• Journal of Periodontal and Implant Science
• /
• 제35권3호
• /
• pp.747-760
• /
• 2005

Periodontal therapy has dealt primarily with attempts at arresting progression of disease. however, more recent techniques have focused on regenerating the periodontal ligament having the capacity to regenerate the periodontium. Recombinant human bone morphogenetic protein-7(rhBMP-7) can differentiate the osteoprogenitor cells and induce bone formation. The purpose of this study was to evaluate the effect of BMP-7 on rat periodontal ligament cells differentiation, in vitro. In the control group, cells was cultured with DMEM media. In the experimental groups, cells were cultured with rhBMP-7 in concentration of 10, 25, 50 and 100 ng/ml. Each group was characterized by examining alkaline phosphatase activity at 3 and 5 days of culture and the ability to produce mineralized nodules of rat calvarial cells at 14 days of culture. Synthesis of type I collagen(COL-I), osteocalcin(OCN), and bone sialoprotein(BSP) was evaluated by RT-PCR at 7 days of culture. Activation of Smad proteins and p38 MAP kinase was determined by western blot analysis of the cell lysates. Alkaline phosphatase activity was significantly increased in the concentration of BMP-7 50 ng/ml and 100 ng/ml compared to the control(p<0.05). The mineralized bone nodule formation was greater with addition of 50 ng/ml and 100 ng/ml BMP-7 than the control(p<0.01). In 7 days' culture, the expressions of COL-I, BSP, and OCN was increased by BMP-7 in concentration of 10 $ng/ml{\sim}100$ ng/ml. In western blot analysis, BMP-7 treated culture cells expressed Smad 1,5,8 in dose-dependent manner, whereas BMP-7 did not activate phosphorylated form of p38 MAP kinase. These result suggested that BMP-7 stimulate rat periodontal ligament cells to differentiate toward osteoblast phenotype and increase bone matrix production by activation of BMP-Smad pathway.

• Journal of Periodontal and Implant Science
• /
• 제34권2호
• /
• pp.333-344
• /
• 2004

The enamel matrix derivative (EMD) has been recently used in the periodontal regenerative techniques. The present study was established to investigate the influence of EMD on human periodontal ligament cells using expression of mRNA of periodontal ligament specific gene (PDLs)17, PDLs22, type I collagen when EMD applied to periodontal ligament cells. Periodontal ligament cells were obtained from a healthy periodontium and cultured in Dulbecco's modified Eagle's medium (DMEM) plus 10% fetal bovine serum and ${\beta}-glycerophosphate$ with ascorbic acid. Test groups were two; One adds EMD in culture media and another added EMD and Dexamethasone (DEX) in culture media. Positive control group added DEX in culture media, and negative control group adds niether of EMD nor DEX. $Emdogain^{(R)}$ (Biora, Sweden, 30 mg/ml) was diluted by 75 ${\mu}g/ml$ concentration to culture media. For reverse transcription-polymerase chain reaction (RT-PCR), total RNA isolated on days 0, 7, 14 and 21. mRNA of PDLs17 was expressed on days 14 and 21 in EMD or DEX group, and expressed on days 7, 14 and 21 in EMD plus DEX group, the other side, expressed on days 21 in negative control group. mRNA of PDLs22 expressed on days 7, 14 and 21 in EMD group, and expressed on days 14 and 21 in DEX group, and expressed on days 7, 14 and 21 in EMD plus DEX group. Negative control group expressed on days 14 and 21. Type I collagen was expressed on all days and all groups. These results indicate that EMD promotes differentiation of periodontal ligament cells, and this is considered to offer basis that can apply EMD to periodontal tissue regeneration technique.

• Journal of Periodontal and Implant Science
• /
• 제25권3호
• /
• pp.720-732
• /
• 1995

