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一种用于定量DNA细胞荧光测定法的改良吖啶黄素-福尔根试剂。

An improved acriflavine-Feulgen reagent for quantitative DNA cytofluorometry.

作者信息

Levinson J W, Langlois R G, Maher V M, McCormick J J

出版信息

J Histochem Cytochem. 1978 Aug;26(8):680-4. doi: 10.1177/26.8.690406.

Abstract

We have modified the acriflavine-Feulgen histochemical method for the quantitative determination of DNA by performing the staining of hydrolyzed cells affixed to cover slips with acriflavine dissolved in 90% ethanol. Compared to conventional techniques, in which the acriflavine is dissolved in aqueous HCl plus potassium metabisulfite, this method not only decreased non-Feulgen (background) staining in both the nucleus and the cytoplasm, but also increased the fluorescent intensity of Feulgen stained nuclei more than four-fold. Cells stained by our modified method exhibited a fluorescence maximum of 507 nm, which is similar to the 500 nm fluorescence maximum obtained with acriflavine bound to apurinic acid solution by a modification of the acriflavine-Feulgen method. These fluorescence maxima are in contrast to the 510 nm to 625 nm fluorescence maxima which are obtained when cells are stained according to conventional protocols. The fluorescence intensities of nuclei of synchronized cells stained by the modified method were proportional to DNA content. Thus, by the criteria of staining specificity, in situ and in solution fluorescence spectra agreement and quantitative staining, we conclude that our modified acriflavine-Feulgen method is more satisfactory for quantitatively measuring DNA in situ by cytofluorometry than the usual acriflavine-Feulgen method.

摘要

我们改进了吖啶黄-福尔根组织化学方法用于DNA的定量测定,具体做法是用溶于90%乙醇的吖啶黄对贴附在盖玻片上的水解细胞进行染色。与传统技术(吖啶黄溶于盐酸水溶液加焦亚硫酸钾)相比,该方法不仅降低了细胞核和细胞质中的非福尔根(背景)染色,还使福尔根染色细胞核的荧光强度增加了四倍多。用我们改进方法染色的细胞荧光最大值为507nm,这与通过改进吖啶黄-福尔根方法使吖啶黄与脱嘌呤酸溶液结合所获得的500nm荧光最大值相似。这些荧光最大值与按照传统方案对细胞进行染色时所获得的510nm至625nm荧光最大值形成对比。用改进方法对同步化细胞的细胞核进行染色,其荧光强度与DNA含量成正比。因此,根据染色特异性、原位和溶液荧光光谱一致性以及定量染色的标准,我们得出结论,与常用的吖啶黄-福尔根方法相比,我们改进的吖啶黄-福尔根方法在通过细胞荧光测定法定量原位测量DNA方面更令人满意。

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