RU2265445C1 - Biotransplant, method for its obtaining (variants) and method for treating parodontium diseases - Google Patents

Abstract

FIELD: biopharmacology, medicine.

SUBSTANCE: the present innovation deals with preparing the culture of genetically unmodified chondroprogenitor cells and method for treating parodontium diseases. Biotransplants, methods for their obtaining and method for treating parodontium diseases deal with introducing the suspension of mesenchymal stem and chondroprogenitor cells or their combination that contains 1-50 mln. cells/ml, intraligamentally from lateral and medial sides of every tooth and subperiosteally, into mandibular and maxillary parodontal parts.

EFFECT: higher efficiency of therapy.

13 cl, 1 ex

Description

The invention relates to the preparation of a culture of genetically unmodified chondroprogenic cells and a method for the treatment of periodontal diseases.

Periodontal disease continues to be one of the most pressing problems of dentistry. According to various authors, by 25-30 years, up to 50% of the population have some form of periodontal tissue damage. One of the most common forms is periodontitis, which begins with an initial lesion of the marginal part of the gums, followed by the involvement of all periodontal structures in the pathological process. Chronic periodontitis is characterized by a progressive course with resorption of the bone tissue of the alveolar process, death of the retaining apparatus of the tooth and loss (removal) of the latter. Existing methods of local anti-inflammatory therapy are not always effective and do not contribute to the restoration of bone tissue of the alveolar processes. Therefore, it is necessary to search for new drugs for the treatment of chronic periodontitis, aimed at the active repair of inflammatory and destructive injuries.

Modern methods of treatment of periodontitis are not only to eliminate periodontal infection, but also to conduct reparative osteosynthesis using a variety of osteoplastic materials. These methods are quite widely used in modern periodontics, in order to achieve effective regeneration of periodontal tissues, since there is the possibility of restoration of cement of the root of the tooth, periodontal ligament and alveolar bone. Unfortunately, to date, complete regeneration of periodontal tissues has not yet been possible.

Recently, in dental practice, along with osteoplastic drugs such as hydroxyapatite and collagen, the use of osteocyte precursor cells - mesenchymal stem and chondro-progenitor cells as cell replacement therapy, to stimulate directed regeneration of periodontal tissues is widespread.

Treatment of various forms of periodontal disease includes conservative and surgical methods of therapy. Conservative treatment of periodontal disease involves the elimination of local pathogenic factors, the removal of tartar, teeth with mobility of the III-IV degree, the replacement of poor-quality fillings, crowns, bridges. For the treatment of inflamed gum tissue, agents are used to suppress the mixed pathogenic microflora of the gingival pockets. A significant place in the complex therapy of periodontal disease is given to surgical treatment: curettage, gingivotymnia, gingiveectomy, etc. Of the currently existing methods of treatment of periodontitis, surgical tactics are considered the most effective, since they radically solve the problem associated with destructive changes in bone tissue. Such changes are the result of resorption of calcium salts from the bone and a consequence of the inflammatory process in periodontal pockets. As a result, defects in bone tissue are filled with pathological tissues - granulations, the presence of which, in turn, leads to even faster bone resorption. The situation is aggravated by the fact that under adverse conditions, granulation can degenerate into periodontal cysts. During surgery, unhealthy tissue is removed, and bone defects are filled with various osteoplastic materials. These substances stimulate bone formation, significantly improve the recovery processes in damaged tissues, contribute to the rapid healing and restoration of bone structure, and also have anti-inflammatory effects.

Currently, various biological and synthetic materials are widely used for bone tissue regeneration, including the use of auto- and allogeneic fibroblasts, bone marrow cell elements, etc., for the purpose of directed osteoregeneration (Ashton et al., 1980. Aston et al. , 1986. Brittberg et al., 1994). As shown by several authors, the used biological and synthetic materials do not cause sufficient stimulation of reparative processes to restore the structure and function of periodontal bone tissue (Coletty et al., 1972. Furukawa et al., 1980).

