Epitope mapping and functional studies with three monoclonal antibodies to the C‐KIT receptor tyrosine kinase, YB5.B8, 17F11, and SR‐1

表位 内化 单克隆抗体 分子生物学 受体酪氨酸激酶 生物 酪氨酸激酶 细胞培养 表位定位 抗体 化学 细胞生物学 受体 生物化学 免疫学 遗传学
作者
Leonie K. Ashman,Hans‐Jörg Bühring,Gabriella W. Aylett,Virginia C. Broudy,Claudia Müller
出处
期刊:Journal of Cellular Physiology [Wiley]
卷期号:158 (3): 545-554 被引量:29
标识
DOI:10.1002/jcp.1041580321
摘要

Abstract Three monoclonal antibodies (MAbs) to the human c‐kit receptor tyrosine kinase (P145 c‐kit ), derived in independent laboratories, have been extensively used in studies of c‐kit expression and the role of its ligand, steel factor (SLF), in hemopoiesis and mast cell differentiation and function. In this study, the relationship between the epitopes they identify, and their effects on SLF binding, receptor internalization, and signal transduction are compared. Epitope mapping studies carried out on the high P145 c‐kit ‐expressing cell line HEL‐DR showed that SR‐1 identifies an epitope independent of those bound by YB5.B8 and 17F11, while the latter two antibodies bound to distinct but interacting epitopes. SR‐1 potently blocked the binding of SLF to P145 c‐kit on these cells and also on cells of the factor‐dependent line MO7e. In contrast, YB5.B8 and 17F11 had minimal effects on ligand binding. Conversely, SLF partially blocked the binding of SR‐1 and YB5.B8 to cells, while binding of 17F11 was actually enhanced by SLF on some target cells. Preincubation of HEL‐DR and MO7e cells with MAbs prior to exposure to SLF revealed that 17F11 itself brought about partial down‐regulation of P145 c‐kit and did not inhibit SLF‐mediated down‐regulation. SR‐1 caused minimal down‐regulation and inhibited SLF‐mediated receptor internalization. YB5.B8 had minimal effects on either cell line in this assay. To determine whether the antibodies had any agonist activity, they were compared with SLF for their ability to bring about receptor phosphorylation in intact MO7e cells. All three antibodies induced detectable tyrosine phosphorylation with 17F11 being the most effective, while YB5.B8 was the least effective. Finally, the ability of the antibodies to influence the proliferation of the MO7e cells was examined. As expected, SR‐1 potently inhibited the proliferative response to SLF, while 17F11 weakly inhibited and YB5.B8 had negligible effect. In the absence of SLF both 17F11 and YB5.B8 displayed very weak but reproducible agonist activity. © 1994 Wiley‐Liss, Inc.
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