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使用 DNA 染料荧光增强剂定量固定黏附细胞。

Quantification of fixed adherent cells using a strong enhancer of the fluorescence of DNA dyes.

机构信息

Institute of Molecular and Translational Medicine, Faculty of Medicine and Dentistry, Palacký University in Olomouc, Olomouc, 779 00, Czech Republic.

出版信息

Sci Rep. 2019 Jun 18;9(1):8701. doi: 10.1038/s41598-019-45217-9.

Abstract

Cell quantification is widely used in basic or applied research. The current sensitive methods of cell quantification are exclusively based on the analysis of non-fixed cells and do not allow the simultaneous detection of various cellular components. A fast, sensitive and cheap method of the quantification of fixed adherent cells is described here. It is based on the incubation of DAPI- or Hoechst 33342-stained cells in a solution containing SDS. The presence of SDS results in the quick de-staining of DNA and simultaneously, in an up-to-1,000-fold increase of the fluorescence intensity of the used dyes. This increase can be attributed to the micelle formation of SDS. The method is sufficiently sensitive to reveal around 50-70 human diploid cells. It is compatible with immunocytochemical detections, the detection of DNA replication and cell cycle analysis by image cytometry. The procedure was successfully tested for the analysis of cytotoxicity. The method is suitable for the quantification of cells exhibiting low metabolic activity including senescent cells. The developed procedure provides high linearity and the signal is high for at least 20 days at room temperature. Only around 90 to 120 minutes is required for the procedure's completion.

摘要

细胞定量广泛应用于基础或应用研究。目前,细胞定量的敏感方法完全基于非固定细胞的分析,不允许同时检测各种细胞成分。本文描述了一种快速、敏感和廉价的固定贴壁细胞定量方法。它基于 DAPI 或 Hoechst 33342 染色细胞在含有 SDS 的溶液中的孵育。SDS 的存在导致 DNA 快速褪色,同时使用的染料的荧光强度增加高达 1000 倍。这种增加可以归因于 SDS 的胶束形成。该方法足够灵敏,可检测到约 50-70 个人二倍体细胞。它与免疫细胞化学检测、通过图像细胞术检测 DNA 复制和细胞周期分析兼容。该程序已成功用于细胞毒性分析。该方法适用于定量代谢活性低的细胞,包括衰老细胞。所开发的程序提供了高线性度,信号在室温下至少 20 天内保持高。该程序完成仅需约 90 至 120 分钟。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/bb76/6581942/a972842b8314/41598_2019_45217_Fig1_HTML.jpg

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