A composite living skin equivalent is described comprising an epidermal layer of cultured keratinocyte cells, a layer of non-porous collagen, and a dermal layer of cultured fibroblast cells in a porous cross-linked collagen sponge matrix. Preferably the non-porous collagen is Type 1, Type 3 or mixtures of Types 1 and 3 bovine collagen, which has been pepsin treated. A process for preparing the skin equivalent is described, as well as a test kit for in vitro testing of the skin equivalent. The skin equivalent has use for skin grafting as well as in vitro testing of the effects of various substances on skin.
The questions raised in reexamination request No. 90/003,418, filed Apr. 25, 1994, have been considered and the results thereof are reflected in this reissue patent which constitutes the reexamination certificate required by 35 U.S.C. 307 as provided in 37 CFR 1.570(e).
|
1. A composite living skin equivalent which comprises relative to a horizontal plane:
a) a sponge first layer comprising a cross-linked collagen sponge, said first layer having upper and lower surfaces, said sponge containing cultured fibroblast cells therein, b) a non-porous second layer comprising a high purity non-porous collagen essentially free of exogenous glycosaminoglycans, said second layer having upper and lower surfaces, the lower surface thereof being in contact with the upper surface of said first layer, and c) a layer comprising cultured keratinocyte cells in contact with the upper surface of said non-porous collagen second layer.
2. The composite living skin equivalent of
3. The composite living skin equivlent of claim 2 14 wherein the collagen of at least one of the layers is bovine source derived.
4. The composite living skin equivalent of
5. The composite living skin equivalent of
6. The composite living skin equivalent of
7. The composite living skin equivalent of
8. The composite living skin equivalent of
9. The composite living skin equivalent of
10. The composite living skin equivalent of
11. The composite living skin equivalent of
12. A composite living skin equivalent which comprises relative to a horizontal plane:
a) a sponge first layer comprising a cross-linked collagen sponge, said first layer having upper and lower surfaces, said sponge containing cultured fibroblast cells therein, b) a non-porous gel second layer comprising a high purity collagen essentially free of exogenous glycosaminoglycans, said second layer having upper and lower surfaces, the lower surface thereof being in contact with the upper surface of said first layer, and c) a layer comprising cultured keratinocyte cells in contact with the upper surface of said non-porous collagen second layer. 13. The composite living skin equivalent of
glycosaminoglycans. 14. The composite living skin equivalent of claim 13 wherein said sponge first layer is derived from collagen which is essentially free of exogenous denatured collagen. |
|||||||||||||||||||||||||||||
The present invention relates to living skin equivalents and, in particular, to composite living skin equivalents comprising an epidermal layer of cultured keratinocyte cells, a layer of highly purified, non-porous collagen and a dermal layer of cultured fibroblast cells in a porous, cross-linked collagen sponge. The invention also relates to a method of preparing the composite living skin equivalent.
Skin equivalents have many uses not only as a replacement for human or animal skin for skin grafting, but also as test skin for determining the effects of pharmaceutical substances and cosmetics on skin.
A major difficulty in pharmacological, chemical and cosmetic testing is the difficulties in determining the efficacy and safety of the products on skin. One advantage of the skin equivalents of the invention is their use as an indicator of the effects produced by such substances through in vitro testing on test skin.
Also, skin grafting of denuded areas, of granulating wounds and of burns, still present major healing problems despite advances in grafting techniques. Split thickness autografts and epidermal autografts (cultured autogenic keratinocytes) have been used with variable success. However, both forms of treatment have many disadvantages. For example, split-thickness autografts are generally unavailable in large body surface area (BSA) burns, cause further injury to the patient, are of limited use in the treatment of patients with Dystrophic Epidermolysis bullosa (DEB), show limited tissue expansion, require repeated surgical operations and protracted hospitalization and give rise to undesirable cosmetic results. Epidermal autografts require time to be produced, have a low success ("take") rate of between 30-50%, often form spontaneous blisters, are fragile and difficult to handle, exhibit contraction to 60-70% of their original size, are vulnerable during approximately the first 15 days after grafting and are of virtually no use in the treatment of deep burns where both the dermis and epidermis have been destroyed.
An alternative form of treatment is epidermal allografts (cultured allogenic keratinocytes). American researchers have treated patients with second degree burns by grafting epidermal allografts onto wounds with some success. The benefits of such an allograft include a ready supply of such grafts can be maintained so that the patients might be covered in a single procedure with a material which allows permanent healing to occur, it eliminates autografting which increases the area of wounds and leaves painful infection-prone donor sites, burn wounds covered with cultured allografts heal as quickly as burn wounds that have been covered with autografts, and enables the treatment of patients with DEB.
However, epidermal allografts still experience many of the limitations of epidermal autografts.
Full thickness skin injuries from burns destroy both the epidermis and dermis, and treatment with cultured skin needs to replace both of these components.
