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用于流式细胞术的相分辨荧光寿命测量。

Phase-resolved fluorescence lifetime measurements for flow cytometry.

作者信息

Pinsky B G, Ladasky J J, Lakowicz J R, Berndt K, Hoffman R A

机构信息

Becton Dickinson Immunocytometry Systems, San Jose, California 95131.

出版信息

Cytometry. 1993;14(2):123-35. doi: 10.1002/cyto.990140204.

Abstract

A flow cytometer capable of measuring fluorescence lifetimes by the phase shift method has been built and evaluated. Under optimal conditions, the resolution of the fluorescence lifetime measurement is shown to be under 200 picoseconds. Pulse intensity variations are normalized using limiting amplifiers and electronic filtering. Normalization of signal intensities provides a lifetime measurement that is independent of fluorescence intensity over at least a 50-fold (17 dB) range in fluorescence intensity. The fluorescence lifetimes of unbound dye, fluorescent beads, cells stained with ethidium bromide, propidium iodide, and phycoerythrin-conjugated monoclonal antibodies have been measured. The fluorescence lifetimes measured for these particles are well correlated with lifetime measurements made using a standard fluorimeter. Cells stained with ethidium bromide and propidium iodide at various nucleotide-to-dye ratios are shown to exhibit similar behavior to static cuvette measurements. The fluorescence lifetime parameter is also shown to resolve phycoerthyrin fluorescence from propidium iodide fluorescence.

摘要

一台能够通过相移法测量荧光寿命的流式细胞仪已被构建并评估。在最佳条件下,荧光寿命测量的分辨率显示在200皮秒以下。使用限幅放大器和电子滤波对脉冲强度变化进行归一化。信号强度的归一化提供了一种寿命测量方法,该方法在至少50倍(17分贝)的荧光强度范围内与荧光强度无关。已测量了未结合染料、荧光珠、用溴化乙锭、碘化丙啶和藻红蛋白偶联单克隆抗体染色的细胞的荧光寿命。这些颗粒的荧光寿命测量值与使用标准荧光计进行的寿命测量值高度相关。用不同核苷酸与染料比例的溴化乙锭和碘化丙啶染色的细胞表现出与静态比色皿测量相似的行为。荧光寿命参数还显示出能够区分碘化丙啶荧光和藻红蛋白荧光。

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