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Distribution of type I Fc epsilon-receptors on the surface of mast cells probed by fluorescence resonance energy transfer.

机译:通过荧光共振能量转移探测的肥大细胞表面I型Fcε受体的分布。

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摘要

The aggregation state of type I Fc epsilon-receptors (Fc epsilon RI) on the surface of single living mast cells was investigated by resonance fluorescence energy transfer. Derivatization of Fc epsilon RI specific ligands, i.e., immunoglobulin E or Fab fragments of a Fc epsilon RI specific monoclonal antibody, with donor and acceptor fluorophores provided a means for measuring receptor clustering through energy transfer between the receptor probes. The efficiency of energy transfer between the ligands carrying distinct fluorophores was determined on single cells in a microscope by analyzing the photobleaching kinetics of the donor fluorophore in the presence and absence of receptor ligands labeled with acceptor fluorophores. To rationalize the energy transfer data, we developed a theoretical model describing the dependence of the energy transfer efficiency on the geometry of the fluorescently labeled macromolecular ligands and their aggregation state on the cell surface. To this end, the transfer process was numerically calculated first for one pair and then for an ensemble of Fc epsilon RI bound ligands on the cell surface. The model stipulates that the aggregation state of the Fc epsilon RI is governed by an attractive lipid-protein mediated interaction potential. The corresponding pair-distribution function characterizes the spatial distribution of the ensemble. Using this approach, the energy transfer efficiency of the ensemble was calculated for different degrees of receptor aggregation. Comparison of the theoretical modeling results with the experimental energy transfer data clearly suggests that the Fc epsilon RI are monovalent, randomly distributed plasma membrane proteins. The method provides a novel approach for determining the aggregation state of cell surface components.
机译:通过共振荧光能量转移研究了单个活肥大细胞表面上的I型Fcε-受体(FcεRI)的聚集状态。 FcεRI特异性配体即FcεRI特异性单克隆抗体的免疫球蛋白E或Fab片段的衍生化,具有供体和受体荧光团,提供了一种通过受体探针之间的能量转移来测量受体簇的方法。通过在存在和不存在被受体荧光团标记的受体配体的情况下分析供体荧光团的光漂白动力学,在显微镜中的单个细胞上确定了携带不同荧光团的配体之间能量转移的效率。为了合理化能量转移数据,我们开发了一个理论模型,描述了能量转移效率对荧光标记的高分子配体的几何形状及其在细胞表面的聚集状态的依赖性。为此,首先在数值上计算一对的转移过程,然后在细胞表面上对FcεRI结合的配体进行整体计算。该模型规定FcεRI的聚集状态由有吸引力的脂质-蛋白介导的相互作用势控制。相应的对分布函数表征集合的空间分布。使用这种方法,针对不同程度的受体聚集计算了集合的能量转移效率。理论建模结果与实验能量转移数据的比较清楚地表明,FcεRI是单价,随机分布的质膜蛋白。该方法提供了确定细胞表面组分聚集状态的新颖方法。

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