efficacy of nutrient channels in thick constructs was investigated. In Study 3 of Example 7, the number of the channels was increased to study the effects of channels in larger diameter, thick constructs.Material and Methods for Example 7 A. Sample Preparation and Tissue Culture.
Chondrocyte-seeded agarose hydrogel disks were prepared using primary immature bovine chondrocytes (carpal/metacarpal joint) isolated via enzymatic digestion. Cells were encapsulated in 2% (w/v) low melting temperature agarose (Type VII, Sigma) in phosphate buffered saline at 30×106 cells/ml for Study 1 of Example 7 and 60×106 cells/ml for Studies 2 and 3 of Example 7.
In Study 1 of Example 7, the gel-cell mixture was cast into slabs of two different thicknesses: 0.78 (thin) and 2.34 mm (thick). Disks (diameter 4.00 mm) were cored from the slabs and cultured in defined serum-free chondrogenic medium (Dulbecco's Modified Eagle's Medium, 1% insulin transferrin selenium+Premix, 50 μg/mL-proline, 0.1 μM dexamethasone, 0.9 mM sodium pyruvate, antibiotics), supplemented with ascorbate (50 μg/ml). Recombinant human Transforming Growth Factor-b3 (10 ng/ml) (R&D Systems) was administered the first 2 weeks of culture. Culture media were changed three times a week.
In Study 2 of Example 7, a 1 mm diameter channel was created in the middle of the cell-seeded agarose disk (2.34 mm thick, and diameter 4.00 mm) using a biopsy punch (
For Study 3 of Example 7, 10 mm disks were punched and three 1 mm diameter channels were sub-cored in a centered equilateral triangular pattern, with a mutual separation of 4.3 mm.B. Mechanical Testing.
The spatially averaged mechanical properties of construct disks were evaluated at selected time points using a custom table top testing device. The EY was determined under unconfined compression at 10% strain, followed by tests for dynamic moduli (G*) at 0.1, 0.5, and 1 Hz and 1% strain amplitude. The actual area of the channels was deducted from the total cross-sectional area of the constructs for the stress calculations. The relative error introduced by any overestimation of the actual channel size, proportional to the ratio of the area of a 1 mm hole over a 4 mm disk, was expected to be no greater than about 6%. Following average property measurements, constructs were halved and tested for local axial mechanical properties under unconfined compression on a custom microscope testing device and using optimized digital image correlation (
One-half of each construct was weighed wet, lyophilized, reweighed dry, and digested in 0.5 mg/ml Proteinase-K (Fisher Scientific) at 56 C for 16 h. The PicoGreen assay (Invitrogen) was used to quantify the DNA content of the constructs with Lambda phage DNA (0-1 mg/ml) as a standard. The GAG content was measured using dimethylmethylene blue (DMMB, Sigma) dye-binding assay with shark chondroitin sulfate (0-50 mg/ml) as a standard. The overall collagen content was assessed by measuring the orthohydroxyproline (OHP) content via dimethylaminobenzaldehyde and chloramine T assay. Collagen content was calculated by assuming a 1:7.5 OHP-to-collagen mass ratio. The collagen and GAG contents were normalized to the disk wet weight.D. Histological Analysis.
The other halves of the constructs were fixed in a fixative solution (5% acetic acid, 3.7% formaldehyde, 70% ethanol) for 24 h and stored in 70% ethanol solution. After serial dehydration in ethanol, the constructs were embedded in paraffin, sectioned to 8 mm, and mounted onto microscope slides. The samples were then de-waxed, rehydrated, and stained with Safranin-O (Sigma) and Picrosirius red (Sigma) dyes to determine the distribution of GAG and collagen, respectively.E. Finite Element Modeling (FEM).
Osmotic swelling of the tissue-engineered constructs was modeled using a custom finite element program. The objective was to identify conditions that could replicate experimental findings of central cracking in one of the tested groups. The cylindrical engineered construct was divided into two concentric regions; an inner core and outer peripheral region, with respective sizes determined from polarized light images of construct histological slices. This assumption was based on the fact that increasing birefringence was observed in the constructs with increasing culture time and the pattern of histological staining roughly correlates with the pattern of the polarized light microscopy. A hexahedral mesh was created for one-eighth of the tissue-engineered construct with boundary conditions prescribed based on symmetry. Several combinations of material properties were explored, consistent with experimental measurements, which might explain the crack formation observed in the control group for Study 2 of Example 7. In the final analysis the tensile moduli of the respective regions were assigned values consistent with the intensity and distribution of Picrosirius red staining of collagen across the constructs, suitably scaled using an upper limit from experimental values previously reported. A tensile stiffness of 2.5 MPa and 120 kPa were thus assigned to the periphery and core of the mesh, respectively. GAG content was estimated to be 8% of the wet weight in the core and 10% in the periphery of the constructs based on the results of the GAG quantification assay. Assuming two negative charges per chondroitin sulfate isomer and a molecular weight of 513 g/mol, a fixed charge density (cF) was calculated from the GAG content to be 458 mEq/L (10% GAG) and 367 mEq/L (8% GAG). The water content was estimated to be 85% of wet weight based on the difference between the dry weight and wet weight of the constructs. The material properties used in FEM are summarized in Table 2.