Hansborough, J. F and Boyce, S. T (JAMA 1989, 2125-2130) reported the application of auto epidermal cells onto a dermal equivalent which is then grafted onto a wound. The main disadvantage of this method lies in the preparation of the dermal equivalent.
Furthermore, this method involved the use of chondroitin-6-sulfate (GAG) which has weak bonding to the collagen at neutral pH, and thus may be released into the wound environment causing unforeseen long term effects on human subjects. GAG has been reported to increase scar formation in wounds which is something to be avoided in grafts. Another effect of GAG containing collagen sponges consisting in reduction of collagen blood clotting capacity can be considered rather unfavourable for application in bleeding wounds. Fibrin clot contributes to an adhesion of the graft to the wound.
Also, in this method, the collagen sponge is stabilized by being crosslinked with with 0.25% glutaraldehyde (GTA). Such crosslinked collagen is resorbed at a slower rate and is resistant to bacterial or fungal infection. At the same time the ingrowth of cells, infiltrating the GTA crosslinked collagen matrix is less. Collagen crosslinked with GTA may retain this agent as a high molecular weight polymer which is continuously hydrolyzed and monomeric GTA is released and detactable for up to 6 weeks. The cytotoxic effect of GTA on fibroblasts in tissue culture suggests that it is not an ideal crosslinking agent for a dermal equivalent which is infiltrated by hosts cells and in which the bovine collagen matrix is rapidly degraded thus releasing GTA into body fluids.
Recently, living skin equivalent grafts comprising a dermal layer of rat fibroblast cells cast in soluble collagen and a epidermal layer of cultured rat keratinocytes were successfully grafted as allografts onto Sprague Dawley rats by Bell et.al. (Journal Investigative Dermatology, 1983; 81:2s-10s). Histological examination of the graft revealed that the epidermal layer had fully differentiated to form desmosomes, tonofilaments, keratohyalin and a basement lamella. However, attempts to reproduce the living skin equivalent using human fibroblasts and keratinocytes met only with limited success. The keratinocytes failed to fully differentiate to form a basement lamella and the dermo-epidermal function was a straight line.
Problems of epidermalizing the surface of the above dermal equivalent resulted in Bell modifying his method by using skin biopsies as a source of keratinocytes, as described in the International PCT application, published as WO 86/02273. The problems with this approach are that the skin substitute thus produced is not uniform over its entire surface, since the biopsy, including the dermal portion, remains inserted in the dermis substitute. Also, the surface-area of the skin substitute obtained is limited by the number of biopsies that may be taken from a single person. The biopsy taking involve a medical procedure with potential problem of infection and scar formation. The punch biopsies of skin equivalent as a means of expanding the production of additional skin equivalent is a time consuming process. As a result, such a skin equivalent has not been used clinically. In 1988, a paper in the journal "Burns" by Colounb et al reported a 100% failure rate using Bell's method.
Bernard et al, the inventors of Australian Patent Application AU-A-13743/88 try to avoid the above problems by utilizing the culturing capacity of keratinocytes contained in the sheath of a hair follicle. The skin biopsy is replaced by a hair follicle enclosed in its sheath, which is implanted in a perpendicular position in the free surface of dermis substitute being formed. The main criticism of the above invention is the nature of the dermis and the fact that the period of epidermal growth may take several months.
Thus, there is a need for the development of living skin equivalent grafts comprising both the epidermal and dermal layers that can be easily prepared and maintained in sufficient quantities to enable a single treatment of skin wounds.
In developing a living skin equivalent it is desirable that it comprise at least some or all of the following features: it should enable rapid and sustained adherance to the wound surface, it should be tissue compatable, it should have an inner surface in contact with the wound surface that promotes the ingrowth of fibrovascular tissue, and/or it should provide protection from infection and prevention of fluid loss.
It is therefore an object of the present invention to provide cultured living skin equivalents that exhibit at least some of these features and which will substantially overcome, or ameliorate one or more of the abovementioned problems.
One aspect of the present invention concerns composite living skin equivalents comprising an epidermal layer of cultured keratinocyte cells, a layer of high purity, non-porous collagen and a dermal layer of cultured fibroblast cells in a porous, cross-linked collagen sponge.
Another aspect of the present invention involves a process for the preparation of composite living skin equivalents which comprises: obtaining a skin sample, treating the skin sample enzymically to separate the epidermis from the dermis, treating the epidermis enzymically to release the keratinocyte cells, culturing the epidermal keratinocytes until confluence, in parallel, or separately, treating the dermis enzymatically to release the fibroblast cells, culturing the fibroblasts cells until sub-confluence, inoculating a porous, cross-linked collagen sponge membrane with the cultured fibroblast cells, incubating the inoculated collagen sponge on its surface to allow the growth of the fibroblast cells throughout the collagen sponge, inverting the collagen sponge, and laminating the other surface of the sponge with a thin layer of high purity, preferably pepsin treated, nonporous collagen to form a layered sponge complex, incubating the complex to polymerize the non-porous collagen, and then inoculating it with cultured keratinocyte cells, and incubating the composite skin equivalent complex to promote the growth of the cells.
