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A study of some variables in a tetrazolium dye (MTT) based assay for cell growth and chemosensitivity.

机译:在基于四唑鎓染料(MTT)的细胞生长和化学敏感性测定中一些变量的研究。

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摘要

We have studied various factors involved in the optimal use of a tetrazolium (MTT) based colorimetric assay for cell growth and chemosensitivity. The assay is dependent on the ability of viable cells to metabolise a water-soluble tetrazolium salt into a water-insoluble formazan product. We have found that DMSO is the best solvent for dissolving the formazan product, especially where a significant amount of residual medium is left in the wells of the microtitre tray used for the assay. A reaction occurs between medium and a solution of MTT formazan in DMSO which changes the shape of the absorbance spectrum of the solution. The resulting optical density is not however greatly dependent upon the volume of added medium in the range 1-10 microliters. Between 10 and 40 microliters of added medium results in a gradually lower optical density than that produced by the smaller volumes. Above 40 microliters, the optical density increases again due to turbidity as protein precipitation occurs. When cells are incubated with MTT, the resulting optical density of the formazan product is dependent upon both the concentration of MTT and the incubation time. The optical density is stable for several hours after solution of the formazan in DMSO. A linear relationship is seen between optical density and cell number for incubation times of 2, 4, 6 or 24 h with 20 microliters of MTT (5 mg ml-1) added to 200 microliters medium. We have adopted 4 h as the standard incubation time for the assay. Only a small amount of MTT formazan product can be detected in the growth medium of wells in which cells have been exposed to MTT. Comparative chemosensitivity data for EMT6 mouse tumour cells show good agreement between results obtained using the MTT assay and results based on total cell count after a fixed period of growth.
机译:我们已经研究了各种因素,这些因素涉及基于四唑(MTT)的比色测定对细胞生长和化学敏感性的最佳使用。该测定取决于活细胞将水溶性四唑盐代谢为水不溶性甲maz产物的能力。我们发现DMSO是溶解甲maz产物的最佳溶剂,尤其是在用于测定的微量滴定盘孔中残留大量残留介质的情况下。介质与MTT甲maz的DMSO溶液之间发生反应,从而改变溶液的吸收光谱形状。但是,所得的光密度在很大程度上不取决于1-10微升范围内的添加介质的体积。在10到40微升之间添加的介质会导致光密度逐渐低于较小体积产生的光密度。超过40微升时,由于发生蛋白沉淀,浊度再次使光密度增加。当细胞与MTT一起孵育时,甲product产物的最终光密度取决于MTT的浓度和孵育时间。将甲maz溶于DMSO后,光密度在数小时内保持稳定。在向200微升培养基中添加20微升MTT(5 mg ml-1)的2、4、6或24 h的孵育时间中,可以看到光密度与细胞数量之间存在线性关系。我们将4小时作为测定的标准孵育时间。在细胞已经暴露于MTT的孔的生长培养基中,只能检测到少量的MTT甲maz产物。 EMT6小鼠肿瘤细胞的比较化学敏感性数据显示,使用MTT分析获得的结果与固定生长期后基于总细胞数的结果之间具有良好的一致性。

著录项

  • 作者

    Twentyman, P. R.; Luscombe, M.;

  • 作者单位
  • 年度 1987
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  • 原文格式 PDF
  • 正文语种 {"code":"en","name":"English","id":9}
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