• Radiation Oncology Journal
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• 제20권3호
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• pp.253-263
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• 2002

목적 : bFGF (basic fibroblast growth factor)는 섬유아세포(fibroblast)에서 분비하는 대표적인 성장인자로 섬유아세포뿐 아니라 간질조직과 골수 및 다른 상피 근원세포의 성장에도 관여하며 방사선보호제 역할에 관한 연구가 시도되고 있다. 이 연구는 방사선보호제로서의 bFGF의 기능을 알아보고자 하였다. 대상 및 방법 : 간엽조직 기원(mesenchymal origin)인 마우스육종 180 종양세포를 생쥐 대퇴부 피하에 이식하고 bFGF를 투여한 후 전신방사선조사(6, 8, 10 Gy)하여 생쥐의 생존률을 조사하고 bFGF (3, $6\;{\mu}g$/쥐)의 방사선보호효과를 관찰하였다. 동시에 이식한 마우스 180 고형종양을 국소방사선조사한 후 bFGF가 종양성장에 미치는 영향을 알아보았다. 또한 bFGF에 의한 방사선보호효과의 기전을 이해 하고자 소장점막, 골수, 폐조직 및 이식종양조직에 대한 병리 조직학적 검사와 DNA terminal transferase nick-end labeling assay 방법으로 아포프토시스(apoptosis) 빈도를 측정하였다. 결과 : 1) 방사선조사단독군에 비해 방사선조사와 $6\;{\mu}g$ bFGF 투여병행군에서 생쥐의 골수치사를 감소시켜 생존률이 증가되었다(p<0.05). 2) 방사선조사단독군에 비해 방사선조사와 $6\;{\mu}g$ bFGF 투여병행군에서 공장 소낭선 깊이 및 미세융모 길이가 의의 있게 증가되었다(p<0.05). 소낭선세포의 아포프토시스 빈도는 방사선조사단독군에 비해 방사선조사와 bFGF 투여병행군에서 방사선조사후 8시간, 24시간에 감소하였으며 bFGF를 고용량 투여한 군에서 뚜렷하였다. 3) 골수조직에서는 방사선조사 후 7일, 14일째 세포 밀도가 방사선조사단독군에 비해 방사선조사와 $6\;{\mu}g$ bFGF 투여병행군에서 증가하였으며 특히 거핵구(megakaryocyte) 계열의 증가가 뚜렷하였다. 4) 폐조직의 H-E 염색 조직소견에서 방사선단독군과 방사선조사와 bFGF 투여병행군 간의 차이는 없었다. 5) 골수 및 폐 조직에서 bFGF 투여에 따른 초기 아포프토시스 빈도의 차이는 려었다(p>0.05). 6) 양성대조군과 bFGF단독투여군 비교시 bFGF투여에 의한 종양성장은 관찰되지 않았으며(p>0.05) 방사선조사단독군과 방사선조사와 $6\;{\mu}g$ bFGF 투여병행군에서도 종양성장곡선의 차이는 없었다(p>0.05). 결론 : 이상의 결과로 bFGF는 소장점막 및 골수세포에 방사선보호효과가 있었으며 그 기전은 조혈모세포 및 소장낭선세포의 성장 및 재생을 촉진하고 조기에 방사선으로 유도된 아포프토시스를 감소시키기 때문인 것으로 생각된다.

• 대한소아치과학회지
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• 제24권1호
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• pp.1-17
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• 1997

백서 태자 두개관을 효소처리하여 얻은 조골세포 유사세포군의 증식능 및 골결절의 형성에 미치는 dexamethasone의 영향과 형성된 골결절의 조직학적 형태 관찰을 위하여, 12 well 배양접시의 각 well 당 $4{\times}10^4cell$ 을 접종하였으며, 30일간 표준배양액으로만 배양한 군, 표준배양액에 ascorbic acid와 Na-${\beta}$-glycerophosphate를 첨가한 군, 그리고 각각에 dexa methasone을 첨가한 군등 4군으로 분리 배양하여 다음과 같은 결과를 얻었다. 1. 골세포의 증식율은 표준용액으로 배양한 군에 비해 dexamethasone 을 단독으로 투여한 군에서 약간 증가하는 경향을 보였으나 통계적인 유의성은 없었다 (p<0.05). 2. 골세포의 증식율은 ascorbic acid 에 의해 영향을 많이 받았으며, 특히 ascorbic acid와 dexamethasone을 동시에 투여했을때 더욱 현저히 세포증식율이 감소됨을 볼 수 있었다(p<0.05). 3. 배양 초기에는 세포들이 주로 섬유아세포 양으로 나타났으나, 밀생상태에 이르면서 점차 다각형 형태로 바뀌었다. 4. 배양 9일후 지방세포와 연골세포들이 관찰되었으며, 이들은 모두 dexamethasone이 첨가된 군에서 발견되었다. 5. 골결절은 ascorbic acid와 Na-${\beta}$-glycerophosphate가 첨가된 군에서만 형성되었으며, dexamethasone 을 병용첨가한 군에서 광화된 골결절이 현저히 증가됨을 관찰할 수 있었다. 6. 골결절 형성이 되지 않은 부위의 세포들은 평면형상을 이루고 있었으나, 골결절 부위를 덮고있는 세포들은 많은 세포돌기를 가진 조골세포양 세포들로 나타났으며, ascorbic acid, Na-${\beta}$-glycerophosphate 그리고 dexamethasone 을 첨가한 군에서는 침상의 돌기를 가진 광화물질들이 다발의 교원섬유들 사이에 현저히 많이 존재하였으며, 골결절 내부에는 매몰된 골세포(osteocyte)양 세포들이 관찰되었다.

