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一种用于在流式细胞术中扣除细胞自发荧光的单激光方法。

A single laser method for subtraction of cell autofluorescence in flow cytometry.

作者信息

Alberti S, Parks D R, Herzenberg L A

出版信息

Cytometry. 1987 Mar;8(2):114-9. doi: 10.1002/cyto.990080203.

Abstract

In flow cytometry cell autofluorescence often interferes with efforts to measure low levels of bound fluorescent antibody. We have developed a way to correct for autofluorescence on a cell-by-cell basis. This results in improved estimates of real staining and better separation of the fluorescence histograms of stained and non-stained cells. Using a single laser, two-color fluorescence measurement system and two-color compensation electronics, autofluorescence and one fluorescent reagent are measured (rather than two fluorescent reagents). With fluorescein-conjugated antibodies the signal in the 515 to 555 nm range (green fluorescence) includes both fluorescein emission and part of the cellular autofluorescence. In the cases we have investigated, autofluorescence collected at wavelengths above 580 nm ("red") is well correlated with the green autofluorescence of the cells. A fraction of this red fluorescence is subtracted from the green fluorescence to produce an adjusted fluorescein output on which unstained cells have zero average signal. Use of this method facilitates the selection of rare cells transfected with surface antigen genes. Culture conditions affect the level of autofluorescence and the balance between red and green autofluorescence. When applied with fluorescein-conjugated reagents, the technique is compatible with the use of propidium iodide for live/dead cell discrimination.

摘要

在流式细胞术中,细胞自发荧光常常干扰测量低水平结合荧光抗体的工作。我们已开发出一种逐细胞校正自发荧光的方法。这使得对真实染色的估计得到改善,并且染色细胞和未染色细胞的荧光直方图分离得更好。使用单激光、双色荧光测量系统和双色补偿电子设备,测量自发荧光和一种荧光试剂(而非两种荧光试剂)。对于荧光素偶联抗体,515至555纳米范围内的信号(绿色荧光)包括荧光素发射和部分细胞自发荧光。在我们研究的案例中,在波长高于580纳米(“红色”)处收集的自发荧光与细胞的绿色自发荧光高度相关。从绿色荧光中减去一部分这种红色荧光,以产生调整后的荧光素输出,在该输出上未染色细胞的平均信号为零。使用这种方法有助于选择转染了表面抗原基因的稀有细胞。培养条件会影响自发荧光水平以及红色和绿色自发荧光之间的平衡。当与荧光素偶联试剂一起使用时,该技术与使用碘化丙啶进行活/死细胞鉴别兼容。

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