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通过从经脂多糖预处理的人外周血单核细胞中释放⁵¹Cr来测定抗体和补体依赖性细胞损伤。

Antibody- and complement-dependent cell injury assayed by 51Cr release from human peripheral blood mononuclear cells pretreated with lipopolysaccharide.

作者信息

Repo H, Leirisalo-Repo M, Nurminen M, Mäkelä P H

出版信息

Infect Immun. 1987 Mar;55(3):507-12. doi: 10.1128/iai.55.3.507-512.1987.

Abstract

Exposure of human peripheral blood mononuclear (MN) cells to deesterified (alkali-treated) lipopolysaccharide (LPS-OH) and then to 51Cr rendered the cells susceptible to 51Cr release in the presence of specific antibody and complement. The assay was optimized by using rough (Rb2 or Re) LPS. 51Cr release did not occur from cells preexposed to untreated or electrodialyzed LPS. Studies of isolated monocytes and lymphocytes revealed that the majority of the 51Cr released was derived from monocytes. The optimum concentration of LPS-OH was 10 micrograms/ml. Antiyersinia agglutinin-positive serum, but not a negative serum, obtained from patients with reactive yersinia arthritis caused 51Cr release from MN cells pretreated with yersinia LPS-OH. This implies that during yersinia infection antibodies are generated that can attack the cell membrane--LPS-OH complex. We conclude that the method provides a tool to demonstrate binding of LPS to MN cells in a manner that leads to cell injury in an immune host.

摘要

将人外周血单个核(MN)细胞暴露于脱酯(碱处理)脂多糖(LPS-OH),然后再暴露于51Cr,可使细胞在特异性抗体和补体存在的情况下易于发生51Cr释放。通过使用粗糙型(Rb2或Re)LPS对该检测方法进行了优化。预先暴露于未处理或经电渗析的LPS的细胞未发生51Cr释放。对分离的单核细胞和淋巴细胞的研究表明,释放的51Cr大部分来源于单核细胞。LPS-OH的最佳浓度为10微克/毫升。从反应性耶尔森菌关节炎患者获得的抗耶尔森菌凝集素阳性血清(而非阴性血清)可导致经耶尔森菌LPS-OH预处理的MN细胞发生51Cr释放。这意味着在耶尔森菌感染期间会产生能够攻击细胞膜-LPS-OH复合物的抗体。我们得出结论,该方法提供了一种工具,可证明LPS以导致免疫宿主细胞损伤的方式与MN细胞结合。

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