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荧光伴刀豆球蛋白A与淋巴细胞结合的Scatchard分析

Scatchard analysis of fluorescent concanavalin A binding to lymphocytes.

作者信息

Gordon I L

机构信息

Department of Surgery, University of California Irvine, USA.

出版信息

Cytometry. 1995 Jul 1;20(3):238-44. doi: 10.1002/cyto.990200307.

Abstract

Standard Scatchard analysis of ligand binding to cell receptors requires the use of isotopes and is imprecise at low ligand concentrations. To evaluate the feasibility of Scatchard analysis via fluorescence flow cytometry, the binding of fluorescein isothiocyanate-derivatized concanavalin A (FITC-ConA) to murine lymphocytes at 4 degrees C was compared to 125I-ConA binding. A FACS IV flow cytometer (Becton-Dickinson, Mountain View, CA) was used for analysis of cells after fluorescent ligand binding. A simple spectrophotometric technique was used to calibrate the relation between cytometer-determined fluorescence and ligand binding per cell. As FITC-ConA binding showed a quasi-Gaussian distribution, the mean number of molecules bound per cell was easily calculated. Scatchard analysis of FITC-ConA binding yielded results (1.9 x 10(6) receptors/cell, K = 3.6 x 10(-15)) similar to those obtained with 125I-ConA (1.4 x 10(6) receptors/cell, K = 5.2 x 10(-15)). Cytometric Scatchard plots showed less scatter and seemed more precise, suggesting superiority to radioactive ligand measurements, particularly at low ligand concentrations.

摘要

配体与细胞受体结合的标准Scatchard分析需要使用同位素,并且在低配体浓度下不准确。为了评估通过荧光流式细胞术进行Scatchard分析的可行性,将异硫氰酸荧光素衍生的伴刀豆球蛋白A(FITC-ConA)在4℃下与小鼠淋巴细胞的结合与125I-ConA结合进行了比较。使用FACS IV流式细胞仪(Becton-Dickinson,加利福尼亚州山景城)分析荧光配体结合后的细胞。使用一种简单的分光光度技术来校准细胞仪测定的荧光与每个细胞的配体结合之间的关系。由于FITC-ConA结合呈现准高斯分布,因此很容易计算出每个细胞结合的分子平均数。FITC-ConA结合的Scatchard分析得出的结果(1.9×10^6个受体/细胞,K = 3.6×10^-15)与用125I-ConA获得的结果(1.4×10^6个受体/细胞,K = 5.2×10^-15)相似。细胞测量的Scatchard图显示出较少的散点,似乎更精确,表明优于放射性配体测量,特别是在低配体浓度下。

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