Known methods for producing human chondroprogenitor cells from fetal cartilage tissue obtained at different gestation periods include sequential mechanical and enzymatic disaggregation of the original cartilage tissue using various enzyme solutions and their combination (collagenase, pronase, hyaluronidase, deoxyribonuclease, etc.) in various concentrations. Depending on the methods of disaggregation, you can get a different number of cells with the necessary phenotype and a different number of viable cells from 50 to 80%. For the cultivation of chondroprogenitor cells, non-coated Petri dishes, culture bottles, and various non-selective substrates from collagen, agarose, etc. are used (Brittberg et al., 1994. Fuchs et al., 2002). The listed methods of culturing cells in a monolayer do not allow for more than 2-3 passages without loss of the phenotype of chondroprogenitor cells, which are dedifferentiated into fibroblast-like cells. Known methods for the cultivation of chondroprogenitor cells in suspension using various three-dimensional carriers (alginate, polyglycolide, polylactate, atelocollagen), which allows you to conduct culture for a longer time without losing the phenotype of the cells (Kimura et al., 1984. Matsusaki et al., 1998).

Chondroprogenitor cells obtained from fetal cartilage by sequential disaggregation and cultivation in selective media during transplantation with high efficiency proliferate, migrate, integrate into the lesion, differentiate into osteocytes, depending on the microenvironment, synthesize extracellular matrix, stimulate angiogenesis (Patent RU 21 , 10/12/2000).

Bone tissue regeneration during damage and systemic resorption occurs due to mesenchymal stem cells (MSCs), which are the precursors of osteoblasts and contribute to the formation of remodeling units. Currently, the use of MSCs for systemic and local regeneration of bone tissue is increasingly used. Mesenchymal stem cells are mainly derived from donor bone marrow, but there are other sources - skeletal muscle, subcutaneous adipose tissue, fetal organs of hematopoiesis (liver, thymus, spleen). MSCs from fetal organs of hematopoiesis and methods for their preparation are practically not studied. The described methods for growing MSCs from bone marrow and lipoaspirates make it possible to obtain heterogeneous populations of stromal cells, only a small percentage of which are stem cells (S. J. Forbes et al., 2002). The cells of the mature stroma do not possess the property of differentiating into different cell lines and, thus, are therapeutically ineffective. After transplantation, stromal cells migrate mainly to the connective tissue and accumulate there. With standard passage at high inoculum doses, the proportion of mature stromal cells increases rapidly.

The use of a homogeneous (at least 80%) population of pluripotent MSCs as a transplant allows to increase the effectiveness of treatment, increase the reproducibility of the results and avoid undesirable effects.

The objective of the present invention is to obtain a homogeneous culture of mesenchymal stem and chondrogenetic cells for implantation with the aim of directed osteoregeneration in periodontal diseases in order to increase the effectiveness of treatment.

To solve this problem, a group of inventions is proposed, united by a common inventive concept.

A biotransplant is proposed for the treatment of periodontal diseases, which is a suspension of human chondroprogenitor cells, including a culture of genetically unmodified human chondroprogenitor cells, containing at least 80% aggrecon and collagen II expressing cells, obtained from the hyaline cartilage tissue of human embryos of the 1-2 trimester of pregnancy and selectively propagated under cultivation conditions.

The biograft contains a freshly prepared culture.

A biograft can contain a cryopreserved cell culture using dimethyl sulfoxide as a cryoprotectant.

A method for producing a biograft for the treatment of periodontal diseases is proposed, consisting in the fact that the cartilage tissue of human embryos of 1-2 trimesters of pregnancy is washed, crushed and enzymatically disaggregated for 40-90 minutes, the resulting suspension of primary dissociated chondrogenic cells is seeded with a density of at least 1 × 10 ⁶ cells / ml and cultured on DMEM / F12 growth medium containing 10% fetal calf serum, 1% ITS (insulin, transferin, selenite), 50 μg / ml ascorbic acid, 10 μg / ml gentamicin, 5 μg / ml ampho tericin B and growth factors, when a cell culture of a confluent state is reached, they are passaged using a trypsin solution, with a seeding density of at least 10 × 10 ⁵ cells / ml, and cultivation is carried out for 18-25 days at 37 ° C in an atmosphere of 5% CO ₂ .

Tissue disaggregation is carried out by incubating it with an enzyme in a solution containing 0.01-0.15% collagenase solution and 0.05-0.1% pronase E solution in a ratio of 1: 1.

Passport culture no more than 2 times.

A suspension of primary dissociated cartilage cells is cultured on bare Petri dishes.

A biotransplant is also proposed for the treatment of periodontal diseases, containing mesenchymal stem cells (MSCs) obtained from fetal or donor material, or from the recipient's own tissues, while the tissue is disaggregated, the resulting cell suspension is resuspended and cultured on a growth medium containing transferrin, insulin, fibroblast growth factor and heparin before mature stroma cells accumulate in the culture.

