EPITOPE ANALYSIS OF HUMAN IL-6 RECEPTOR GP80 MOLECULE WITH MONOCLONAL-ANTIBODIES

被引:0
|
作者
LIAUTARD, J
GAILLARD, JP
MANI, JC
MONTEROJULIAN, F
DUPERRAY, C
LU, ZY
JOURDAN, M
KLEIN, B
BRAILLY, H
BROCHIER, J
机构
[1] INSERM,U291,F-34197 MONTPELLIER 05,FRANCE
[2] UFR PHARM,CNRS,UMR 9921,F-34060 MONTPELLIER 01,FRANCE
[3] IMMUNOTECH SA,F-13276 MARSEILLE 09,FRANCE
[4] INST GENET MOLEC,CNRS,F-34033 MONTPELLIER 01,FRANCE
关键词
HUMAN; IL-6; RECEPTOR; MONOCLONAL ANTIBODY; EPITOPE;
D O I
暂无
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Gp80 human IL-6R was studied using 7 murine mAb (M37, M91, M113, M139, M164, M182 and M195) obtained after fusion of splenocytes of Balb/c mice immunised with a mixture of recombinant IL-6 receptor (rIL-6R) and cells from 2 cell lines expressing IL-6R. These were U266, which is IL-6 independent and XG-1 which is IL-6-dependent. In ELISA the 7 mAb reacted against the rIL-6R and against the natural soluble form found in plasma (nIL-6R), which both lack transmembrane and cytoplasmic domains. However, M195 reacted less with the natural than with the recombinant soluble IL-6R. Using FACS analysis, the 7 mAb were shown to bind to U266 cells but not to the Namalva cell line which is deprived of IL-6R. This showed that they all recognised the membrane form of the IL-6R. Three of the anti-IL-6R mAb reacted with rIL-6R by Western blotting. Four different epitopes of the molecule were identified, either by cross-blocking experiments of mAb binding to IL6R in ELISA or by the biosensor Biacore technology. A group of 4 mAb (M37, M113, M139 and M164) and another mAb (M195) identified 2 different epitopes involved in IL-6 binding. These antibodies were able to inhibit the binding of IL-6 to IL-6R and the proliferation of the IL-6-dependent XG-1 cell line. M91 and M182 recognized 2 other epitopes that were not involved in IL-6 binding. As expected, M91 did not inhibit XG-1 proliferation; in contrast, M182 interfered with the proliferative response of the XG-1 cell line. This suggests that the epitope recognized by M182 is involved in the interaction between IL-6-gp80 complex and gp130 necessary for signal transmission. Using 2 mAb recognizing 2 different epitopes, we designed a sandwich ELISA to measure soluble IL-6R in biological fluids.
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收藏
页码:293 / 300
页数:8
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