미분화중배엽세포의 분화에 관여한다고 알려진 변형성장인자-${\beta}1$이 초기배양한 치주인대세포와 치은섬유아세포에 각기 다른 농도와 시간에 따라 변형성장인자-${\beta}1$을 주입했을때 두 세포의 세포증식능에 미치는 영향을 알아보고 각 조건에 따른 두 세포간의 증식능을 상호 비교해 보고자 본 실험을 실시하였다. 교정치료를 목적으로 내원한 환자의 제 1 소구치 부위의 정상치은을 절제하고, 건강한 제 1 소구치를 발거하여 치은섬유아세포와 치주인대세포를 분리, 배양하여 변형성장인자-${\beta}1$을 주입시키지 않은 군을 대조군으로 하고, 변형성장인자-${\beta}1$을 각각 0.25, 0.5, 1, 2.5, 5ng/ml로 주입시킨 군을 실험군으로하여 24시간, 48시간, 72시간 동안 배양하였으며, 각 시간별 배양 24시간 전에 $1{\mu}Ci/ml$ $[^3H]-thymidine$을 첨가하여 $[^3H]-thymidine$이 DNA내로 편재되는 속도로써 두세포군의 증식능을 측정하여 다음과 같은 결과를 얻었다. DNA합성능에 미치는 변형성장인자-${\beta}1$의 효과는 치주인대세포와 치은섬유아세포 모두에서 투여한 변형성장인자-${\beta}1$의 효과는 치주인대세포와 치은섬유아세포 모두에서 투여한 변형성장인자에 대하여 농도의존적으로 세포가 증식 하는 것으로 나타났다. 치은섬유아세포에 변형성장인자-${\beta}1$을 투여한 군에서는 24, 48, 72시간 모두에서 각 대조군에 비하여 농도의존적으로 증가하는 경향을 보였다. 24시간 적용시 대조군에 비해 1,2.5, 5 ng/ml투여군에서 통계적으로 유의한 차이(P<0.05)를 나타내었고, 48시간 적용시에는 대조군에 비해 1, 2.5, 5 ng/ml 투여군에서 통계적으로 유의한 차이(P<0.05)를 나타내었다. 48시간 적용시에 가장 높은 증식능을 보였으며 72시간 적용시에는 48시간 적용에 비해 전반적으로 증식능이 감소하는 경향을 보였다. 치주인대세포의 DNA 합성능에 미치는 변형성장인자-${\beta}$의 효과는, 변형성장인자-${\beta}$를 각각 24시간, 48시간 적용하였을�� 각 대조군에 비하여 농도의존적으로 증가하는 경향을 보였으며, 24시간 적용시에 대조군에 비해 1, 2.5, 5ng/ml 투여군에서 통계적으로 유의한 차이(P<0.05)를 나타내었고, 48시간 적용시에 대조군에 비해 2.5, 5ng/ml 투여군에서 통계적으로 유의한 차이(P<0.05)를 나타애었다. 72시간 적용시에는 5ng/ml의 농도에서 증식능이 감소하는 경향을 보였다. 48시간 적용시에 역시 가장 높은 증식능을 보였으며 72시간 적용에서는 48시간 적용에 비해 전반적으로 증식능이 감소되는 경향을 나타내었다. 변형성장인자-${\beta}1$의 적용에 따른 치주인대세포와 농도별 비교에서 치은섬유아세포군이 치주인대세포군보다 더 높은것으로 나타났다.

• 한국응용약물학회:학술대회논문집
• /
• 한국응용약물학회 2003년도 Annual Meeting of KSAP : International Symposium on Pharmaceutical and Biomedical Sciences on Obesity
• /
• pp.80-80
• /
• 2003

Insulin-dependent or Type 1 diabetes mellitus (IDDM) has been associated with an increased severity of periodontal disease. Since periodontal ligament (PDL) cells play a significant role in maintenance and regeneration of mineralized tissue, the success of procedures, such as guided tissue regeneration, is directly related to the ability of these cells to augment mineralized tissue. In this study, we investigated the time- and dose-dependent effect of high glucose on the proliferation and collagen synthesis of human periodontal ligament (PDL) cells. PDL cells were treated with high glucose (22mM, 33mM, 44mM) for 1 or 2 days. High glucose significantly inhibited proliferation of PDL cells as a time- and dose-dependent manner as evidenced by MTT assay. PDL cells were cultured in high glucose media (22mM, 33mM, 44mM) for 24 h. The ratio of collagen content to total protein was evaluated, and the gene expression of type I collagen was assessed by RT - PCR. The high concentration of glucose inhibited collagen synthesis, a marker of bone formation activity. This study indicated high glucose concentration could alter the metabolism of periodontal ligament cell, leading to alveolar bone destruction.

• Journal of the Korean Association of Oral and Maxillofacial Surgeons
• /
• 제36권1호
• /
• pp.7-15
• /
• 2010

Complex human tissues harbor stem cells and precursor cells, which are responsible for tissue development or repair. Recently, dental tissues such as dental pulp, periodontal ligament (PDL), dental follicle have been identified as easily accessible sources of undifferentiated cells. These tissues contain mesenchymal stem cells that can be differentiate into bone, cartilage, fat or muscle by exposing them to specific growth conditions. In this study, the authors procured the stem cell from pulp, PDL, and dental follicle and differentiate them into osteoblast and examine the bone induction capacity. Dental pulp stem cell (DPSC), periodontal ligament stem cell (PDLSC), and dental follicle precursor cell (DFPC) were obtained from human 3rd molar and cultured. Each cell was analyzed for presence of stem cell by fluorescence activated cell sorter (FACs) against CD44, CD105 and CD34, CD45. Each stem cell was cultured, expanded and grown in an osteogenic culture medium to allow formation of a layer of extracellular bone matrix. Osteogenic pathway was checked by alizarin red staining, alkaline phosphatase (ALP) activity test and RT-PCR for ALP and osteocalcin (OCN) gene expression. According to results from FACs, mesenchymal stem cell existed in pulp, PDL, and dental follicle. As culturing with bone differentiation medium, stem cells were differentiated to osteoblast like cell. Compare with stem cell from pulp, PDL and dental follicle-originated stem cell has more osteogenic effect and it was assumed that the character of donor cell was able to affect on differential potency of stem cell. From this article, we are able to verify the pulp, PDL, and dental follicle from extracted tooth, and these can be a source of osteoblast and stem cell for tissue engineering.

