人白细胞介素-1 β单克隆抗体及其在敏感的双位点酶联免疫吸附试验中的应用。

Lymphokine research Pub Date : 1989-01-01
S Fontaine, C Damais, D Lando, M A Cousin
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引用次数: 0

摘要

制备了5种针对人重组白细胞介素-1 β (il -1 β,氨基酸117-269)的单克隆抗体(mab),编码分别为#111、122、206、209和609。其中四种单克隆抗体(#111、122、206和609)已被鉴定能够抑制重组和天然白介素-1 β的生物活性。竞争研究表明,分子的三个不重叠的表位被单克隆抗体识别。MAbs #609和206是基于高亲和力而选择的,并一起用于双位点ELISA检测IL-1 β。ELISA的灵敏度为1 pg/孔(10 ~ 20 pg/ml)。该试验未检测到rHuIL-1 α、rHuIL-2、rhuifn - α、rHuIL-6和天然a-和b-FGF。然后将免疫测定法与当前的测定法进行比较,例如对小鼠胸腺细胞的共丝分裂效应,以检测ifn - γ和/或lps刺激的人血液单核细胞的细胞内和细胞外区室中的IL-1 β。我们证实ifn - γ在LPS的作用下增强了IL-1 β的分泌(即使是高剂量1微克/毫升),而不是细胞内IL-1 β的前体。该免疫测定法也可用于检测血浆、血清和滑液中的IL-1 β。
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Monoclonal antibodies to human interleukin-1 beta and their use in a sensitive two-site enzyme linked immunosorbent assay.

Five Monoclonal Antibodies (MAbs) coded respectively #111, 122, 206, 209 and 609 were produced against human recombinant Interleukin-1 beta (rIL-1 beta, amino acids 117-269). Four of these MAbs (#111, 122, 206 and 609) have been identified able to inhibit the biological activity of recombinant and natural Interleukin-1 beta. Competition studies suggested that three non-overlapping epitopes of the molecule were recognized by the MAbs. MAbs #609 and 206 have been selected on the basis of high affinity and used together in a two-site ELISA to detect IL-1 beta. The sensitivity of this ELISA was 1 pg/well (10-20 pg/ml). The assay did not detect rHuIL-1 alpha, rHuIL-2, rHuTNF-alpha, rHuIFN-gamma, rHuIL-6, and natural a- and b-FGF. The immunoassay was then compared to current assay such as co-mitogenic effect on murine thymocytes for detection of IL-1 beta in the intra- and extracellular compartments of IFN-gamma and/or LPS-stimulated human blood monocytes. We confirm that IFN-gamma potentiates IL-1 beta secretion in response to LPS (even with high dose 1 microgram/ml) but not the intracellular precursor of IL-1 beta. This immunoassay could be used also to detect IL-1 beta in plasma, sera and synovial fluids.

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