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作 者:杨文艺[1] 严轶文[1] 洪江[1] 孙宝贵[1]
机构地区:[1]上海交通大学第一人民医院心内科,上海200080
出 处:《上海交通大学学报(医学版)》2007年第3期307-310,共4页Journal of Shanghai Jiao tong University:Medical Science
基 金:上海市科委基金(03DJ14019)~~
摘 要:目的探讨外周血单个核细胞向平滑肌祖细胞分化的培养方法。方法分离人外周血单个核细胞,接种于加有牛垂体提取物的M-199培养基中,第8天予以血小板源性生长因子-BB(PDGF-BB)刺激促进细胞分化,刺激15 d后运用RT-PCR、免疫荧光法和Western blot检测平滑肌细胞特异性α-辅肌动蛋白(α-SMA)、平滑肌肌球蛋白重链(SMMHC)、调宁蛋白(Calponin)、CD34、Tie-2和Flk-1的表达,并以流式细胞技术检测培养细胞α-SMA阳性表达率,对培养细胞进行鉴定。结果在PDGF-BB刺激培养15 d后细胞表达平滑肌细胞的标记α-SMA、SM MHC和Calponin,同时表达干细胞的标记CD34,并发现其Flk-1阳性表达,Tie-2阴性表达。PDGF-BB刺激后细胞α-SMA阳性表达率为(90.57±5.63)%,与阴性对照细胞之间有统计学差异(P<0.05)。结论外周血单个核细胞分离后第8天,使用PDGF-BB刺激可使其向平滑肌前体细胞分化,提出了一种新的外周血单个核细胞向平滑肌细胞分化的培养方法。Objective To optimize methods of culturing smooth muscle progenitor cells (SPCs) from mononuclear cells (MNCs) of peripheral blood. Methods Human MNCs isolated from buffy coat were seeded on M-199 with bovine pituitary extraction. On the eighth day outgrowth cells were stimulated with platelet-derived growth factor-BB (PDGF-BB). Fifteen days later, immunofluorescence, Western blot or RT-PCR was used to analyzed the expression of smooth muscle cell specific α-actin (α-SMA), smooth muscle myosin heavy chain(SM MHC), Calponin, CD34, Tie-2 and Flk-1, and fluorescence activated cell sorter was employed to examine α-SMA positive cells ratio. Results The cells stimulated by PDGF-BB for 15 d were positive for α-SMA, SM MHC, Calponin, CD34 and Flk-1, but negative for Tie-2. The α-SMA positive cells ratio was (90.57 ± 5.63 )% , significantly different from that of the control( P 〈 0.05 ). Conclusion Circulating MNCs stimulated by PDGF-BB from the eighth day may differentiate into SPCs in vitro. A new method of culturing SPCs from MNCs of peripheral blood is established.
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