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免疫调节剂的筛选:异源生物体外对巨噬细胞化学发光的影响

Screening for immunomodulators: effects of xenobiotics on macrophage chemiluminescence in vitro.

作者信息

Tam P E, Hinsdill R D

机构信息

Department of Bacteriology, University of Wisconsin, Madison 53706.

出版信息

Fundam Appl Toxicol. 1990 Apr;14(3):542-53. doi: 10.1016/0272-0590(90)90258-l.

Abstract

Macrophage chemiluminescence (CL) was evaluated as a primary screening assay by assessing the modulatory activity of 17 different chemicals. The chemicals were either known immunomodulatory drugs or environmental toxicants with reported immunomodulatory activity. Elicited mouse peritoneal macrophages were exposed to the chemicals in vitro, and CL was measured in response to an opsonized yeast stimulus. Ten chemicals (hydrocortisone, dextran sulfate, di-n-octyltin dichloride, dimethyltin dichloride, azathioprine, lambda carrageenan (l-carrageenan), lead, N-propyl gallate, gallic acid, and indomethacin) were identified as effective modulators of CL. The polyanions dextran sulfate and l-carrageenan either suppressed or enhanced CL, depending on the experimental conditions, while the remaining modulators were inhibitory. A series of secondary assays was used to verify this modulatory activity and to explore different mechanisms of action. Each effective modulator altered only a few specific components of the more complex CL response, and the following general mechanisms were apparent. At least 2 chemicals showed distinct antioxidant activity and thus probably did not alter functional aspects of macrophage CL. Chemicals which blocked Fc receptor function delayed the peak CL of macrophages stimulated by opsonized yeast. Nine of the 10 modulators inhibited hydrogen peroxide release, but only 3 inhibited the release of superoxide. Finally, some effective modulators were chemicals known to interact with cell membranes or specific membrane receptors, and these were able to directly induce a CL response without the addition of opsonized yeast as a stimulus. Thus, macrophage CL was a simple, quantitative, yet sensitive immunotoxicologic screening assay capable of identifying many known immunomodulatory drugs. Supplementary assays were useful both in confirming the functional effects of these chemicals on CL and in delineating potential mechanisms by which modulation of CL can occur.

摘要

通过评估17种不同化学物质的调节活性,将巨噬细胞化学发光(CL)作为一种初步筛选测定方法。这些化学物质要么是已知的免疫调节药物,要么是具有报道的免疫调节活性的环境毒物。将诱导的小鼠腹腔巨噬细胞在体外暴露于这些化学物质,并测量对调理酵母刺激的CL反应。十种化学物质(氢化可的松、硫酸葡聚糖、二正辛基二氯化锡、二甲基二氯化锡、硫唑嘌呤、λ-角叉菜胶(l-角叉菜胶)、铅、没食子酸丙酯、没食子酸和吲哚美辛)被确定为CL的有效调节剂。多阴离子硫酸葡聚糖和l-角叉菜胶根据实验条件要么抑制要么增强CL,而其余调节剂具有抑制作用。使用一系列二级测定来验证这种调节活性并探索不同的作用机制。每种有效调节剂仅改变更复杂的CL反应的一些特定成分,以下一般机制很明显。至少有2种化学物质表现出明显的抗氧化活性,因此可能不会改变巨噬细胞CL的功能方面。阻断Fc受体功能的化学物质延迟了调理酵母刺激的巨噬细胞的CL峰值。10种调节剂中有9种抑制过氧化氢释放,但只有3种抑制超氧化物释放。最后,一些有效调节剂是已知与细胞膜或特定膜受体相互作用的化学物质,并且这些物质能够在不添加调理酵母作为刺激的情况下直接诱导CL反应。因此,巨噬细胞CL是一种简单、定量且敏感的免疫毒理学筛选测定方法,能够识别许多已知的免疫调节药物。补充测定对于确认这些化学物质对CL的功能影响以及描绘CL调节可能发生的潜在机制都很有用。

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