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一种用于人实体瘤多参数细胞分析的细胞自发荧光简单校正方法。

A simple correction for cell autofluorescence for multiparameter cell-based analysis of human solid tumors.

作者信息

Smith Charles A, Pollice Agnese, Emlet David, Shackney Stanley E

机构信息

Laboratory of Cancer Cell Biology and Genetics, Department of Human Oncology, Allegheny Singer Research Institute, Allegheny General Hospital, Pittsburgh, Pennsylvania 15212, USA.

出版信息

Cytometry B Clin Cytom. 2006 Mar;70(2):91-103. doi: 10.1002/cyto.b.20090.

Abstract

BACKGROUND

Corrections that have been proposed to minimize the unwanted contribution of cell autofluorescence to the total fluorescence signal often require either specialized instrumentation or the sacrifice of a data channel so as to perform a measurement that can be used to correct for autofluorescence in individual cells. Here we propose a simple cell by cell correction for autofluorescence that is suitable for multiparameter laser scanning cytometry (LSC) studies in human solid tumors that relies on the ratio of mean autofluorescence to mean total cell fluorescence (mean Flauto/mean Fltotal). This approach assumes a correlation between the autofluorescence component and the total signal in individual cells. This correction does not require specialized instrumentation, and does not sacrifice a data channel in multiparameter studies. A potential disadvantage is that errors may be introduced by the assumption of a correlation between the two components of the total fluorescence signal in individual cells in samples in which no such correlation exists.

METHODS

Distributions of cell autofluorescence and total Her-2/neu cell fluorescence were obtained separately by LSC in three human breast cancer cell lines and in three samples of primary human lung cancer. In the breast cancer cell lines, autofluorescence measurements and Her-2/neu measurements were also obtained on the same cells.

RESULTS

We show that there is a partial correlation between autofluorescence and total Her-2/neu/FITC fluorescence in individual cells in the three breast cancer cell lines. We also show that the results of a ratio-based autofluorescence correction agree with those based on a true cell by cell correction. Computer simulation studies suggest that in samples with no correlation between the autofluorescence component and the true probe/dye fluorescence component, the ratio correction produces robust estimates of the mean true fluorescence signal, with relatively small but systematic underestimates of the coefficient of variation of such measurements under conditions commonly encountered in the measurement of human solid tumors.

CONCLUSIONS

A simple cell by cell correction for autofluorescence based on the ratio of mean Flauto to mean Fltotal can be applied in cell samples in which there is a correlation between cell autofluorescence and true probe/dye fluorescence in individual cells. In cell samples that lack this correlation, or in which it is not known whether such a correlation exists, this correction can be used with the reservation that there is a systematic but relatively small underestimation of the degree of variability of the measurements.

摘要

背景

为尽量减少细胞自发荧光对总荧光信号的不必要贡献而提出的校正方法,通常需要专门的仪器设备,或者牺牲一个数据通道来进行测量,以便校正单个细胞中的自发荧光。在此,我们提出一种针对自发荧光的简单逐个细胞校正方法,适用于人类实体瘤的多参数激光扫描细胞术(LSC)研究,该方法依赖于平均自发荧光与平均总细胞荧光的比值(平均自发荧光/平均总荧光)。此方法假定单个细胞中自发荧光成分与总信号之间存在相关性。这种校正不需要专门的仪器设备,并且在多参数研究中不会牺牲数据通道。一个潜在的缺点是,在样本中单个细胞的总荧光信号的两个成分之间不存在这种相关性的情况下,由于假定两者存在相关性,可能会引入误差。

方法

通过LSC分别获取三种人乳腺癌细胞系以及三个原发性人肺癌样本中细胞自发荧光和Her-2/neu细胞总荧光的分布。在乳腺癌细胞系中,还对同一细胞进行了自发荧光测量和Her-2/neu测量。

结果

我们表明,在三种乳腺癌细胞系的单个细胞中,自发荧光与总Her-2/neu/FITC荧光之间存在部分相关性。我们还表明,基于比值的自发荧光校正结果与基于真正逐个细胞校正的结果一致。计算机模拟研究表明,在自发荧光成分与真正探针/染料荧光成分之间不存在相关性的样本中,比值校正能对平均真实荧光信号进行可靠估计,在人类实体瘤测量中常见的条件下,此类测量的变异系数会有相对较小但系统性的低估。

结论

基于平均自发荧光与平均总荧光比值的简单逐个细胞自发荧光校正方法,可应用于单个细胞中细胞自发荧光与真正探针/染料荧光之间存在相关性的细胞样本。在缺乏这种相关性或不知是否存在这种相关性的细胞样本中,使用这种校正时需注意测量的变异性程度会有系统性但相对较小的低估。

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