Statistica (Statsoft) was used to perform statistical analyses using two way analysis of variance (ANOVA) and the Tukey honestly significant differences Post Hoc test of the means (n=4-6 samples per group) with culture duration and experimental groups as independent factors.Results of Study 1.
Study 1 of Example 7 showed the EY of the thin constructs were two-fold greater than that of the thick constructs, reaching values of 246±21 kPa and 592±111 kPa on days 32 and 48, respectively [P<0.005,
On day 48, the GAG content of the thin constructs reached 8.4±0.49% wet weight (% w/w) compared to thick constructs which had GAG content of only 4.8±0.23% w/w. The collagen content of the thin constructs was significantly higher than that of the thick constructs on both day 32 (1.71±0.31% w/w vs. 1.00±0.10% w/w, P<0.005) and day 48 (2.73±0.43% w/w vs. 2.36±0.19% w/w, P<0.05). The difference in collagen content between the two groups on day 48 was less than that on day 32. The thin constructs had a greater DNA content and GAG/DNA ratio as compared to the thick constructs after day 16. Increased GAG content in the thin constructs is attributable to both increased cell proliferation and elevated GAG production of individual cells.
Spatial EY profiles across the longitudinal depth of the cylindrical disks varied among the groups. The thin constructs had a significantly softer layer on the surface taking up a large part of the applied compressive strain and a uniformly stiff center with minimal strain [
Study 2 showed the process of punching channels did not affect cell viability at the cutting surface or other areas of the constructs. The moduli of the constructs with a channel were significantly higher than controls from day 28 onward. Furthermore, the moduli of the control disks (without a channel) started to plateau after day 28 and stagnated afterward until day 56, reaching values of EY=600 kPa and G*=2.7 MPa, respectively, whereas those of the disks with a channel continued to increase until day 42 and plateaued at a higher level of EY=1000 kPa and G*=3.6 MPa. The channel constructs also possessed more uniform local stiffness along the axial direction, whereas constructs without channels developed significantly stiffer edges and a softer central core as indicated by the U-shaped strain profile across the depth of the constructs [
The channels were gradually filled in with translucent material and infiltrated by cells [
A large crack parallel to the axial disk faces was observed in the center of the control constructs on day 56 [
For Study 3, large constructs of 10 mm diameter with channels developed significantly higher mechanical stiffness as compared to the control constructs without channels [
The results of Study 1 of Example 7 show that reducing the thickness of cell-seeded agarose constructs by one-third promotes more uniform material properties through the construct depth, as a result of the reduced transport path length. The mechanism underlying the softer outer layers observed in the thin constructs is unclear, and may be related to diffusive loss of GAG from the periphery. It appears that there may be a critical length >0.78 mm where diffusion limitations will lead to inhomogeneous cartilaginous tissue development under free-swelling culture conditions. While Study 1 showed that thin constructs developed superior material properties, there remains a clinical need for thicker tissue constructs (e.g., about 5 mm thick for the human patella or tibial plateau).
Study 2 showed that channels created on day 0 clearly provide many advantages, such as improved material properties and more homogeneous composition, and no apparent adverse effects. An array of channels can permit cultivation of single constructs having appropriate thickness, with the channels eventually filling naturally. The application of physiologic deformational loading with concomitant convective transport would be expected to further enhance the passive strategies to increase nutrient diffusion described in this investigation.
Diffusion channels with a diameter of less than about 1 mm became occluded within 1 week of culture, channels having a 1.5 mm diameter channels remained completely open after 28 days; and 1 mm diameter channels gradually shrank in size and were partially sealed up by day 28. Channels introduced at a late stage of culture, when the cells had already produced significant extracellular matrix, rather than immediately after construct fabrication on day 0, did not influence construct properties 14 days later. For the application of channels to be most efficacious, the channels should remain open long enough to play a role in providing greater nutrient access to chondrocytes when significant tissue matrix elaboration has occurred (and where a plateauing of tissue properties is often noted).