Preferably the primary culture of fibroblasts is prepared by: obtaining a dermal sample, suspending the dermal sample in a solution of collagenase to release the fibroblast cells, incubating the culture, centrifuging the culture to produce a cell pellet of fibroblasts, removing the culture medium, washing the cell pellet to remove extraneous culture medium, determining the cell number and viability, inoculating culture flasks with the cells and culturing to subconfluence.
Preferably the non-porous, highly purified collagen is selected from Type 1, type 3, or mixtures of type 1 and type 3 collagen. For example, a suitable bovine hide collagen is that obtainable from Sigma.
The collagen is purified ideally by treatment with pepsin, to remove antigenic substances.
The collagen sponge used can be any suitable such collagen sponge, for example that obtainable from Mitaplast.
The keratinocytes used in the invention are preferably prepared by the "drop" method. The keratinocytes are released from the epidermis to provide a single cell suspension. Separate drops of this suspension are spotted evenly on culture media and incubated, so that the cells spread and eventually coalesce.
The invention will now be described by way of non-limiting examples and with reference to the accompanying illustrations wherein;
FIG. 1 is a schematic representation of the process for producing the composite living skin equivalents of the present invention.
FIG. 2 a) shows the histological appearance of the composite living skin equivalent 10 mg/ml 10 ng/ml human epidermal growth factor, 0.4 mg/ml hydrocortisone and 10-9 M cholera toxin at pH 7.2 and 35°C for 10 days.
The skin equivalent remains immersed in the above culture medium throughout the incubation period.
Prior to the clinical or in vitro application of the composite living skin equivalent, medium without bovine pituitary extract is added to the culture medium.
Surprisingly, in clinical applications, the composite living skin equivalent of the present invention results in a rapid normalization of the interface between the epidermis and dermis of the healed transplants. Histological examination of the skin equivalent of the present invention after 2 weeks culture in vitro revealed a multilayered epidermis growing on a homogeneous membrane. Histological examination of a biopsy sample of a skin equivalent of the present invention taken 2 weeks after grafting confirmed the formation of stratun corneum with a fully keratinized epidermis on a dermis populated by non-inflammatory connective tissue cells (refer FIG. 2a). Significantly there is an undulating and morphologically mature epidermal-dermal junction when viewed by light and electron-microscopy. There was an interdigitations of rete ridges and dermal papillae that are characteristic of normal skin and are important if the interface between the epidermis and the dermis are to be normalized.
If the skin equivalent is cultured initially immersed for 4 days in the DMEM culture medium with a Ca++ of 0.05×10-3 M and then for 10 days with the epidermis exposed (air liquid interphase) in DMEM medium containing a raised concentration of Ca++ of 0.05×10-3 M then its possible to detect a multilayered, differentiated epidermis which consists of a basal cell layer on a well developed basal lamina and several layers of suprabasal cells which show early keratinization.
The above in vitro system closely resembles human skin instructural arrangement and biosynthetic output and may be adapted to test the safety of chemicals pesticides and skin irritation of cosmetic substances. Test substances applied to the surface of this system may cause irritation of the cells and trigger the release of mediators of the inflammatory response which can be measured in the culture fluid. This system may be suitable for in vitro cytotoxicity testing: the total cellular-protein assay and the neutral red uptake assay which measure protein concentration in cells provide a quantifiable assay for the presence of living and dead cells.
The skin equivalent can be cultured in glass bottles or dishes, and the various chemicals to be tested applied to this cultured skin. By continuing to supply suitable culture media the skin will continue to grow until the test is complete.
The collagen sponge provides a temporary matrix which enables the rapid and sustained adherence of the composite living skin equivalent to a wound surface, in a human or animal, which provides a surface in contact with the wound surface that allows fibrovascular ingrowth from the wound surface and which allows for neodermal structures to develop. The collagen matrix is altered and gradually broken down and replaced by endogenous collagen as the fibroblasts interact with it physically and contribute to it biosynthetically. However, as the collagen sponges are cross-linked collagen, they do not contract and so can be stored for some time, and do not exhibit contraction when grafted onto wounds.
The pepsin-treated, non-porous collagen placed on the upper surface of the collagen sponge prevents invasion of the collagen sponge by cultured keratinocyte cells and thus ensures the compartmentalization of the skin equivalent into epidermal and dermal layers. This laminate layer is also gradually broken down to allow the normal interface between the dermis and epidermis to form.