The following tissues are used as fetal material: bone marrow, thymus, liver, adipose tissue of human embryos of the 1st trimester of pregnancy.

The following tissues are used as donor material: bone marrow, thymus, liver, adipose tissue.

To obtain autologous MSCs, tissues are used: bone marrow, adipose tissue.

A method for producing a biograft for the treatment of periodontal diseases is proposed, namely, mesenchymal stem cells (MSCs) obtained from fetal, donor or autologous material are enzymatically disaggregated, the resulting cell suspension is resuspended in DMEM / F12 growth medium containing 15% fetal calf serum and 2 mM glutamine, hereinafter seeded at seeding 1-20 million. mononuclear cells per 1 cm ² and incubated at 37 ° C under 5% CO _2, upon reaching 50% confluence culture monolayer trip iniziruyut and replated at a density of 10-30 cells per 1 cm ² in growth medium containing 10 ug / ml transferrin, 1 microgram / ml insulin, 10 ng / ml fibroblast growth factor - 2 and 8 units / mL heparin, and with increasing seed dose cultivation lead to the accumulation of mature stroma in the culture.

A method for the treatment of periodontal diseases is proposed, which consists in using a suspension of mesenchymal stem or chondroprogenitor cells or a combination of 1: 1, containing 1-50 million cells / ml, is administered itraligamentally from the lateral and medial sides of each tooth and subperiostally to the periodontal areas upper and lower jaws.

One of the objects is the culture of genetically unmodified human chondroprogenitor cells. The culture was obtained from the hyaline cartilage of human embryos of 1-2 trimesters of pregnancy and contains aggrecan and collagen II-expressing cells of at least 80% and not more than 20% of impurity cells. The second object is a method for producing chondroprogenitor cells. Cartilage tissue of human embryos of the 1-2 trimester of pregnancy is washed, mechanically crushed and subjected to enzymatic disaggregation for 40-90 minutes in a solution containing 0.01-0.1% type II collagenase solution, 0.05-0.1% pronase solution E. Suspension of primary dissociated chondroprogenitor cells is seeded with a density of at least 1 × 10 ⁶ cells / ml and cultured in a medium containing DMEM / F12 growth medium, 10% fetal calf serum supplemented with growth additives and growth factors.

The environment is repeatedly changed. Upon reaching the cell culture of the confluent state, passaging is carried out using a trypsin solution to disaggregate the monolayer. Sowing density - 1 × 10 ⁶ cells / ml.

Cells are cultured for 18-25 days at 37 ° C in an atmosphere of 5% CO ₂ . Passport culture no more than two times.

The method is as follows.

For the preparation of a biograft, fetal abortive material is used, obtained by artificially aborting pregnancy in healthy women previously examined for the presence of viral and bacterial infections. Fetal material is transferred into a sterile vessel with a solution of Hanks and gentamicin (80 mg / l). Further work is done under sterile conditions in a laminar box. The cartilaginous tissue extracted with the help of surgical instruments is thoroughly washed from blood clots, and all soft tissues (skin, fascia, muscles, tendons, ligaments) and bone tissue are maximally separated. The resulting cartilage is crushed to pieces of at least 1 mm ³ . Then subjected to enzymatic and mechanical disaggregation - the release of cellular elements from the tissue matrix.

The method of disaggregation consists in using a 0.1% type II collagenase solution (Sigma), a 0.05% pronase E solution (Sigma), in one-stage incubation of cartilage tissue pieces for 40-90 min in a two-component (1: 1) enzyme solution, subsequent grinding by repeated pipetting to obtain a unicellular suspension. The resulting suspension is washed three times by centrifugation at 700 rpm. A suspension of primary dissociated cartilage cells obtained from fetal cartilage tissue was cultured on uncovered Petri culture plates in medium containing DMEM + F12 growth medium (1: 1, Gibco BRL), 10% fetal calf serum (NPE PanEco), 1% ITS (insulin, transferrin, selenite. NPE PanEco), 50 μg / ml ascorbic acid (Sigma), 10 μg / ml gentamicin, 5 μg / ml amphotericin B with the addition of growth factors 5-20 ng / ml bFGF (Sigma) and / or 0.1-10 ng / ml TGFβ ₁ (Sigma). The environment is replaced every 3 days. When the cell culture reaches a confluent state, passaging should be performed using a 0.05% trypsin solution to disaggregate the monolayer of the same culture medium with a culture density of at least 10 × 10 ⁵ cells / ml. It is possible to carry out no more than two passages due to dedifferentiation and a change in the phenotype (reduction in the number of aggrecan and collagen II-expressing cells) of the resulting cells.

