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单克隆抗体与液相中的蛋白质抗原或与固相支持物结合的蛋白质抗原的结合。

Binding of monoclonal antibody to protein antigen in fluid phase or bound to solid supports.

作者信息

Kennel S J

出版信息

J Immunol Methods. 1982 Nov 26;55(1):1-12. doi: 10.1016/0022-1759(82)90070-9.

DOI:10.1016/0022-1759(82)90070-9
PMID:7153517
Abstract

Rat monoclonal antibody (MoAb) to fragment D (FgD) of human fibrinogen was used to characterize the direct binding of antibody to protein in solution or bound to solid supports. Purified IgG, F(ab')2 and Fab' were prepared from ascites fluid of hybridoma 104-14B which is a fusion product of spleen cells from a rat immunized with FgD and the mouse myeloma cell line, P3-X63-Ag8. Two-dimensional electrophoresis of radioiodinated antibody preparations demonstrated the presence of hybrid immunoglobulin molecules, but only structures having rat heavy and rat light chains had active antibody combining sites. The affinity constant for IgG as well as F(ab')2 and Fab', 6 X 10(9) M-1, was identical when tested using fluid phase antigen (125I-labeled FgD). Affinity constants determined for direct binding of iodinated IgG using FgD immobilized on solid supports showed a slight dependence on the antigen concentration used in the measurement. These values ranged from 0.5 X 10(9) M-1 at high antigen concentrations (1.3 X 10(-7) M) to 9 X 10(9) M-1 at low antigen concentration (1.3 X 10(-10) M). Binding constants for F(ab')2 and Fab' gave similar results indicating that binding was homogeneous and univalent. The capacity of solid state antigen to bind antibody varied with the method used to bind FgD to the solid support. FgD bound directly to polystyrene plates was least efficient at binding labeled antibody; FgD bound to plates through intermediate carriers poly(L-lysine) was only slightly more efficient, while antigen bound to Sepharose beads by cyanogen bromide activation was the most active.

摘要

用人纤维蛋白原D片段(FgD)的大鼠单克隆抗体(MoAb)来表征抗体与溶液中或结合于固相载体上的蛋白质的直接结合。从杂交瘤104-14B的腹水制备纯化的IgG、F(ab')2和Fab',该杂交瘤是用FgD免疫的大鼠脾细胞与小鼠骨髓瘤细胞系P3-X63-Ag8的融合产物。放射性碘化抗体制剂的二维电泳显示存在杂合免疫球蛋白分子,但只有具有大鼠重链和大鼠轻链的结构具有活性抗体结合位点。当使用液相抗原(125I标记的FgD)进行测试时,IgG以及F(ab')2和Fab'的亲和常数均为6×10(9) M-1。使用固定在固相载体上的FgD测定碘化IgG直接结合的亲和常数显示,其对测量中使用的抗原浓度略有依赖性。这些值在高抗原浓度(1.3×10(-7) M)时为0.5×10(9) M-1,在低抗原浓度(1.3×10(-10) M)时为9×10(9) M-1。F(ab')2和Fab'的结合常数给出了类似的结果,表明结合是均匀且单价的。固态抗原结合抗体的能力因将FgD结合到固相载体上的方法而异。直接结合到聚苯乙烯板上的FgD结合标记抗体的效率最低;通过中间载体聚(L-赖氨酸)结合到板上的FgD效率仅略高,而通过溴化氰活化结合到琼脂糖珠上的抗原活性最高。

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