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单细胞上的荧光共振能量转移。应用于单价半抗原与细胞结合免疫球蛋白E的结合研究。

Fluorescence resonance energy transfer on single living cells. Application to binding of monovalent haptens to cell-bound immunoglobulin E.

作者信息

Kubitscheck U, Kircheis M, Schweitzer-Stenner R, Dreybrodt W, Jovin T M, Pecht I

机构信息

Institute for Experimental Physics, University of Bremen, Germany.

出版信息

Biophys J. 1991 Aug;60(2):307-18. doi: 10.1016/S0006-3495(91)82055-0.

Abstract

We have determined the specific binding of 2,4-dinitrophenyl (DNP)-haptens to two different monoclonal immunoglobulin (IgE) molecules bound to Fc epsilon-receptors on the cell surface of single, living rat basophilic leukemia cells subclone 2H3 cells. The measurements were performed at 4 degrees, 15 degrees, and 25 degrees C using a recently developed technique that permits the quantitative determination of fluorescence resonance energy transfer between two fluorophores on single cells in a microscope from the photobleaching kinetics of the donor fluorophore. We introduce here a method for performing binding studies on individual attached cells. At 25 degrees C, the titration studies yielded equilibrium binding constants Kint of 9 x 10(8), 8 x 10(8), and 8 x 10(7) M-1 for the monovalent haptens N-2,4-DNP-epsilon-amino-n-caproic acid, N epsilon-2,4-DNP-L-lysine, and N-2,4-DNP-gamma-amino-n-butyric acid, respectively. Our data indicate that the affinity constants for the first two haptens binding to IgE on adherent cells are 4 to 11 times larger than that of the corresponding values obtained by fluorescence quenching experiments with the same haptens and IgE molecules either in solution or bound to cells in suspension.

摘要

我们已经确定了2,4 - 二硝基苯基(DNP)半抗原与两种不同的单克隆免疫球蛋白(IgE)分子的特异性结合,这两种IgE分子结合在单个活大鼠嗜碱性白血病细胞亚克隆2H3细胞表面的Fcε受体上。测量是在4℃、15℃和25℃下进行的,使用了一种最近开发的技术,该技术可以根据供体荧光团的光漂白动力学,从显微镜下单个细胞上的两个荧光团之间定量测定荧光共振能量转移。我们在此介绍一种对单个贴壁细胞进行结合研究的方法。在25℃下,滴定研究得出单价半抗原N - 2,4 - DNP - ε - 氨基 - n - 己酸、Nε - 2,4 - DNP - L - 赖氨酸和N - 2,4 - DNP - γ - 氨基 - n - 丁酸的平衡结合常数Kint分别为9×10⁸、8×10⁸和8×10⁷ M⁻¹。我们的数据表明,前两种半抗原与贴壁细胞上IgE结合的亲和常数比用相同半抗原和IgE分子在溶液中或悬浮细胞中进行荧光猝灭实验得到的相应值大4至11倍。

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