In Study 2, constructs (2.34 mm thick) were seeded with 60 million cells/ml, which is twice that of Study 1. This culture condition is expected to increase the effect of nutrient limitations on tissue development, with increases in construct dimension and nutrient consumption. The introduction of nutrient channels in the current study not only elevated construct stiffness but also delayed the plateauing of the mechanical properties of the constructs (
The central crack observed in the control constructs likely resulted from osmotic swelling due to GAG as well as low tensile stiffness in the center of the control constructs due to absence of organized collagen network as compared to the periphery. Cracks are not typically found in low seeding density (30 million cells/ml) constructs. Its occurrence in the high-seeding density constructs is reflective of the higher GAG content achieved with the higher seeding density. The finite element model provides insights to the structure-function relationships developed in the engineered cartilage tissue. In the engineered cartilage, GAG levels were similar to, or even higher than native levels (about 6% w/w), producing significant osmotic pressures (estimated at about 0.12 MPa when using ideal Donnan law) and swelling. Whereas swelling is resisted by the collagen matrix in native tissue, the constructs' collagen levels were only a fraction of the native values (about 20% w/w), and mostly deficient at the center of the construct. The FE model of a construct deficient in collagen at its center predicted a swelling strain there that was four times greater than in the peripheral region. As the yield strain for 2% w/v Type VII agarose is about 0.2, these results suggest that exceedingly high swelling-strains in the central region of the constructs may give rise to construct cracking. Therefore, the elevated GAG content and non-uniform distribution of collagen created conditions that supported internal cracking.
Applied mechanical loading has been shown to promote solute transport into cartilage and engineered constructs. However, the enhancement of nutrient transport into engineered constructs with dynamic loading will be less significant in constructs of larger dimension (such as targeted for repair of an entire articular surface) or with more elaborated matrix, which can hinder the transport of the nutrients. While mechanical loading continues to be attractive in promoting the growth of engineered cartilage (via a biophysical stimulus and enhanced transport), mechanical loading regimes can be supplemented by providing nutrient channels in the cell-seeded scaffolds, particularly when producing larger sized engineered tissue. While the introduction of channels or “holes” in the engineered cartilage may raise some concerns, the results of Example 7 indicate these channels are likely to completely seal themselves with additional culturing as the channels are beginning to be filled in with tissue by culture day 56. If constructs with unsealed channels were to be implanted, they would be expected to seal in vivo, as observations in the literature indicate that cartilage defects of less than 3 mm diameter heal spontaneously. In addition, clinically accepted cartilage repair strategies that use single or multiple osteochondral grafts also introduce irregular holes to the articular surface.Example 8 The Response of Adult Engineered Canine Cartilage to the Sequential or Combined Application of TGF-β3 and IGF-1
As described above, growth factor “priming” during monolayer expansion results in mature canine chondrocytes that can form an engineered cartilage tissue with physiologic tissue properties. These properties can be further improved with the addition of insulin-like growth factor-I (IGF-I) during culture. In the present example, this growth factor was added using two different temporal profiles since the timing and combination of various stimuli can elicit vastly different responses in engineered cartilage tissue.Materials and Methods A. Experimental Design.
The experimental design is shown in
Canine chondrocytes were isolated from the cartilage of adult mongrel dogs (2-5 years old, 90+ lbs.). Cells were passaged in DMEM with 10% FBS, 1 ng/mL TGF-β1, 5 ng/mL FGF-2, and 10 ng/mL PDGF-BB. Passaged chondrocytes were suspended in 2% agarose at 30×106 cells/mL. Disks (4.0 mm diameter×1.5 mm) were cultured in 35 mL of chondrogenic media and ascorbate at 37° C. and 5% CO2. TGF-β3 at 10 ng/mL was added for the first 14 days in culture and then the constructs were split in to three groups: TGF-β3 only (“+TGF−IGF”), IGF-I only (100 ng/mL, “−TGF+IGF”), or TGF-β3 with IGF-I (“+TGF+IGF”). Media was changed every 48 h.C. Mechanical Testing.
Young's modulus (EY) and dynamic modulus (G*) of samples (n=4-5 per group) was calculated from static and 1 Hz unconfined compression testing on day 0, 14, 28, and 42. Following testing, constructs were weighed wet and frozen for biochemical analysis.D. Biochemical Analysis.
GAG and collagen contents were measured for each sample and normalized to construct wet weight (% w/w).E. Statistics.
