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荧光染料标记对抗体亲和力和染料光物理性质的影响。

The Effect of Fluorophore Conjugation on Antibody Affinity and the Photophysical Properties of Dyes.

机构信息

Department of Biophysics and Cell Biology, Faculty of Medicine, University of Debrecen, Debrecen, Hungary; MTA-DE Cell Biology and Signaling Research Group, Faculty of Medicine, University of Debrecen, Debrecen, Hungary.

Department of Biophysics and Cell Biology, Faculty of Medicine, University of Debrecen, Debrecen, Hungary.

出版信息

Biophys J. 2018 Feb 6;114(3):688-700. doi: 10.1016/j.bpj.2017.12.011.

Abstract

Because the degree of labeling (DOL) of cell-bound antibodies, often required in quantitative fluorescence measurements, is largely unknown, we investigated the effect of labeling with two different fluorophores (AlexaFluor546, AlexaFluor647) in a systematic way using antibody stock solutions with different DOLs. Here, we show that the mean DOL of the cell-bound antibody fraction is lower than that of the stock using single molecule fluorescence measurements. The effect is so pronounced that the mean DOL levels off at approximately two fluorophores/IgG for some antibodies. We developed a method for comparing the average DOL of antibody stocks to that of the isolated, cell-bound fraction based on fluorescence anisotropy measurements confirming the aforementioned conclusions. We created a model in which individual antibody species with different DOLs, present in an antibody stock solution, were assumed to have distinct affinities and quantum yields. The model calculations confirmed that a calibration curve constructed from the anisotropy of antibody stocks can be used for determining the DOL of the bound fraction. The fluorescence intensity of the cell-bound antibody fractions and of the antibody stocks exhibited distinctly different dependence on the DOL. The behavior of the two dyes was systematically different in this respect. Fitting of the model to these data revealed that labeling with each dye affects quantum yield and antibody affinity differentially. These measurements also implied that fluorophores in multiply labeled antibodies exhibit self-quenching and lead to decreased antibody affinity, conclusions directly confirmed by steady-state intensity measurements and competitive binding assays. Although the fluorescence lifetime of antibodies labeled with multiple fluorophores decreased, the magnitude of this change was not sufficient to account for self-quenching indicating that both dynamic and static quenching processes occur involving H-aggregate formation. Our results reveal multiple effects of fluorophore conjugation, which must not be overlooked in quantitative cell biological measurements.

摘要

由于细胞结合抗体的标记程度(DOL)在定量荧光测量中通常是未知的,我们使用具有不同 DOL 的抗体储备溶液系统地研究了用两种不同荧光染料(AlexaFluor546、AlexaFluor647)标记的影响。在这里,我们通过使用单分子荧光测量显示出细胞结合抗体部分的平均 DOL 低于储备溶液中的 DOL。这种影响非常明显,以至于对于某些抗体,平均 DOL 水平在大约两个荧光染料/IgG 时趋于平稳。我们开发了一种基于荧光各向异性测量的方法,用于将抗体储备的平均 DOL 与分离的细胞结合部分进行比较,从而证实了上述结论。我们创建了一个模型,其中假定抗体储备溶液中存在不同 DOL 的单个抗体种类具有不同的亲和力和量子产率。模型计算证实,从各向异性构建的抗体储备校准曲线可用于确定结合部分的 DOL。细胞结合抗体部分和抗体储备的荧光强度表现出明显不同的 DOL 依赖性。两种染料在这方面的行为在系统上有所不同。将模型拟合到这些数据表明,用每种染料标记都会以不同的方式影响量子产率和抗体亲和力。这些测量还暗示,多标记抗体中的荧光染料会发生自猝灭,导致抗体亲和力降低,这一结论直接通过稳态强度测量和竞争结合测定得到证实。尽管用多个荧光染料标记的抗体的荧光寿命降低,但这种变化的幅度不足以说明自猝灭,表明涉及 H-聚集体形成的动态和静态猝灭过程都会发生。我们的结果揭示了荧光染料偶联的多种影响,在定量细胞生物学测量中不能忽视这些影响。

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