暨南大学学报(自然科学与医学版)
暨南大學學報(自然科學與醫學版)
기남대학학보(자연과학여의학판)
JOURNAL OF JINAN UNIVERSITY(NATURAL SCIENCE)
2009年
6期
640-643
,共4页
纪玲%武延格%孙学峰%王正%杨林
紀玲%武延格%孫學峰%王正%楊林
기령%무연격%손학봉%왕정%양림
组织工程%软骨细胞%DiI荧光标记
組織工程%軟骨細胞%DiI熒光標記
조직공정%연골세포%DiI형광표기
tissue engineering%chondrocyte%DiI fluorescent labeling
目的:通过Dil荧光染料标记观察软骨细胞在聚乳酸/乙醇酸共聚物支架(PLGA)体外和体内培养环境中的生长状态,为研究组织工程化软骨探索一种理想的软骨细胞示踪方法.方法:体外分离培养大鼠剑突软骨细胞,应用DiI标记软骨细胞,通过MTT法测定细胞的增殖活性.DiI荧光标记的软骨细胞种植于PLGA支架上分两组:一组体外培养1周,另一组体外培养1周后,再植入同系大鼠大网膜体内培养1周.分别取出细胞一支架复合物,在荧光显微镜下观察体外和体内条件下软骨细胞的荧光表达情况.结果:应用DiI标记不影响软骨细胞的增殖,MTT测定结果显示标记组和对照组的A值未见显著性差异(P>0.05).标记后的软骨细胞显示环状红色荧光,胞核未着色.体外培养和体内培养的软骨细胞一支架复合物,均可在荧光显微镜下观察到红色荧光表达.结论:DiI荧光染料能够有效标记软骨细胞,标记的细胞一支架复合物可直接在荧光显微镜下进行观察,可作为体外和体内构建组织工程软骨的较好的示踪方法.
目的:通過Dil熒光染料標記觀察軟骨細胞在聚乳痠/乙醇痠共聚物支架(PLGA)體外和體內培養環境中的生長狀態,為研究組織工程化軟骨探索一種理想的軟骨細胞示蹤方法.方法:體外分離培養大鼠劍突軟骨細胞,應用DiI標記軟骨細胞,通過MTT法測定細胞的增殖活性.DiI熒光標記的軟骨細胞種植于PLGA支架上分兩組:一組體外培養1週,另一組體外培養1週後,再植入同繫大鼠大網膜體內培養1週.分彆取齣細胞一支架複閤物,在熒光顯微鏡下觀察體外和體內條件下軟骨細胞的熒光錶達情況.結果:應用DiI標記不影響軟骨細胞的增殖,MTT測定結果顯示標記組和對照組的A值未見顯著性差異(P>0.05).標記後的軟骨細胞顯示環狀紅色熒光,胞覈未著色.體外培養和體內培養的軟骨細胞一支架複閤物,均可在熒光顯微鏡下觀察到紅色熒光錶達.結論:DiI熒光染料能夠有效標記軟骨細胞,標記的細胞一支架複閤物可直接在熒光顯微鏡下進行觀察,可作為體外和體內構建組織工程軟骨的較好的示蹤方法.
목적:통과Dil형광염료표기관찰연골세포재취유산/을순산공취물지가(PLGA)체외화체내배양배경중적생장상태,위연구조직공정화연골탐색일충이상적연골세포시종방법.방법:체외분리배양대서검돌연골세포,응용DiI표기연골세포,통과MTT법측정세포적증식활성.DiI형광표기적연골세포충식우PLGA지가상분량조:일조체외배양1주,령일조체외배양1주후,재식입동계대서대망막체내배양1주.분별취출세포일지가복합물,재형광현미경하관찰체외화체내조건하연골세포적형광표체정황.결과:응용DiI표기불영향연골세포적증식,MTT측정결과현시표기조화대조조적A치미견현저성차이(P>0.05).표기후적연골세포현시배상홍색형광,포핵미착색.체외배양화체내배양적연골세포일지가복합물,균가재형광현미경하관찰도홍색형광표체.결론:DiI형광염료능구유효표기연골세포,표기적세포일지가복합물가직접재형광현미경하진행관찰,가작위체외화체내구건조직공정연골적교호적시종방법.
Aim:To find out a ideal cell labeling method for the study of tissue engineering cartilage, through observing the growth state of chondrocytes labeled by DiI and seeded on DegraPol scaffold in vitro and in vivo. Methods: Chondrocytes isolated from rat xyphoid was labeled by Dil, MTT test was used to determine the proliferation status of chondrocytes. Chondrocytes labeled by DiI were seeded onto PLAG scaffold, cultivated in vitro 1 week and cultivated in vivo 1 week after 1 week in vitro culture, respective-ly. The growth state of the DiI labeled cells by fluorescent microscope. Results: The fluoresce dye DiI showed no effect on the living status of chondrocytes. MTT test showed there was no significant difference between the proliferation of DiI labeled and unmarked chondrocytes. The chondrocytes labeled by DiI were observed clearly by fluorescent microscope. Conclusion:The chondrocytes labeled by DiI are well compatible with PLGA scaffold and observed continuously by fluorescent microscope. DiI label can be used as a good tracing method to observe tissue engineering cartilage.