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作 者:陈孙霞 王晓庆 徐晓恩[1] 姜英华[1] 刘锋[1]
机构地区:[1]复旦大学生物医学研究院,上海200032 [2]复旦大学化学系,上海200433
出 处:《复旦学报(医学版)》2014年第5期602-609,共8页Fudan University Journal of Medical Sciences
基 金:国家重点基础研究发展计划(973计划)(2011CB910702;2013CB911201)~~
摘 要:目的提高mCherry红色荧光蛋白(red fluorescence protein,RFP)在结肠癌细胞中的表达,从而可以通过检测共培养体系中细胞的荧光值来分析结肠癌细胞的增殖,以利于结肠癌肿瘤微环境的研究。方法用293FT细胞制备pBMN-mCherry病毒液。利用多次感染(1~4次)的方法提高RFP在结肠癌细胞系HT29、LoVo、SW620及HCTll6中的表达,经流式细胞仪检测得到不同感染次数细胞RFP标记的阳性率,并将高阳性表达RFP的结肠癌细胞HT29的荧光值与细胞数量关系进行比较,分析评价两者的线性关系。结果通过优化,荧光标记效率大幅度提高。结肠癌肿瘤成纤维细胞共培养中,荧光值与细胞数量线性关系R^2〉0.9;该方法成功用于检测共培养体系中单种细胞增殖。结论在结肠癌细胞和成纤维细胞的共培养体系中,结肠癌细胞的增殖可以通过检测细胞荧光值来分析。Objective To improve the expression efficiency of the mCherry red fluorescence protein (RFP) in colorectal cancer cells. So that the proliferation of colon cancer cells in the co-culture system can be easily monitored by measuring the fluorescence signals, which is suitable for colorectal cancer microenvironment analysis. Methods 293FT cells were used to produce the pBMN-mCherry virus, which was used to infect the colon cancer cell lines HT29, LoVo, SW620 and HCT116. The labeling procedure was repeated up to four times to improve the labeling efficiency of the RFP. The positively labeled cells of each round labeling were detected by flow cytometer. The fluorescence value of HT29 with highly labeled RFP was compared with its cell count and the linear relationship between both values was evaluated. Results After optimization, the fluorescence labeling efficiency was greatly
关 键 词:红色荧光蛋白(RFP) 共培养 细胞增殖 结肠癌
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