The composite living skin equivalents of the present invention are approximately 0.8 mm thick and are therefore stronger than epidermal grafts and more easily handled during grafting. The success ("take") rate for the skin equivalents of the present invention is approximately 90%, which may be attributed to the presence of the dermal layer which promotes development of vascularization of the graft. Finally, the composite living skin equivalents of the present invention enables the graft to be applied in one stage, thereby requiring a only a single graft acceptance event. To facilitate transport and application of the composite living skin equivalent, vaseline gauze may be placed over the cultured graft.
The fibroblasts and keratinocytes used in accordance with the present invention may be either autogenic or allogenic. The use of allogenic cells enables the production and storage of the living skin equivalent of the present invention thereby avoiding delays in procuring grafts for the treatment of wounds. Both cell types, keratinocytes and fibroblasts could be stores frozen for months as single cell suspensions, using published methods. After thawing these cells were viable and grew readily in culture and thus were suitable to be sued for the production of skin equivalent. The skin equivalent has been grafted successfully to a human volunteer. Since cooling supresses the immunogenicity of skin grafts (Baldwin WM et al. Transplantation 1973; 15:419-422) cryopreservation of allogenic cells helps in attenuating some undesirable antigens. The availability of composite living skin equivalents for the treatment of surface area wounds can provide a virtually unlimited quantity of graftable skin as a source of permanent wound coverage.
The present invention will now be described in the following examples using human allogenic skin cells.
Composite grafts were made from separate, parallel cultures of allogenic human keratinocytes (HK) and human fibroblasts (HF) and a cellular bovine collagen membrane. The dermal membrane was modified using type 1 bovine collagen to provide a planar surface for cultured HKs.
Human skin was obtained from surgical specimens i.e. neonatal circumcision (foreskin). After the excision the skin was placed in a sterile container with Dulbecco's modified Eagle's medium (DMEM). Specimens were delivered within a short time to the tissue culture laboratory where the epidermis was separated from the dermis enzymically according to the method of Eisinger, M (Method in Skin Research, Editor D. Skerrow 1985 p193).
Keratinocytes were cultured as a single cell suspension by the method of Eisinger which was modified as follows: HKs were cultured in DMEM supplemented with 2% fetal bovine serum, epidermal growth factor, insulin and hydrocortisone at pH 7.2. Confluent cultures were ready for harvest after 12 to 14 days either for subculture or for inoculation onto the collagen membrane.
Fibroblasts were released from dermal fragments by digesting these with Clostridium histolyticum collagenase. HFs were then grown in DMEM using standard methods.
The collagen sponge members (6 cm diameter), stored frozen in Petri dishes, were washed with sterile water and dehydrated in an incubator at 37°C in order to compact the membranes. The sponges were then incubated overnight in DMEM supplemented with conditioned medium. Subconfluent cultures of HFs were innoculated at a density of 4×105 cells/ml onto the surface of the sponge. The sponge was then placed in DMEM in an incubator at 37°C, 5% carbon dioxide and saturated humidity for 10 days.
Medium was changed every second day. At the end of that period the sponges were turned over and a nonporous surface was prepared to provide a planar surface for cultured HKs.
Lamination was performed by applying a thin film of pepsin-treated, non-porous, sterile type 1 bovine collagen. The films were prepared from commercially available purified type 1 collagen which was pepsinized to remove teliopeptides and sterilized by Gamma radiation. The collagen solution was brought to neutral pH and applied as a thin film onto the surface of the collagen sponge and incubated for 60 minutes at 37° C.
Cultured HKs were then innoculated in drops at a density of 1×105 per drop on to the nonporous surface of the sponge and incubated for 10 days in DMEM with supplements mentioned above. Before clinical application culture medium without bovine pituitary extract was added to the culture dishes. Vaseline gauze was placed over the cultured graft to facilitate the transporting and securing of the graft to the wound bed.
In 8 operations performed on 5 children using the living skin equivalents of the present invention; the success rate was 90%.
Clinical and histological appearance of the above grafts in the eight operations of the DEB children suggested that there was no rejection.
However, in order to determine direct evidence of the long term survival of cultured allografts or their contribution to permanent epithelium, clinical trials were performed on healthy adult volunteers described in the o following example.
Composite grafts and allografts were derived the same way as outlined in Example 1. Having providing a planar surface for cultured keratinocytes, human keratinocytes attached to the surface of the cross linked bovine collagen substrate. This "skin culture sandwich" was then transplanted on bloc on to the wound bed of human patients where the collagen matrix served as a framework to allow fibrovascular ingrowth from the underlying wound bed thus permitting human keratinocytes survival, and the formation of the neodermal structures.
Clinical studies were performed on four volunteers for the removal of decorative tatoos. Each volunteer had four skin areas excised on an arm. In two areas, the skin was excised down to the fat while the remaining two excisions left dermal elements in place. Full depth and partial thickness excissions were grafted with cultured skin and split thickness autograft skin (as controls). Weekly dressings were performed until the wounds were completely healed. The wounds were photographed, biopsies were performed for histology and DNA fingerprinting.
