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脂多糖对人单核细胞系补体(C3)合成的刺激作用。

LPS stimulation of complement (C3) synthesis by a human monocyte cell line.

作者信息

Nichols W K

出版信息

Complement. 1984;1(2):108-15. doi: 10.1159/000467823.

DOI:10.1159/000467823
PMID:6599386
Abstract

The human monocyte-like cell line, U937, was utilized as a model system to assess the influence of lipopolysaccharides (LPS) from Escherichia coli and other immunomodulatory agents on the biosynthesis of complement component C3 by monocytoid cells. The amount of C3 accumulated in the medium of cultured cells was measured by an enzyme-linked immunoabsorbent assay (ELISA). In the presence of LPS (0.01 and 0.10 microgram/ml) C3 production by U937 cells was increased by 2- and 5-fold, respectively. C3 production was also increased in the presence of lymphokine-containing supernatants obtained from human peripheral blood mononuclear cells after their stimulation with concanavalin A-sepharose. Human gamma-interferon (50-500 units/ml) stimulated C3 production by U937 cells. Stimulation of C3 production by LPS or mononuclear cell supernatants was blocked by cycloheximide. LPS (0.10 and 1.0 microgram/ml) also stimulated PGE2 production by U937 cells but failed to increase PGE2 at the lowest concentration (0.01 micrograms/ml) shown to increase C3 biosynthesis. Although exogenous PGE1 (10(-7) and 10(-6) M) promoted a small increase in C3 production, the effect of LPS was not decreased by a concentration of indomethacin (10(-6) M) that inhibited biosynthesis of PGE2. Therefore, LPS-induced C3 synthesis is not mediated by an increase in PGE2 in U937 cells. In summary, these observations suggest that C3 biosynthesis by monocytes/macrophages can be modulated by mediators of cellular immune responses found in the microenvironment of a localized inflammatory reaction.

摘要

人类单核细胞样细胞系U937被用作模型系统,以评估大肠杆菌来源的脂多糖(LPS)和其他免疫调节因子对单核细胞样细胞补体成分C3生物合成的影响。通过酶联免疫吸附测定(ELISA)测量培养细胞培养基中积累的C3量。在LPS(0.01和0.10微克/毫升)存在下,U937细胞的C3产量分别增加了2倍和5倍。在用伴刀豆球蛋白A-琼脂糖刺激后,从人外周血单核细胞获得的含淋巴因子的上清液存在时,C3产量也增加。人γ干扰素(50 - 500单位/毫升)刺激U937细胞产生C3。LPS或单核细胞上清液对C3产生的刺激被环己酰亚胺阻断。LPS(0.10和1.0微克/毫升)也刺激U937细胞产生PGE2,但在显示可增加C3生物合成的最低浓度(0.01微克/毫升)时未能增加PGE2。尽管外源性PGE1(10^(-7)和10^(-6) M)促进C3产量略有增加,但抑制PGE2生物合成的吲哚美辛浓度(10^(-6) M)并未降低LPS的作用。因此,LPS诱导的C3合成不是由U937细胞中PGE2的增加介导的。总之,这些观察结果表明,单核细胞/巨噬细胞的C3生物合成可被局部炎症反应微环境中发现的细胞免疫反应介质调节。

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