Data were analyzed using 2-way ANOVA (α=0.05), with time and growth factor treatment as factors. Fisher LSD post-hoc test was used to determine significant differences between means (p≦0.05).Results
Engineered canine cartilage cultured with TGF-β3 only (+TGF−IGF) improved in tissue properties by day 14 and continued to do so over the 42 day time period reaching values of EY˜150 kPa, G*˜1.2 MPa, GAG˜3.25% w/w, and collagen˜2.5% w/w (
The addition of IGF-I in combination with TGF-β3 led to the highest compressive Young's modulus and GAG content in the engineered cartilage tissues cultivated in this study, comparable to previously measured values for canine patella-femoral groove cartilage. The results between the sequential substitution and combination of TGF-β3 with IGF-I imply that there exists “cross talk” between growth factor signaling in adult canine chondrocytes. From a clinical perspective, the results reinforce the potential to expand mature allogeneic or autologous chondrocytes for regenerative medicine strategies (tissue engineering, ACI).
1. A method for culturing chondrocytes for incorporation into a biocompatible implant, the method comprising:
- passaging a plurality of adult living chondrocytes in the presence of one or more growth factors,
- suspending the chondrocytes in a gelable scaffold material,
- culturing the chondrocytes and the gelable scaffold material in a medium comprising transforming growth factor-beta3 (TGF-beta3).
2. The method of claim 1 further comprising casting the suspension of chondrocytes and gelable scaffold material into one or more slabs.
3. The method of claim 2 further comprising coring the one or more slabs to create one or more disks.
4. The method of claim 1 further comprising securing the suspension of chondrocytes and gelable scaffold material to a biocompatible porous substrate.
5. The method of claim 4 wherein the securing comprises transferring the suspension of chondrocytes and gelable scaffold material to a mold and immersing the biocompatible porous substrate into the chondrocytes and gelable scaffold material, the porous substrate being substantially free of trabecular bone.
6. The method of claim 5 wherein the biocompatible porous substrate comprises a metal.
7. The method of claim 5 wherein the biocompatible porous substrate comprises tantalum.
8. The method of claim 5 wherein the porous substrate comprises a porous substrate selected from the group consisting of synthetic polymers and biologic materials.
9. The method of claim 8 wherein the synthetic polymer is selected from the group consisting of polycaprolactone, poly-l-lactic acid, and polyglycolic acid.
10. The method of claim 8 wherein the biologic material is selected from the group consisting of collagen and hydroxyapatite.
11. The method of claim 1 wherein the passaging comprises passaging chondrocytes obtained from an autologous donor.
12. The method of claim 1 wherein the passaging comprises passaging chondrocytes obtained from an allogeneic donor.
13. The method of claim 1 wherein the passaging comprises passaging adult canine chondrocytes.
14. The method of claim 1 wherein the passaging comprises passaging the chondrocytes in the continuous presence of one or more growth factors.
15. The method of claim 1 wherein the suspending comprises suspending the chondrocytes in an agarose gelable scaffold material.
16. The method of claim 1 wherein the suspending comprises suspending the chondrocytes in a low-melt agarose gelable scaffold material.
17. The method of claim 1 wherein the suspending comprises mixing a volume of a chondrocyte suspension with an approximately equal volume of about 4% agarose to yield a final agarose concentration of about 2%.
18. The method of claim 1 wherein the suspending comprises suspending the chondrocytes in the gelable scaffold material to yield a chondrocyte concentration of about 10 million cells/ml to about 60 million cells/ml.
19. The method of claim 18 wherein the suspending comprises suspending the chondrocytes in the gelable scaffold material to yield a chondrocyte concentration of about 30 million cells/ml.
20. The method of claim 1 wherein the culturing comprises culturing the chondrocytes and gelable scaffold material for a period of about 28 days to about 60 days.
21. The method of claim 20 wherein the culturing comprises culturing the chondrocytes and gelable scaffold material for a period of about 8 weeks.
22. The method of claim 1 wherein the culturing comprises culturing the chondrocytes and gelable scaffold material for 60 days with continuous TGF-beta3 supplementation.
23. The method of claim 1 wherein the culturing comprises culturing the chondrocytes and gelable scaffold material in a medium which is substantially serum-free.
Filed: Dec 12, 2013
Publication Date: Apr 3, 2014
Applicants: The Trustees of Columbia University in the City of New York (New York, NY), THE CURATORS OF THE UNIVERSITY OF MISSOURI (Columbia, MO)
Inventors: Clark T. Hung (Ardsley, NY), Gerard A. Ateshian (New York, NY), Eric G. Lima (Patterson, NY), James L. Cook (Columbia, MO), Li Ming Bian (New York, NY)
Application Number: 14/104,600
International Classification: B29C 39/00 (20060101); B29C 39/10 (20060101); C12N 5/077 (20060101);