Volunteer 1 had two areas grafted with cultured skin and the other two with an autograph. After 2 weeks the grafts had taken and there was no evidence of graft contraction. Biopsies of the central area of the grafts had a well differentiated and multilayered epidermis, and the dermis contained numerous fibroblasts and non-inflamatory cells in a loosely packed collagen matrix. FIGS. 3 and 5 show the histology of a skin biopsy from a cultured graft, 2 weeks post-operatively. FIG. 4 shows the skin equivalent before grafting. DNA fingerprinting indicated that there was a mixed population of cells both donor and recipient indicating that some of the dermal cells were derived from the patients since there was evidence of marked dermal cellularity.
Volunteer 2. The graft did not take in any of the areas. At three weeks there was histological evidence of a granulating wound.
Volunteer 3. After 4 weeks all the grafts had healed without any contraction. From a histology examination, there was a fully differentiated epidermis and a hypecellular dermis. DNA fingerprinting showed a mixed population of donor and recipient cells.
Volunteer 4. After 8 weeks the graft showed some contraction (approximately 15-20%) with the central graft area of this patient had a fully differentiated epidermis and a mature dermis without adnexae.
It should be obvious to persons skilled in the art that numerous variations and modifications could be made to the invention as described above, without departing from the overall scope and spirit of the present invention.
| Patent | Priority | Assignee | Title |
| 10070948, | Jun 27 2008 | Sofradim Production | Biosynthetic implant for soft tissue repair |
| 10073085, | Mar 29 2011 | TORAY INDUSTRIES, INC | Method for producing artificial skin model, and artificial skin model |
| 10080639, | Dec 29 2011 | Sofradim Production | Prosthesis for inguinal hernia |
| 10159555, | Sep 28 2012 | Sofradim Production | Packaging for a hernia repair device |
| 10184032, | Feb 17 2015 | Sofradim Production | Method for preparing a chitosan-based matrix comprising a fiber reinforcement member |
| 10213283, | Jun 07 2013 | Sofradim Production | Textile-based prosthesis for laparoscopic surgery |
| 10327882, | Sep 29 2014 | Sofradim Production | Whale concept—folding mesh for TIPP procedure for inguinal hernia |
| 10342652, | Dec 29 2011 | Sofradim Production | Barbed prosthetic knit and hernia repair mesh made therefrom as well as process for making said prosthetic knit |
| 10363690, | Aug 02 2012 | Sofradim Production | Method for preparing a chitosan-based porous layer |
| 10368971, | Dec 03 2007 | Sofradim Production | Implant for parastomal hernia |
| 10405960, | Jun 07 2013 | Sofradim Production | Textile-based prothesis for laparoscopic surgery |
| 10472750, | Mar 16 2011 | Sofradim Production | Prosthesis comprising a three-dimensional and openworked knit |
| 10646321, | Jan 25 2016 | Sofradim Production | Prosthesis for hernia repair |
| 10653508, | Sep 29 2014 | Sofradim Production | Textile-based prosthesis for treatment of inguinal hernia |
| 10660741, | Apr 24 2015 | Sofradim Production | Prosthesis for supporting a breast structure |
| 10675137, | May 02 2017 | Sofradim Production | Prosthesis for inguinal hernia repair |
| 10682215, | Oct 21 2016 | Sofradim Production | Method for forming a mesh having a barbed suture attached thereto and the mesh thus obtained |
| 10709538, | Jul 13 2011 | Sofradim Production | Umbilical hernia prosthesis |
| 10743976, | Jun 19 2015 | Sofradim Production; Covidien LP | Synthetic prosthesis comprising a knit and a non porous film and method for forming same |
| 10745835, | Dec 05 2014 | Sofradim Production | Prosthetic porous knit |
| 10815345, | Feb 17 2015 | Sofradim Production | Method for preparing a chitosan-based matrix comprising a fiber reinforcement member |
| 10865505, | Sep 04 2009 | Sofradim Production | Gripping fabric coated with a bioresorbable impenetrable layer |
| 11039912, | Jul 13 2011 | Sofradim Production | Umbilical hernia prosthesis |
| 11266489, | Dec 29 2011 | Sofradim Production | Barbed prosthetic knit and hernia repair mesh made therefrom as well as process for making said prosthetic knit |
| 11291536, | Sep 29 2014 | Sofradim Production | Whale concept-folding mesh for TIPP procedure for inguinal hernia |
