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流式细胞术中荧光(微珠)可追溯性的概念:利用饱和与微观单分子漂白

Concept for the traceability of fluorescence (beads) in flow cytometry: exploiting saturation and microscopic single molecule bleaching.

作者信息

Neukammer Jörg, Gohlke Carsten, Krämer Benedikt, Roos Martin

机构信息

Physikalisch-Technische Bundesanstalt (PTB), Working Group 8.32, Berlin, Germany.

出版信息

J Fluoresc. 2005 May;15(3):433-41. doi: 10.1007/s10895-005-2635-y.

Abstract

We have determined the fluorescence yield of stained micro beads, used for calibration purposes in flow cytometry, as function of the irradiance of the exciting laser beam. A rate equation model has been applied to derive the number of fluorescence molecules carried by each micro bead. To derive in situ photo-physical properties of the specific dye, required for the rate equation model, we discuss an approach based on flow cytometric sorting of micro beads, which have passed two laser beams with properly chosen different irradiances, and subsequent observation of single molecule bleaching employing high sensitivity microscopy. The feasibility of our approach is demonstrated presenting first results concerning saturation of fluorescence of beads in flow and single molecule bleaching by high sensitivity microscopy.

摘要

我们已确定用于流式细胞术校准目的的染色微珠的荧光产率与激发激光束辐照度的函数关系。应用速率方程模型来推导每个微珠携带的荧光分子数量。为了推导速率方程模型所需的特定染料的原位光物理性质,我们讨论了一种基于对已通过两个辐照度适当不同的激光束的微珠进行流式细胞术分选,并随后使用高灵敏度显微镜观察单分子漂白的方法。通过展示关于流动中微珠荧光饱和以及高灵敏度显微镜下的单分子漂白的初步结果,证明了我们方法的可行性。

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