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伴刀豆球蛋白A介导的胸腺细胞凝集:一种细胞黏附定量研究的模型。

Concanavalin-A-mediated thymocyte agglutination: a model for a quantitative study of cell adhesion.

作者信息

Capo C, Garrouste F, Benoliel A M, Bongrand P, Ryter A, Bell G I

出版信息

J Cell Sci. 1982 Aug;56:21-48. doi: 10.1242/jcs.56.1.21.

DOI:10.1242/jcs.56.1.21
PMID:7166565
Abstract

This report describes a quantitative study of the agglutination of rat thymocytes with concanavalin A (ConA). The probability that two ConA-coated cells remain bound after centrifugation was determined over a wide range of lectin concentrations. The minimal force required to separate agglutinated cells and the number of ConA molecules bound per cell were measured in similar experimental conditions. Agglutinated cells were examined by electron microscopy to estimate the area of membrane involved in adhesion. The dependence of agglutination on cell metabolism was studied: cold (4 degrees C), sodium azide (15 mM) and cytochalasin B (10 micrograms/ml) inhibited thymocyte adhesion. The importance of lateral movements of ConA molecules was assayed by measuring the adhesion of ConA-coated glutaraldehyde-fixed thymocytes to untreated cells: substantial binding occurred, but at a reduced level relative to untreated cells. A mathematical analysis of experimental data allowed the following conclusions. (1) At least 10(3) ConA bonds were involved in cross-linking two bound cells, which required the lectin molecules to be concentrated in the binding area, at least when low ConA concentrations (0.5 microgram/ml or less) were used. (2) The dependence of the binding probability on lectin concentration was fairly linear when the latter was small, which implied that the limiting step in cell-cell adhesion was the formation of a bond between a single ConA molecule and a ligand on the other cell. (3) The mean intercellular-contact time for the formation of this first bond was about 10 S for high concentrations of ligand (8 micrograms/ml). It was possible to fit the above data into a physically consistent quantitative model of cell adhesion.

摘要

本报告描述了用伴刀豆球蛋白A(ConA)对大鼠胸腺细胞凝集进行的定量研究。在广泛的凝集素浓度范围内,测定了两个ConA包被的细胞在离心后仍保持结合的概率。在类似的实验条件下,测量了分离凝集细胞所需的最小力以及每个细胞结合的ConA分子数量。通过电子显微镜检查凝集细胞,以估计参与黏附的膜面积。研究了凝集对细胞代谢的依赖性:低温(4℃)、叠氮化钠(15 mM)和细胞松弛素B(10微克/毫升)抑制胸腺细胞黏附。通过测量ConA包被的戊二醛固定胸腺细胞与未处理细胞的黏附来测定ConA分子侧向运动的重要性:发生了大量结合,但相对于未处理细胞,结合水平有所降低。对实验数据的数学分析得出了以下结论。(1)至少10³个ConA键参与了两个结合细胞的交联,这要求凝集素分子集中在结合区域,至少在使用低ConA浓度(0.5微克/毫升或更低)时如此。(2)当凝集素浓度较低时,结合概率对凝集素浓度的依赖性相当线性,这意味着细胞间黏附的限速步骤是单个ConA分子与另一个细胞上的配体形成键。(3)对于高浓度配体(8微克/毫升),形成第一个键的平均细胞间接触时间约为10秒。可以将上述数据拟合到一个物理上一致的细胞黏附定量模型中。

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