• Journal of Periodontal and Implant Science
• /
• 제31권4호
• /
• pp.823-832
• /
• 2001

Periodontal therapy has dealt primarily with attempts at arresting progression of disease, however, more recent techniques have focused on regenerating the periodontal ligament having the capacity to regenerate the periodontium. The effect of chitosan(poly-N-acetyl glucosaminoglycan), a carbohydrate biopolymer extracted from chitin, on periodontal ligament regeneration is of particular interest. The purpose of this study was to evaluate the effect of chitosan on the human periodontal ligament fibroblasts(hPDLFs) in vitro, with special focus on their proliferative properties by M'IT assay, the synthesis of type I collagen by reverse transcription-polymerase chain reaction(RT-PCR) and the activity of alkaline phosphatase(ALP). Fibroblast populations were obtained from individuals with a healthy periodontium and cultured with ${\alpha}MEM$ as the control group. The experimental groups were cultured with chitosan in concentration of 0.01,0.1, 1,2mg/ml. The results are as follows; 1. Chitosan-induced proliferative responses of hPDLFs reached a plateau at the concentration of O.lmg/ml(p<0.05). 2. When hPDLFs were stimulated with 0.lmg/ml chitosan, mRNA expression of type I collagen was up-regulated. 3. When hPDLFs were stimulated with 0.lmg/ml chitosan, ALP activity was significantly up-regulated(p<0.05). In summary, chitosan(0.lmg/ml) enhanced the type I collagen synthesis in the early stage, and afterwards, facilitated differentiation into osteogenic cells. The results of this in vitro experiment suggest that chitosan potentiates the differentiation of osteoprogenitor cells and may facilitate the formation of bone.

• Journal of Periodontal and Implant Science
• /
• 제23권1호
• /
• pp.97-108
• /
• 1993

치주조직의 초기치유과정에서 가장 중요한 역할을 하는 치주인대세포의 부착과 전개에 대한 형태학적 관찰을 위하여 교정치료 목적으로 발거된 치아로부터 치주인대조직을 채취하여 초기배양하고 동일한 양($5{\times}10^3ml$)의 치주인대 세포를, 2장의 유리가 포함된 35mm 배양접시에 접종한 후, $CO_2$ 배양기에서 배양하여 세포배양개시후 10분, 30분, 90분, 6시간, 12시간, 24시간의 시간간격에 따라서 광학위상차현미경과 주사전자현미경을 이용하여 세포부착과 전개양상을 관찰한 결과 다음과 같은 결과률 얻었다. 10분간 배양한 세포는 구형을 나타내었으며, 기질측의 세포질이 박판엽상으로 확장되어 기질에 부착개시한 양상이 보였다. 배양 30분 후 판모양의 세포돌기인 박판상돌기에서 세사상돌기롤 내어 부착하는 양상이 관찰되었고, 세포표면은 소기포와 미세융모로 덮여 있었다. 90분간 배양한 세포에서 핵은 세포의 중심부에 위치하였고 세포질이 방사선상으로 확장되어 부착된 양상을 보였으며, 미전개된 세포중심부에는 미세융모와 소기포로 덮여져 있었다. 배양 6시간 후 세포는 신장된 양상을 보였고 타원형의 핵이 관찰되었다. 세포의 양극에서 박판상돌기가 관찰되었고 다시 세사상돌기가 분지되는 양상을 보였는데 이 돌기의 말단부는 팽대되어 기질에 부착하였다. 12시간 배양한 후의 치주인대 세포는 뚜렷한극성화를 보이면서 길게 신장된 양상을 나타내었다. 배양 24시간 경과후 신장된 양상의 핵이 세포의 한쪽극에 치우쳐 있었으며, 세포외형은 길게 신장된 방추상의 형태가 관찰되었다.

