中国组织工程研究
中國組織工程研究
중국조직공정연구
Journal of Clinical Rehabilitative Tissue Engineering Research
2013年
19期
3430-3436
,共7页
干细胞%骨髓干细胞%成脂分化%快速诱导%罗格列酮%吡咯列酮%噻唑烷二酮%胰岛素增敏剂%干细胞图片文章
榦細胞%骨髓榦細胞%成脂分化%快速誘導%囉格列酮%吡咯列酮%噻唑烷二酮%胰島素增敏劑%榦細胞圖片文章
간세포%골수간세포%성지분화%쾌속유도%라격렬동%필각렬동%새서완이동%이도소증민제%간세포도편문장
stem cells%bone marrow-derived stem cells%adipogenic differentiation%rapid induction%rosiglitazone%pioglitazone%thiazolidinediones%insulin sensitizer%stem cel photographs-containing paper
背景:目前常用的成脂刺激剂主要由胰岛素、地塞米松、IBMX 和吲哚美辛组成,该体系涉及处理因素多、诱导周期长且对细胞毒性大,不利于脂肪形成抑制效应的研究.目的:建立快速诱导大鼠骨髓间充质干细胞成脂分化的培养体系.方法:大鼠全骨髓细胞原代培养,胰酶消化传代,富集形态均质的间充质干细胞,利用过氧化物酶体增殖物活化受体γ激动剂噻唑烷二酮类药物罗格列酮和吡咯列酮体外单独诱导大鼠骨髓间充质干细胞成脂分化,设立无糖、低糖和高糖 DMEM 三种基础培养体系,以经典的成脂刺激剂作为阳性对照,在诱导的不同时间点对分化细胞进行形态学观察和油红O染色.结果与结论:与经典成脂刺激剂相比,罗格列酮或吡咯列酮单独均能诱导大鼠骨髓间充质干细胞向脂肪细胞分化,吡咯列酮诱导48 h和罗格列酮诱导72 h均可观察到富含脂滴或脂泡以及油红O染色的阳性细胞,吡咯列酮与罗格列酮的最佳诱导浓度分别为0.125 mmol/L和10μmol/L,而高糖环境利于大鼠骨髓间充质干细胞成脂分化.说明基于高糖培养环境的以吡咯列酮或罗格列酮做为成脂刺激剂的培养体系可快速诱导大鼠骨髓间充质干细胞向脂肪细胞分化.
揹景:目前常用的成脂刺激劑主要由胰島素、地塞米鬆、IBMX 和吲哚美辛組成,該體繫涉及處理因素多、誘導週期長且對細胞毒性大,不利于脂肪形成抑製效應的研究.目的:建立快速誘導大鼠骨髓間充質榦細胞成脂分化的培養體繫.方法:大鼠全骨髓細胞原代培養,胰酶消化傳代,富集形態均質的間充質榦細胞,利用過氧化物酶體增殖物活化受體γ激動劑噻唑烷二酮類藥物囉格列酮和吡咯列酮體外單獨誘導大鼠骨髓間充質榦細胞成脂分化,設立無糖、低糖和高糖 DMEM 三種基礎培養體繫,以經典的成脂刺激劑作為暘性對照,在誘導的不同時間點對分化細胞進行形態學觀察和油紅O染色.結果與結論:與經典成脂刺激劑相比,囉格列酮或吡咯列酮單獨均能誘導大鼠骨髓間充質榦細胞嚮脂肪細胞分化,吡咯列酮誘導48 h和囉格列酮誘導72 h均可觀察到富含脂滴或脂泡以及油紅O染色的暘性細胞,吡咯列酮與囉格列酮的最佳誘導濃度分彆為0.125 mmol/L和10μmol/L,而高糖環境利于大鼠骨髓間充質榦細胞成脂分化.說明基于高糖培養環境的以吡咯列酮或囉格列酮做為成脂刺激劑的培養體繫可快速誘導大鼠骨髓間充質榦細胞嚮脂肪細胞分化.
배경:목전상용적성지자격제주요유이도소、지새미송、IBMX 화신타미신조성,해체계섭급처리인소다、유도주기장차대세포독성대,불리우지방형성억제효응적연구.목적:건립쾌속유도대서골수간충질간세포성지분화적배양체계.방법:대서전골수세포원대배양,이매소화전대,부집형태균질적간충질간세포,이용과양화물매체증식물활화수체γ격동제새서완이동류약물라격렬동화필각렬동체외단독유도대서골수간충질간세포성지분화,설립무당、저당화고당 DMEM 삼충기출배양체계,이경전적성지자격제작위양성대조,재유도적불동시간점대분화세포진행형태학관찰화유홍O염색.결과여결론:여경전성지자격제상비,라격렬동혹필각렬동단독균능유도대서골수간충질간세포향지방세포분화,필각렬동유도48 h화라격렬동유도72 h균가관찰도부함지적혹지포이급유홍O염색적양성세포,필각렬동여라격렬동적최가유도농도분별위0.125 mmol/L화10μmol/L,이고당배경리우대서골수간충질간세포성지분화.설명기우고당배양배경적이필각렬동혹라격렬동주위성지자격제적배양체계가쾌속유도대서골수간충질간세포향지방세포분화.
BACKGROUND:The commonly used adipogenic irritants consist of insulin, dexamethasone, 3-isobutyl-1-methylxanthine and indomethacin. The system is not conducive to the study of adipogenesis inhibitory effect due to the disadvantages of multi-processing factors, long induction period and great cytotoxicity. OBJECTIVE:To develop a rapid culture method to induce adipogenic differentiation of rat bone marrow mesenchymal stem cel s. METHODS:Rat whole bone marrow cel s were primary cultured and passaged with trypsin digestion method. The homogeneous mesenchymal stem cel s were enriched, and adipogenic differentiation of rat bone marrow mesenchymal stem cel s were in vitro induced with thiazolidinediones (rosiglitazone and pioglitazone), the agonists of peroxisome proliferator-activated receptorγ. Glucose-free, low glucose and high glucose Dulbecco's modified Eagle's media were established, and the classic adipogenic irritants were as the positive control. Morphological observation and oil red O staining were performed to observe the differentiated cel s at different time points. RESULTS AND CONCLUSION:Compared with the classic adipogenic irritants, the rosiglitazone and pioglitazone could induce the rat bone marrow mesenchymal stem cel s to differentiate into adipocytes, and accumulations of lipid droplets or lipid vesicles and oil red O staining positive cel s could be observed after induced with pioglitazone for 48 hours and rosiglitazone for 72 hours. The optional concentration of pioglitazone and rosiglitazone for adipogenic induction was 0.125 mmol/L and 10μmol/L, respectively. High glucose could enhance the adipogenic differentiation of rat bone marrow mesenchymal stem cel s. The culture system with the adipogenic irritants of pioglitazone and rosiglitazone under the high glucose environment can rapidly induce the rat bone marrow mesenchymal stem cel s to differentiate into adipocytes.