Mesenchymal stem cell cultures are used to prepare the biograft. MSCs with a primary ability for osteogenic differentiation are isolated from fetal (bone marrow, thymus, liver, adipose tissue), donor (bone marrow, adipose tissue, thymus) or autologous (oblique, adipose tissue) tissues. To isolate fetal cells using abortive material obtained by artificial termination of pregnancy in healthy women, previously examined for the presence of viral and bacterial infections.

The possibility of using biomaterial is achieved at the following gestational periods: liver - 5-8 weeks, thymus - 18-20 weeks, bone marrow - 17-20 weeks, subcutaneous adipose tissue - 17-19 weeks. If the cells are not extracted from aspirates (bone marrow, lipoaspirate), but from dense tissues such as the thymus, the organ is preliminarily crushed and enzymatically disaggregated. The suspension is filtered through a fine mesh stainless steel sieve. The cell suspension (aspirate) is diluted 1: 1 with Hanks saline, centrifuged in 1,500 × g mode, 10 minutes and resuspended in DMEM / F12 growth medium containing 15% fetal calf serum, selected for cell growth in low density, 2 mm glutamine. A cell suspension is plated on plastic Petri dishes with a diameter of 100 mm. The seeding density of the primary cell suspension is 1-20 million mononuclear cells per 1 cm ² depending on the source of excretion. After 1 day, non-adherent cells are removed, the growth medium is replaced. The cultures are incubated at 37 ° C in an atmosphere of 5% CO ₂ . After 6 days, growth of heterogeneous cell populations is observed. Once the culture reaches 50% confluency, the monolayer is trypsinized and replanted onto new plates with a density of 10-30 cells per 1 cm ² in a growth medium additionally containing 10 μg / ml transferrin, 1 μg / ml insulin, 10 ng / ml fibroblast growth factor - 2 and 8 U / ml heparin. After 7-10 days, dense colonies of small cells (7-10 microns in diameter) with a large number of mitoses are selected. The selected colonies are seeded in new plates with a density of 20 cells / cm ² and grown to a state of pre-confluency. The medium is replaced every 2 days. Subsequent passages are made in the same mode. An increase in the seeding dose or a change in the composition of the growth medium leads to the rapid accumulation of mature stroma cells in the culture.

Experimentally selected conditions, combining the criteria for selecting the initial biomaterial and the cultivation mode, are optimal for achieving the following results.

The system of sequential enzymatic disaggregation of the original tissue allows you to get the maximum number of viable cells of the same phenotype with a small admixture of heterotopic cells.

The cultivation mode and selective culture media allow the maximum increase in the number of aggrecan and collagen II-expressing cells.

The cultivation mode and selective culture media make it possible to obtain a homogeneous cell culture containing at least 80% aggrecan and collagen II-expressing cells.

The selection system for the sources of MSCs allows to obtain cell cultures with a primary ability for osteogenic differentiation.

The cultivation mode and selective culture media allow for repeated passage to maximize the homogeneous cell culture of undifferentiated cells.

The cultivation mode and selective culture media allow to preserve the pluripotency of cell cultures.

The cultivation mode and selective culture media allow to obtain a large number of cells for transplantation (series), which ensures reproducibility of treatment results.

As a biograft, a freshly obtained cell culture is used or after its cryopreservation. As cryoprotectant use 7% dimethyl sulfoxide.

The proposed method of treatment is transplantation. Various volumes of cell suspensions containing 1-50 million COD in 1 ml, 1-50 million MSC in 1 ml are used as a biograft, a combination of biografts containing COD and MSC in a ratio of 1: 1 can be used.

Immediately before the start of transplantation, a biological test is performed. A solution containing in 1 ml of 1-50 million chondroprogenitor or mesenchymal stem cells is injected in an amount of 0.1 ml into the soft tissues of the gums. The recipient finds out complaints about the condition, pain, measure blood pressure and count the pulse. Signs of biological incompatibility are: the appearance of pain in the lumbar, epigastric regions, headaches, chest pains, feelings of fear, the presence of sweat and swelling of the face, decreased blood pressure, increased heart rate. The sample is repeated three times. With a negative result, they begin transplantation.