| 11304790, | Jun 07 2013 | Sofradim Production | Textile-based prothesis for laparoscopic surgery |
| 11359313, | Dec 05 2014 | Sofradim Production | Prosthetic porous knit |
| 11389282, | Jan 25 2016 | Sofradim Production | Prosthesis for hernia repair |
| 11439498, | Apr 24 2015 | Sofradim Production | Prosthesis for supporting a breast structure |
| 11471256, | Dec 29 2011 | Sofradim Production | Prosthesis for inguinal hernia |
| 11471257, | Nov 16 2018 | Sofradim Production | Implants suitable for soft tissue repair |
| 11589974, | Sep 29 2014 | Sofradim Production | Textile-based prosthesis for treatment of inguinal hernia |
| 11612472, | Mar 16 2011 | Sofradim Production | Prosthesis comprising a three-dimensional and openworked knit |
| 11622845, | Jun 07 2013 | Sofradim Production | Textile-based prothesis for laparoscopic surgery |
| 11672636, | May 02 2017 | Sofradim Production | Prosthesis for inguinal hernia repair |
| 11696819, | Oct 21 2016 | Sofradim Production | Method for forming a mesh having a barbed suture attached thereto and the mesh thus obtained |
| 11713526, | Dec 05 2014 | Sofradim Production | Prosthetic porous knit |
| 11826242, | Jun 19 2015 | Sofradim Production | Synthetic prosthesis comprising a knit and a non porous film and method for forming same |
| 11903807, | Jul 13 2011 | Sofradim Production | Umbilical hernia prosthesis |
| 6040493, | Apr 24 1998 | REPLICATION MEDICAL, INC | Bioreactor wound dressing |
| 6498138, | Mar 11 1998 | SOUTHERN CALIFORNIA, UNIVERSITY OF | Method of promoting production of living tissue equivalents |
| 6605466, | Apr 20 1999 | SOCIETE L OREAL S A | Epidermis/dermis equivalents and aged skin equivalents shaped therefrom |
| 6660522, | Apr 20 1999 | Societe l'Oreal S.A. | Epidermis/dermis equivalents and aged skin equivalents shaped therefrom |
| 6890754, | Apr 20 1999 | L'Oreal | Epidermis/dermis equivalents and aged skin equivalents shaped therefrom |
| 8822215, | Jun 20 2008 | Escape Therapeutics, Inc. | Differentiation of mesenchymal stem cells into fibroblasts, compositions comprising mesenchymal stem cell-derived fibroblasts, and methods of using the same |
| 9242026, | Jun 27 2008 | Sofradim Production | Biosynthetic implant for soft tissue repair |
| 9308068, | Dec 03 2007 | Sofradim Production | Implant for parastomal hernia |
| 9347045, | Jun 20 2008 | Escape Therapeutics, Inc. | Differentiation of mesenchymal stem cells into fibroblasts |
| 9382514, | Jun 20 2008 | ESCAPE THERAPEUTICS, INC | Compositions comprising mesenchymal stem cell-derived fibroblasts |
| 9445883, | Dec 29 2011 | Sofradim Production | Barbed prosthetic knit and hernia repair mesh made therefrom as well as process for making said prosthetic knit |
| 9499927, | Sep 25 2012 | Sofradim Production | Method for producing a prosthesis for reinforcing the abdominal wall |
| 9526603, | Sep 30 2011 | Sofradim Production | Reversible stiffening of light weight mesh |
| 9554887, | Mar 16 2011 | Sofradim Production | Prosthesis comprising a three-dimensional and openworked knit |
| 9622843, | Jul 13 2011 | Sofradim Production | Umbilical hernia prosthesis |
| 9750837, | Sep 25 2012 | Sofradim Production | Haemostatic patch and method of preparation |
| 9839505, | Sep 25 2012 | Sofradim Production | Prosthesis comprising a mesh and a strengthening means |
| 9877820, | Sep 29 2014 | Sofradim Production | Textile-based prosthesis for treatment of inguinal hernia |
| 9931198, | Apr 24 2015 | Sofradim Production | Prosthesis for supporting a breast structure |
| 9932695, | Dec 05 2014 | Sofradim Production | Prosthetic porous knit |
| 9980802, | Jul 13 2011 | Sofradim Production | Umbilical hernia prosthesis |
| Patent | Priority | Assignee | Title |
| 4016036, | Nov 14 1975 | Massachusetts Institute of Technology | Process for serially culturing keratinocytes |
| 4024020, | Dec 15 1975 | Monsanto Company | Method of cell culture on polyacrylonitrile surface |
| 4060081, | Jul 15 1975 | Massachusetts Institute of Technology | Multilayer membrane useful as synthetic skin |
| 4107937, | Dec 22 1975 | Linde Aktiengesellschaft | Method of and apparatus for the deep freezing of biological substances |
