中国组织工程研究
中國組織工程研究
중국조직공정연구
Journal of Clinical Rehabilitative Tissue Engineering Research
2014年
30期
4790-4796
,共7页
张瑾%张子琦%张滟%许珉
張瑾%張子琦%張滟%許珉
장근%장자기%장염%허민
生物材料%软骨生物材料%微囊%骨髓间充质干细胞%软骨细胞%共培养%诱导分化
生物材料%軟骨生物材料%微囊%骨髓間充質榦細胞%軟骨細胞%共培養%誘導分化
생물재료%연골생물재료%미낭%골수간충질간세포%연골세포%공배양%유도분화
bone marrow%stem cells%chondrocytes
背景:以往诱导骨髓间充质干细胞定向分化的直接接触共培养法、Transwel 膜非接触共培养诱导法存在干细胞纯度低、增殖缓慢等不足。目的:对比分析微囊化共培养体系与传统Transwel 共培养体系对骨髓间充质干细胞的诱导效果。方法:实验组取第3代兔骨髓间充质干细胞与微囊化的第2代兔关节软骨细胞,按1∶1的比例在Transwel小室进行共培养,同时设置第3代兔骨髓间充质干细胞与第2代兔关节软骨细胞共培养于Transwel 小室的传统共培养组,以及纯干细胞培养组。MTT法对比3组干细胞的增殖率,甲苯胺蓝染色、番红花O染色观察软骨基质的合成,阿利新蓝染色法和Elisa法定量测量糖胺聚糖与Ⅱ型胶原蛋白的合成。结果与结论:传统共培养组细胞增殖率低于实验组与纯干细胞培养组(P<0.05)。实验组细胞糖胺聚糖和Ⅱ型胶原蛋白水平高于传统共培养组、纯干细胞培养组(P<0.05),甲苯胺蓝染色、番红花O染色强度强于传统共培养组、纯干细胞培养组。表明微囊化的软骨细胞能够成功诱导骨髓间充质干细胞向成软骨方向定向分化,且诱导效果优于传统的Transwel 膜分离共培养法。
揹景:以往誘導骨髓間充質榦細胞定嚮分化的直接接觸共培養法、Transwel 膜非接觸共培養誘導法存在榦細胞純度低、增殖緩慢等不足。目的:對比分析微囊化共培養體繫與傳統Transwel 共培養體繫對骨髓間充質榦細胞的誘導效果。方法:實驗組取第3代兔骨髓間充質榦細胞與微囊化的第2代兔關節軟骨細胞,按1∶1的比例在Transwel小室進行共培養,同時設置第3代兔骨髓間充質榦細胞與第2代兔關節軟骨細胞共培養于Transwel 小室的傳統共培養組,以及純榦細胞培養組。MTT法對比3組榦細胞的增殖率,甲苯胺藍染色、番紅花O染色觀察軟骨基質的閤成,阿利新藍染色法和Elisa法定量測量糖胺聚糖與Ⅱ型膠原蛋白的閤成。結果與結論:傳統共培養組細胞增殖率低于實驗組與純榦細胞培養組(P<0.05)。實驗組細胞糖胺聚糖和Ⅱ型膠原蛋白水平高于傳統共培養組、純榦細胞培養組(P<0.05),甲苯胺藍染色、番紅花O染色彊度彊于傳統共培養組、純榦細胞培養組。錶明微囊化的軟骨細胞能夠成功誘導骨髓間充質榦細胞嚮成軟骨方嚮定嚮分化,且誘導效果優于傳統的Transwel 膜分離共培養法。
배경:이왕유도골수간충질간세포정향분화적직접접촉공배양법、Transwel 막비접촉공배양유도법존재간세포순도저、증식완만등불족。목적:대비분석미낭화공배양체계여전통Transwel 공배양체계대골수간충질간세포적유도효과。방법:실험조취제3대토골수간충질간세포여미낭화적제2대토관절연골세포,안1∶1적비례재Transwel소실진행공배양,동시설치제3대토골수간충질간세포여제2대토관절연골세포공배양우Transwel 소실적전통공배양조,이급순간세포배양조。MTT법대비3조간세포적증식솔,갑분알람염색、번홍화O염색관찰연골기질적합성,아리신람염색법화Elisa법정량측량당알취당여Ⅱ형효원단백적합성。결과여결론:전통공배양조세포증식솔저우실험조여순간세포배양조(P<0.05)。실험조세포당알취당화Ⅱ형효원단백수평고우전통공배양조、순간세포배양조(P<0.05),갑분알람염색、번홍화O염색강도강우전통공배양조、순간세포배양조。표명미낭화적연골세포능구성공유도골수간충질간세포향성연골방향정향분화,차유도효과우우전통적Transwel 막분리공배양법。
BACKGROUND:Traditional coculture methods for directional differentiation of bone marrow mesenchymal stem cells, such as direct contact method and Transwel coculture system, appear to have low purity and slow proliferation. OBJECTIVE:To compare the inductive effect of microcapsule coculture system and traditional transwel coculture system on the differentiation of bone marrow mesenchymal stem cells. METHODS:The passage 2 microcapsuled chondrocytes and the passage 3 bone marrow mesenchymal stem cells harvested from rabbits were co-cultured at a ratio of 1:1 in a Transwel chamber. Another passage 2 chondrocytes and passage 3 bone marrow mesenchymal stem cells were co-cultured using traditional transwel coculture system. Pure bone marrow mesenchymal stem cells were served as controls. MTT assay was used to compare cellproliferation, toluidine blue staining and safranine O staining were used for observation of cartilage matrix synthesis, alcian blue staining and ELISA test were used to measure glycosaminoglycans and synthesis of type II col agen, respectively. RESULTS AND CONCLUSION:Compared with the traditional co-culture method, the microcapsule coculture system and pure culture method showed better cellproliferation (P<0.05). The levels of glycosaminoglycans and type II col agen were higher in the microcapsule coculture group than the traditional coculture group and pure culture group (P<0.05). Moreover, the microcapsule coculture group showed better outcomes in toluidine blue staining and safranine O staining than the traditional coculture group and pure culture group. These findings indicate that the microcapsule coculture system is more effective in the induction of bone marrow mesenchymal stem cells than traditional Transwel coculture system.
