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免疫刺激复合物、基质或微胶粒在小鼠脾细胞中诱导细胞相关和分泌型白细胞介素-1的产生。

The induction of cell-associated and secreted IL-1 by iscoms, matrix or micelles in murine splenic cells.

作者信息

Villacres-Eriksson M, Bergström-Mollaoglu M, Kåberg H, Lövgren K, Morein B

机构信息

Swedish University of Agricultural Sciences, Department of Veterinary Microbiology, Uppsala.

出版信息

Clin Exp Immunol. 1993 Jul;93(1):120-5. doi: 10.1111/j.1365-2249.1993.tb06507.x.

Abstract

The kinetics of the expression of membrane-associated IL-1 (mIL-1) and soluble IL-1 (sIL-1) was studied in in vitro stimulated spleen cells from non-primed mice or from mice primed with influenza virus antigens incorporated in the immuno-stimulating complexes (iscoms) or as micelles. Matrix, which is the carrier structure for the antigens in the iscom, was used as a non-antigen stimulus. The IL-1 produced was assayed in an IL-1-dependent cell line and the specificity was demonstrated in a blocking experiment with antiserum to IL-1 alpha. Soluble IL-1 alpha was also quantified in ELISA. Iscoms and matrix induced production of mIL-1 and sIL-1 in cultures from non-treated mice as well as from mice primed 4 days before with iscoms or micelles. Micelles were a less strong stimulus and did not induce production of sIL-1. Micelles induced production of mIL-1 in cultures from non-primed mice or from mice which were recently immunized with micelles. No mIL-1 expression was induced by micelles if the spleen cells originated from mice immunized shortly before with iscoms. Depletion experiments demonstrated that sIL-1 was produced by adherent cells upon stimulation with iscoms or matrix. However, factor(s) from the non-adherent cells seem to be necessary for optimal secretion of sIL-1.

摘要

在体外刺激未致敏小鼠或用掺入免疫刺激复合物(iscoms)或作为胶束的流感病毒抗原致敏的小鼠的脾细胞中,研究了膜相关白细胞介素-1(mIL-1)和可溶性白细胞介素-1(sIL-1)的表达动力学。基质作为iscom中抗原的载体结构,用作非抗原刺激物。在依赖白细胞介素-1的细胞系中测定产生的白细胞介素-1,并在用抗白细胞介素-1α抗血清的阻断实验中证明其特异性。还通过酶联免疫吸附测定法(ELISA)对可溶性白细胞介素-1α进行定量。Iscoms和基质在未处理小鼠以及4天前用iscoms或胶束致敏的小鼠的培养物中诱导mIL-1和sIL-1的产生。胶束是较弱的刺激物,不诱导sIL-1的产生。胶束在未致敏小鼠或最近用胶束免疫的小鼠的培养物中诱导mIL-1的产生。如果脾细胞来自不久前用iscoms免疫的小鼠,则胶束不会诱导mIL-1表达。去除实验表明,sIL-1是由贴壁细胞在用iscoms或基质刺激后产生的。然而,非贴壁细胞中的因子似乎是sIL-1最佳分泌所必需的。

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本文引用的文献

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