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Tracking cell proliferation using the far red fluorescent dye SNARF-1

机译:使用远红色荧光染料SNARF-1跟踪细胞增殖

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Background: The [H-3]thymidine incorporation assay and staining of living cells with fluorescent dyes like carboxyfluorescein diacetate, succinimidyl ester (CFSE) have evolved as valuable methods for studying T cell responses. To assess proliferation of cells already labeled by FITC, CFSE, GFP, or other "green" molecules or to simultaneously track two otherwise indistinguishable cell populations in mixed cell cultures, it would be desirable to have a dye with distinct fluorescent properties for this application. Methods: We analyzed the dilution of the far red fluorescent dye SNARF-1 in proliferating cells by flow cytometric analysis. The results were compared with the CFSE dilution technique as well as the [H-3]thymidine incorporation assay. Results: Staining of primary human lymphocytes revealed that SNARF-1 labeling was equivalent to USE for estimating proportions of proliferating cells in stimulated cell cultures and yielded results comparable to [H-3]thymidine incorporation. We showed that SNARF-1 offers the possibility to simultaneously analyze the proliferation of phenotypically indistinguishable subsets of hematopoietic cells and can also be used to track uniformly proliferating, non hematopoietic cells like HEK293. Conclusions: In summary, we have demonstrated that labeling of cells with SNARF-1 allows for estimating cell proliferation of cells of hematopoietic and non-hematopoietic origin. (c) 2007 Clinical Cytometry Society.
机译:背景:[H-3]胸苷掺入法以及用荧光染料如二乙酸羧基荧光素,琥珀酰亚胺酯(CFSE)对活细胞进行染色已发展成为研究T细胞反应的有价值的方法。为了评估已经被FITC,CFSE,GFP或其他“绿色”分子标记的细胞的增殖,或同时在混合细胞培养物中追踪两个原本无法区分的细胞群,对于这种应用,需要一种具有独特荧光特性的染料。方法:我们通过流式细胞仪分析了增殖细胞中远红色荧光染料SNARF-1的稀释度。将结果与CFSE稀释技术以及[H-3]胸苷掺入法进行了比较。结果:对人类原代淋巴细胞的染色显示,SNARF-1标记与USE等效,可用于估计受刺激细胞培养物中增殖细胞的比例,并产生与[H-3]胸苷掺入相当的结果。我们表明,SNARF-1提供了同时分析造血细胞表型无法区分的亚群增殖的可能性,并且还可以用于追踪均匀增殖的非造血细胞(如HEK293)。结论:总之,我们已经证明了用SNARF-1标记细胞可以估计造血和非造血来源的细胞的细胞增殖。 (c)2007临床细胞计数学会。

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