• Journal of Periodontal and Implant Science
• /
• 제41권1호
• /
• pp.30-43
• /
• 2011

Purpose: Under different culture conditions, periodontal ligament (PDL) stem cells are capable of differentiating into cementoblast-like cells, adipocytes, and collagen-forming cells. Several previous studies reported that because of the stem cells in the PDL, the PDL have a regenerative capacity which, when appropriately triggered, participates in restoring connective tissues and mineralized tissues. Therefore, this study analyzed the genes involved in mineralization during differentiation of human PDL (hPDL) cells, and searched for candidate genes possibly associated with the mineralization of hPDL cells. Methods: To analyze the gene expression pattern of hPDL cells during differentiation, the hPDL cells were cultured in two conditions, with or without osteogenic cocktails (${\beta}$-glycerophosphate, ascorbic acid and dexamethasone), and a DNA microarray analysis of the cells cultured on days 7 and 14 was performed. Reverse transcription-polymerase chain reaction was performed to validate the DNA microarray data. Results: The up-regulated genes on day 7 by hPDL cells cultured in osteogenic medium were thought to be associated with calcium/iron/metal ion binding or homeostasis (PDE1A, HFE and PCDH9) and cell viability (PCDH9), and the down-regulated genes were thought to be associated with proliferation (PHGDH and PSAT1). Also, the up-regulated genes on day 14 by hPDL cells cultured in osteogenic medium were thought to be associated with apoptosis, angiogenesis (ANGPTL4 and FOXO1A), and adipogenesis (ANGPTL4 and SEC14L2), and the down-regulated genes were thought to be associated with cell migration (SLC16A4). Conclusions: This study suggests that when appropriately triggered, the stem cells in the hPDL differentiate into osteoblasts/cementoblasts, and the genes related to calcium binding (PDE1A and PCDH9), which were strongly expressed at the stage of matrix maturation, may be associated with differentiation of the hPDL cells into osteoblasts/cementoblasts.

• Journal of Periodontal and Implant Science
• /
• 제34권3호
• /
• pp.489-498
• /
• 2004

Recent studies have demonstrated that human periodontal ligament cells express receptor activation of nuclear factor ${\kappa}B$ ligand (RANKL) which enhances the bone resorbing activity of osteoclasts differentiated from hematopoietic preosteoclasts. The purpose of this study is to determine the effects of p38 MAPK and JNK kinase upon regulating RANKL and OPG in response to $IL-1{\beta}$(l ng/ml) in rat periodontal ligament cells. Soluble RANKL was measured by immunoassay. The effects of p38 MAPK on RANKL and OPG expression was determined by RT-PCR. The results were as follows: 1. Periodontal ligament cells which stimulated by $IL-1{\beta}$ increased soluble RANKL synthesis by dose-dependent pattern. 2. p38 MAP kinase inhibitor (SB203580) showed regulation of soluble RANKL expression by dose-dependent manners. 3. p38 MAP kinase inhibitor (SB203580) regulated the expression of RANKL, but it dose regulate the expresseion of OPG. 4. JNK (c-jun $NH_2-terminal$ kinase) inhibitor (PD98059) did not regulate mRANKL and mOPG. These results suggested that p38 MAPK play a significant role in RANKL gene expression.

• Journal of Periodontal and Implant Science
• /
• 제41권2호
• /
• pp.73-78
• /
• 2011

Purpose: For periodontal tissue engineering, it is a primary requisite and a challenge to select the optimum types of cells, properties of scaffold, and growth factor combination to reconstruct a specific tissue in its natural form and with the appropriate function. Owing to fundamental disadvantages associated with using a two-dimensional substrate, several methods of seeding cells into three-dimensional scaffolds have been reported and the authors have asserted its usefulness and effectiveness. In this study, we explore the cell attachment of periodontal ligament fibroblasts on nanohydroxyapatite (n-HA) scaffold using avidin biotin binding system (ABBS). Methods: Human periodontal ligament fibroblasts were isolated from the health tooth extracted for the purpose of orthodontic procedure. HA nanoparticles were prepared and $Ca(NO_3)_2-_4H_2O$ and $(OC_2H_5)_3P$ were selected as precursors of HA sol. The final scaffold was 8 mm in diameter and 3 mm in height disk with porosity value of 81.55%. $1{\times}10^5$ periodontal ligament fibroblasts were applied to each scaffold. The cells were seeded into scaffolds by static, agitating and ABBS seeding method. Results: The number of periodontal ligament fibroblasts attached was greater for ABBS seeding method than for static or agitating method (P<0.05). No meaningful difference has been observed among seeding methods with scanning electron microscopy images. However, increased strength of cell attachment of ABBS could be deduced from the high affinity between avidin and biotin ($Kd=10^{-15}\;M$). Conclusions: The high-affinity ABBS enhances the ability of periodontal ligament fibroblasts to attach to three-dimensionally constructed n-HA scaffold.