| 4117881, | Jun 14 1977 | The United States of America as represented by the Administrator of the | System for and method of freezing biological tissue |
| 4135975, | Dec 14 1977 | RESEARCH CORPORATION TECHNOLOGIES, INC | Obtaining human cell lines that elaborate colony stimulating activity for marrow cells of man and other species and methods of preparing same |
| 4144126, | May 21 1975 | Beecham Group Limited | Cell culture method |
| 4228243, | Nov 16 1976 | Toray Industries, Inc. | Cell culture propagation apparatus |
| 4254226, | Jan 02 1979 | SLOAN KETTERING INSTITUTE FOR CANCER RESEARCH | Process for growing human epidermal cells in tissue culture |
| 4280954, | Jul 15 1975 | Massachusetts Institute of Technology | Crosslinked collagen-mucopolysaccharide composite materials |
| 4299819, | Jan 02 1979 | Sloan-Kettering Institute for Cancer Research | Process for treating burn victims |
| 4304866, | Nov 14 1979 | Massachusetts Institute of Technology | Transplantable sheets of living keratinous tissue |
| 4314380, | Sep 26 1980 | KOKEN CO , LTD | Artificial bone |
| 4342828, | Jul 20 1979 | Morinaga Milk Industry Co., Ltd.; The Green Cross Corp. | Method for producing substance capable of stimulating differentiation and proliferation of human granulopoietic stem cells |
| 4350629, | Jul 29 1981 | Massachusetts Institute of Technology | Procedures for preparing composite materials from collagen and glycosaminoglycan |
| 4352887, | Oct 29 1979 | Albert Einstein College of Medicine of Yeshiva University | Method and article for culturing differentiated cells |
| 4412947, | Sep 12 1979 | Seton Company | Collagen sponge |
| 4418691, | Oct 26 1981 | Massachusetts Institute of Technology | Method of promoting the regeneration of tissue at a wound |
| 4448718, | Sep 13 1983 | Massachusetts Institute of Technology; MASSACHUSETTS INSTITUTE OF TECHNOLOGY, 77 MASSACHUSETTS AVE , CAMBRIDGE, MA 02139 A MA CORP | Method for the preparation of collagen-glycosaminoglycan composite materials |
| 4451397, | Nov 30 1981 | CENTRE TECHNIQUE CUIR, CHAUSSURE, MAROQUINERIE | Method of preparing collagen products |
| 4458678, | Oct 26 1981 | Massachusetts Institute of Technology | Cell-seeding procedures involving fibrous lattices |
| 4481946, | Aug 14 1980 | APPLIED MEDICAL DEVICES, INC , A CORP OF CO | Bone marrow transplant method and apparatus |
| 4485096, | Dec 26 1978 | Massachusetts Institute of Technology | Tissue-equivalent and method for preparation thereof |
| 4485097, | Dec 26 1978 | Massachusetts Institute of Technology | Bone-equivalent and method for preparation thereof |
| 4486188, | Aug 14 1980 | Applied Medical Devices, Inc. | Bone marrow transplant method and apparatus |
| 4489710, | Jun 23 1981 | XOMA Corporation | Composition and method for transplantation therapy |
| 4505266, | Oct 26 1981 | Massachusetts Institute of Technology | Method of using a fibrous lattice |
| 4520821, | Apr 30 1982 | The Regents of the University of California | Growing of long-term biological tissue correction structures in vivo |
| 4522753, | Jul 17 1980 | Massachusetts Institute of Technology | Method for preserving porosity in porous materials |
| 4533635, | Jul 13 1979 | INSTITUT NATIONAL DE LA SANTE ET DE LA RECHERCHE MEDICALE | Process for stimulating the growth of epidermal cells |
| 4546500, | May 08 1981 | Massachusetts Institute of Technology | Fabrication of living blood vessels and glandular tissues |
| 4553272, | Feb 26 1981 | UNIVERSITY OF PITTSBURGH, THE, A NON-PROFIT CORP OF PA | Regeneration of living tissues by growth of isolated cells in porous implant and product thereof |
| 4559304, | Aug 09 1982 | Koken Co., Ltd. | Substratum for cell culture and a method for culturing and isolating cells using same |
| 4565784, | Jan 26 1981 | Trustees of Boston University | Hydrogels capable of supporting cell growth |
| 4604346, | Oct 09 1984 | MASSACHUSETTS INSTITUTE OF TECHNOLOGY, CAMBRIDGE, MA , A CORP OF | Skin-equivalent prepared by the use of punch biopsy |
| 4609551, | Mar 20 1984 | Process of and material for stimulating growth of cartilage and bony tissue at anatomical sites | |
| 4621100, | Mar 25 1981 | The Upjohn Company | Treatment of osteoporosis with prostaglandins |
| 4642118, | Nov 06 1984 | Koken Co., Ltd. | Man-made skin composed of two layers: collagen and a poly-alpha-amino acid |