Premedication with sedative drugs is carried out according to the standard scheme. Using an insulin syringe, a suspension of cells is administered intraligamentally from the lateral and medial sides of each tooth of the upper and lower jaw with several injections. Subperiosteally, several injections of a cell suspension containing 1-50 million COD, MSCs, or a combination thereof, are carried out in the periodontal areas of the upper and lower jaws.

Within 2-4 hours after transplantation, the patient must be monitored by a physician.

The effectiveness of the proposed method consists in increasing the density of bone tissue, directed osteoregeneration of the alveolar processes of the upper and lower jaws.

The observation group included 18 patients who came to the clinic complaining of tooth mobility, gum bleeding, halitosis, and the inability to fully chew food. In clinical and radiological studies, everyone was diagnosed with severe periodontitis, accompanied by atrophy of more than 1/2 of the alveolar bone and 2-3 degrees of tooth mobility. All patients were examined as follows: complete blood count, biochemical blood test, general urinalysis, immunological status, hormonal status (T3, T4, TSH, AT-TG, AT-TPO, FSH, LH, estrogen, progesterone, prolactin, testosterone, insulin, IGF-I, II), a virological study, PCR of blood and scrapings of the oral mucosa (CMV, Ch.spp, Myc.spp, HPV 16/18, Tox.spp, Herpes 1,2), a study for a number of common tumor markers (HGT, CA-125, CA-15.3, CA-19.9, PSA, AFP, CEA). Ultrasound of the abdominal cavity, small pelvis, thyroid gland, X-ray of the chest organs in order to exclude acute pathologies, oncological diseases that could complicate the upcoming intervention were performed for all patients. A correction of the treatment of a number of chronic diseases of the cardiovascular system, gastrointestinal tract, and urinary system has been made.

In most patients, Bacteriodes spp. Was detected using PCR in the oral mucosa, in many, CMV, Mic.spp., EBV, Chl.spp were determined. Appropriate treatment was carried out with drugs selected in accordance with the tropism for the pathogen typed by RT-PCR.

Thus, at the time of stem cell implantation, patients did not have oncological diseases, allergic diseases and reactions, other chronic diseases in the stage of decompensation / exacerbation, acute inflammatory processes, drug addiction, acute poisoning were excluded.

After local traditional treatment of periodontitis, patients were implanted with subperiostal chondroprogenitor cells in the periodontal areas of the alveolar processes of the upper and lower jaws.

Patient I., 52 years old, came to the clinic with complaints of tooth mobility (according to the examination - 2–3 degrees), bleeding gums, bad breath, inability to fully chew food.

On the basis of a clinical and radiological examination, the diagnosis was made: severe periodontitis with atrophy of more than 1 alveolar ridge, tooth mobility of 2-3 degrees. Concomitant somatic diseases: gastric and duodenal ulcer, condition after cholecystectomy, hypertension of the initial sclerotic stage.

Clinical and laboratory examination revealed: leukocytosis, hypercholesterolemia, elevated fractions of triglycerides, impaired lipid metabolism, impaired glucose tolerance, hyperglycemia. Immunological status - increased level of activated T-lymphocytes. Hormonal status within the age norm.

Patient conducted: professional oral hygiene; the teeth of the upper and lower jaw are splintered along the "Glaspen" blocks, a deep curettage of pathological pockets is selectively performed. An artistic restoration of the teeth of both jaws was made.

After the above treatment, based on the voluntary informed consent of the patient (legislative base - Article 43 of the Federal Law "Fundamentals of the Legislation on the Protection of Citizens of the Russian Federation"), cell replacement therapy was carried out - after premedication, a human chondrogenic cell culture was introduced subperiostally for use in cell replacement therapy (passport series ASN No. 15-2-150, the conclusion on the conformity of the manufacturing conditions of GMP: GiproNIIIMedProm, TsGSEN South Administrative District of Moscow 55 / 3.10 dated May 13, 2002).

The day after the implantation of the stem cell preparation, the patient noted the disappearance of pain and bleeding gums. On local examination, the oral mucosa is pale pink, moderately moisturized, and adheres closely to the teeth. General condition is satisfactory. On the fifth day there is no data indicating pathological changes.

The patient notes: increased performance, increased activity, decreased sleep time, increased potency and libido.

