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用于检测细胞培养物中支原体污染的Hoechst 33258染色:一种减少荧光光漂白的方法

Hoechst 33258 staining for detecting mycoplasma contamination in cell cultures: a method for reducing fluorescence photobleaching.

作者信息

Battaglia M, Pozzi D, Grimaldi S, Parasassi T

机构信息

Institute of Experimental Medicine, National Research Council, CNR, Rome, Italy.

出版信息

Biotech Histochem. 1994 May;69(3):152-6. doi: 10.3109/10520299409106277.

Abstract

DNA fluorochrome staining with Hoechst 33258 bisbenzimide is commonly used for detection of mycoplasma contamination in cell cultures. Photobleaching of Hoechst 33258 is pronounced under the conditions of intense illumination, high magnification and resolution required for detection of mycoplasmas. To reduce photobleaching we investigated the effects of some antioxidant molecules, p-phenylenediamine (PPD), n-propyl gallate (NPG) and 1,4-diazabicyclo(2,2,2)octane (DABCO), which are known to reduce the fading rate of fluorescein. Mycoplasma-contaminated cell monolayers were stained with Hoechst 33258 and mounted in glycerol containing different amounts of antioxidant additives. The cells were examined in an epifluorescence microscope, and the emitted light intensity was recorded. Results showed that PPD and, to a lower degree, NPG, retarded the photobleaching of Hoechst 33258-stained cells, whereas DABCO was not effective. However, fluorescence half-life was increased about three-fold by NPG and almost 20-fold by PPD. The rate of fluorescence fading of Hoechst 33258 can therefore be retarded by PPD, with obvious advantages for reading and photographic recording of results.

摘要

用Hoechst 33258双苯甲酰亚胺进行DNA荧光染色常用于检测细胞培养物中的支原体污染。在检测支原体所需的强光照射、高放大倍数和分辨率条件下,Hoechst 33258的光漂白现象很明显。为了减少光漂白,我们研究了一些抗氧化分子对苯二胺(PPD)、没食子酸正丙酯(NPG)和1,4 - 二氮杂双环(2,2,2)辛烷(DABCO)的作用,已知这些分子可降低荧光素的褪色速率。用Hoechst 33258对受支原体污染的细胞单层进行染色,并将其封固在含有不同量抗氧化添加剂的甘油中。在落射荧光显微镜下检查细胞,并记录发射光强度。结果表明,PPD以及程度稍低的NPG可延缓Hoechst 33258染色细胞的光漂白,而DABCO无效。然而,NPG使荧光半衰期增加约三倍,PPD使其增加近20倍。因此,PPD可延缓Hoechst 33258的荧光褪色速率,这对于结果的读取和摄影记录具有明显优势。

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