| 4642292, | Oct 29 1979 | Albert Einstein College of Medicine of Yeshiva University, a Division of | Method for isolation of connective tissue biomatrix |
| 4645669, | Oct 04 1982 | Albert Einstein College of Medicine of Yeshiva University | Culturing and emplacement of differentiated cells in vivo |
| 4673649, | Jul 15 1983 | UNIVERSITY PATENTS, INC | Process and defined medium for growth of human epidermal keratinocyte cells |
| 4703108, | Mar 27 1984 | University of Medicine & Dentistry of New Jersey | Biodegradable matrix and methods for producing same |
| 4769317, | Jun 14 1983 | Process for growing human epidermis, product thereof | |
| 4835102, | Mar 31 1987 | ORGANOGENESIS, INC , 83 ROGERS STREET, CAMBRIDGE, AM 02142 A CORP OF DE | Tissue equivalent test systems |
| 4837379, | Jun 02 1988 | Organogenesis Inc. | Fibrin-collagen tissue equivalents and methods for preparation thereof |
| 4883487, | Apr 19 1986 | Koken Co., Ltd. | Method of producing an artifical skin |
| 4888291, | Jun 19 1987 | President and Fellows of Harvard College | Human epithelium originating from cell cultures |
| 4925924, | Mar 27 1984 | UNIVERSITY OF MEDICINE AND DENTISTRY OF NEW JERSEY, A NJ CORP | Biocompatible synthetic and collagen compositions having a dual-type porosity for treatment of wounds and pressure ulcers and therapeutic methods thereof |
| 4940666, | Jul 15 1983 | University Patents, Inc. | Process and defined medium for growth of human epidermal keratinocyte cells |
| 4950483, | Jun 30 1988 | ANGIOTECH PHARMACEUTICALS US , INC | Collagen wound healing matrices and process for their production |
| 4960423, | Nov 17 1982 | Method of enhancing the attachment of endothelial cells on a matrix and vascular prosthesis with enhanced anti-thrombogenic characteristics | |
| 4963489, | Apr 18 1986 | ADVANCED BIOHEALING, INC | Three-dimensional cell and tissue culture system |
| 4963490, | Sep 07 1987 | Alcan International Limited | Porous inorganic membrane support and method |
| 4970298, | Mar 26 1984 | UNIVERSITY OF MEDICINE AND DENTISTRY OF NEW JERSEY, A CORP OF NJ | Biodegradable matrix and methods for producing same |
| 4975377, | May 14 1987 | Cell growth chambers and method of use thereof | |
| 4996154, | May 04 1989 | Millipore Corporation | Method for growing cellular tissue |
| 5000963, | Jun 14 1983 | Method of treating the skin using human epidermal sheets | |
| 5015584, | Oct 14 1987 | Board of Regents, The University of Texas System | Epidermal graft system |
| 5147401, | Sep 06 1989 | ISOTIS N V | Artificial skin |
| 5273900, | Apr 28 1987 | The Regents of the University of California | Method and apparatus for preparing composite skin replacement |
| AU1374288, | |||
| AU1374388, | |||
| EP200574, | |||
| EP243132, | |||
| EP285474, | |||
| EP314109, | |||
| JP271749, | |||
| WO8301384, | |||
| WO8602273, | |||
| WO8808305, |
| Executed on | Assignor | Assignee | Conveyance | Frame | Reel | Doc |
| Aug 29 2001 | ORTEC INTERNATIONAL, INC | ORCEL LLC | ASSIGNMENT OF ASSIGNORS INTEREST SEE DOCUMENT FOR DETAILS | 012188 | /0948 | |
| Aug 29 2001 | ORCEL LLC | ORTEC INTERNATIONAL INC | SECURITY INTEREST SEE DOCUMENT FOR DETAILS | 012188 | /0957 | |
| Oct 27 2004 | ORCEL LLC | PAUL ROYALTY FUND, L P F K A PAUL CAPITAL ROYALTY ACQUISITION FUND, L P | SECURITY AGREEMENT | 015612 | /0414 |
| Date | Maintenance Fee Events |
| Jul 17 1997 | M283: Payment of Maintenance Fee, 4th Yr, Small Entity. |
| Jul 24 2001 | M284: Payment of Maintenance Fee, 8th Yr, Small Entity. |
| Jun 27 2005 | M2553: Payment of Maintenance Fee, 12th Yr, Small Entity. |
| Date | Maintenance Schedule |
| Dec 10 1999 | 4 years fee payment window open |
| Jun 10 2000 | 6 months grace period start (w surcharge) |
| Dec 10 2000 | patent expiry (for year 4) |
| Dec 10 2002 | 2 years to revive unintentionally abandoned end. (for year 4) |
| Dec 10 2003 | 8 years fee payment window open |
| Jun 10 2004 | 6 months grace period start (w surcharge) |
| Dec 10 2004 | patent expiry (for year 8) |
| Dec 10 2006 | 2 years to revive unintentionally abandoned end. (for year 8) |
| Dec 10 2007 | 12 years fee payment window open |
| Jun 10 2008 | 6 months grace period start (w surcharge) |
| Dec 10 2008 | patent expiry (for year 12) |
| Dec 10 2010 | 2 years to revive unintentionally abandoned end. (for year 12) |