Control clinical and laboratory examination after 15 days: absence of leukocytosis, normalization of lipid metabolism, decrease in T-lymphocyte activity. The general condition of the patient is satisfactory, there are no complaints about the maxillofacial region. At a local examination - there is a positive dynamics, the mucous membrane is pale pink, tightly adjacent to the teeth, there is no bleeding of the gums when probing. After six months, the general condition of the patient is satisfactory. The clinical picture locally is unchanged. An orthopantomogram shows an increase in the optical density of the bone of the alveolar processes (compared with the images before implantation in all patients by an average of 49 ± 3%, p = 0.05), a significant increase in their height along the axes of the biomechanical load.

Thus, the study showed that the implantation of COD leads to the implementation of directed physiological regeneration of bone tissue of the alveolar processes in the adult body in the presence of destructive and inflammatory diseases of periodontal tissues and can be an effective method of treatment of periodontitis.

Claims (13)

1. A biograft for the treatment of periodontal disease, characterized in that it is a suspension of human chondroprogenitor cells, including a culture of genetically unmodified human chondroprogenitor cells containing at least 80% aggrecan and collagen II expressing cells obtained from the hyaline cartilage tissue of human embryos 1-2 -th trimester of pregnancy and selectively propagated under cultivation conditions. 2. The biograft according to claim 1, contains a freshly prepared culture. 3. The biograft according to claim 1, contains a cryopreserved cell culture, using dimethyl sulfoxide as a cryoprotectant. 4. A method of producing a biograft for the treatment of periodontal diseases, characterized in that the cartilage of human embryos of 1-2 trimesters of pregnancy is washed, crushed and enzymatically disaggregated for 40-90 minutes, the resulting suspension of primary dissociated chondrogenic cells is seeded with a density of at least 1 · 10 ⁶ cells / ml and cultured in growth medium DMEM / F12, containing 10% fetal calf serum, 1% ITS (insulin, transferrin, selenite), 50 ug / ml ascorbic acid, 10 ug / ml gentamicin, 5 .mu.g / ml amphotericin B B and growth factors, while achieving a confluent state of the cell culture passaging is carried out using a trypsin solution, the seeding density of at least 10 × 10 ⁵ cells / ml, and cultivation are 18-25 days at 37 ° C under 5% CO _2. 5. The method according to claim 4, where the disaggregation of the tissue is carried out by incubating it with an enzyme in a solution containing a 0.01-0.15% solution of collagenase and a 0.05-0.1% solution of pronase E in a ratio of 1: 1. 6. The method according to claim 4, where the culture is passaged no more than 2 times. 7. The method according to claim 4, a suspension of primary dissociated cartilage cells is cultured on bare Petri dishes. 8. A biograft for the treatment of periodontal diseases, characterized in that it contains mesenchymal stem cells (MSCs) obtained from fetal, donor or autologous material, the tissue is disaggregated, the resulting cell suspension is resuspended and cultured on a growth medium containing transferrin, insulin, fibroblast growth factor and heparin before mature stroma cells accumulate in the culture. 9. The biograft according to claim 8, the following tissues are used as fetal material: bone marrow, thymus, liver, adipose tissue of human embryos of the 1st trimester of pregnancy. 10. Biograft according to claim 8, the following tissues are used as donor material: bone marrow, thymus, liver, adipose tissue. 11. The biograft according to claim 9, the following tissues are used as autologous material: bone marrow, adipose tissue. 12. A method of producing a biograft for the treatment of periodontal diseases, characterized in that mesenchymal stem cells (MSCs) obtained from fetal, donor or autologous materials are enzymatically disaggregated, the resulting cell suspension is resuspended in DMEM / F12 growth medium containing 15% fetal calf serum and 2 mM glutamine, hereinafter seeded at a seeding density of 1-20 million. mononuclear cells per 1 cm and incubated at 37 ° C under 5% CO _2, upon reaching 50% confluence culture monolayer trypsin iruyut and replated at a density of 10-30 cells per 1 cm ² in growth medium containing 10 ug / ml transferrin, 1 g / ml insulin, 10 ng / ml fibroblast growth factor - 2 and 8 units / mL heparin, and with increasing seed dose cultivation lead to the accumulation of mature stroma in the culture. 18. A method of treating periodontal diseases, characterized in that the biograft according to claim 1 and / or claim 4 is used, where a suspension of mesenchymal stem or chondroprogenitor cells or a combination thereof in a ratio of 1: 1, containing 1-50 million cells / ml, injected intraligamentally from the lateral and medial sides of each tooth and subperiosteally into the periodontal areas of the upper and lower jaws.