• Maxillofacial Plastic and Reconstructive Surgery
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• 제28권6호
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• pp.511-519
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• 2006

Autogenous bone grafts have been considered the gold standard for maxillofacial bony defects. However, this procedure could entail a complicated surgical procedure as well as potential donor site morbidity. Possibly the best solution for bone-defect regeneration is a tissue engineering approach, i.e. the use of a combination of a suitable scaffold with osteogenic cells. A major source of osteogenic cells is the bone marrow. Bone marrow-derived mesenchymal stem cells are multipotent and have the ability to differentiate into osteoblastic, chondrocytic, and adipocytic lineage cells. However, the isolation of cells from bone marrow has someproblems when used in clinical setting. Bone marrow aspiration is sometimes potentially more invasive and painful procedure and carries of a risk of morbidity and infection. A minimally invasive, easily accessible alternative would be cells derived from periosteum. The periosteum also contains multipotent cells that have the potential to differentiate into osteoblasts and chondrocytes. In the present study, we evaluated the osteogenic activity and mineralization of cultured human periosteal-derived cells. Periosteal explants were harvested from mandibule during surgical extraction of lower impacted third molar. The periosteal cells were cultured in the osteogenic inductive medium consisting of DMEM supplemented with 10% fetal calf serum, 50g/ml L-ascorbic acid 2-phosphate, 10 nmol dexamethasone and 10 mM -glycerophosphate for 42 days. Periosteal-derived cells showed positive alkaline phosphatase (ALP) staining during 42 days of culture period. The formation of ALP stain showed its maximal manifestation at day 14 of culture period, then decreased in intensity during the culture period. ALP mRNA expression increased up to day 14 with a decrease thereafter. Osteocalcin mRNA expression appeared at day 7 in culture, after that its expression continuously increased in a time-dependent manner up to the entire duration of culture. Von Kossa-positive mineralization nodules were first present at day 14 in culture followed by an increased number of positive nodules during the entire duration of the culture period. In conclusion, our study showed that cultured human periosteal-derived cells differentiated into active osteoblastic cells that were involved in synthesis of bone matrix and the subsequent mineralization of the matrix. As the periosteal-derived cells, easily harvested from intraoral procedure such as surgical extraction of impacted third molar, has the excellent potential of osteogenic capacity, tissue-engineered bone using periosteal-derived cells could be the best choice in reconstruction of maxillofacial bony defects.

• Maxillofacial Plastic and Reconstructive Surgery
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• 제29권4호
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• pp.279-288
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• 2007

In the present study, we focused on stem cells in the dental papilla of the tooth germ. The tooth germ, sometimes called the tooth bud, is the primordial structure from which a tooth is formed. The tooth germ consists of the enamel organ, the dental papilla, and the dental follicle. The dental papilla lies below a cellular aggregation of the enamel organ. Mesenchymal cells within the dental papilla are responsible for formation of dentin and pulp of a tooth. Tooth germ disappears as a tooth is formed, but that of a third molar stays in the jawbone of a human until the age of 10 to 16, because third molars grow slowly. Impacted third molar tooth germs from young adults are sometimes extracted for orthodontic treatment. In the present study, we evaluated the osteogenic activity and mineralization of cultured human dental papilla-derived cells. Dental papillas were harvested from mandible during surgical extraction of lower impacted third molar from 3 patients aged 13-15 years. After passage 3, the dental papilla-derived cells were trypsinized and subsequently suspended in the osteogenic induction DMEM medium supplemented with 10% fetal bovine serum, 50 g/ml L-ascorbic acid 2-phosphate, 10 nM dexamethasone and 10 mM -glycerophosphate at a density of $1\;{\times}10^6\;cells/dish$ in a 100-mm culture dish. The dental papilla-derived cells were then cultured for 6 weeks and the medium was changes every 3 days during the incubation period. Dental papilla-derived cells showed positive alkaline phosphatase (ALP) staining during 42 days of culture period. The formation of ALP stain showed its maximal manifestation at day 7 of culture period, then decreased in intensity during the culture period. ALP mRNA level was largely elevated at 1 weeks and gradually decreased with culture time. Osteocalcin mRNA expression appeared at day 14 in culture, after that its expression continuously increased in a time-dependent manner up to day 28. The expression remained constant thereafter. Runx2 expression appeared at day 7 with no detection thereafter. Von Kossa-positive mineralization nodules were first present at day 14 in culture followed by an increased number of positive nodules during the entire duration of the culture period. Osteocalcin secretion was detectable in the culture medium from 1 week. The secretion of osteocalcin from dental papilla-derived cells into the medium greatly increased after 3 weeks although it showed a shallow increase by then. In conclusion, our study showed that cultured human dental papilla-derived cells differentiated into active osteoblastic cells that were involved in synthesis of bone matrix and the subsequent mineralization of the matrix.