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肺泡巨噬细胞衍生的中性粒细胞趋化活性的释放需要补体成分C5。

Complement component C5 is required for release of alveolar macrophage-derived neutrophil chemotactic activity.

作者信息

Robbins R A, Russ W D, Thomas K R, Rasmussen J K, Kay H D

出版信息

Am Rev Respir Dis. 1987 Mar;135(3):659-64. doi: 10.1164/arrd.1987.135.3.659.

Abstract

The influx of neutrophils into the alveolar structures can be induced by stimulation of the resident lung phagocyte, the alveolar macrophage, to release a potent neutrophil chemoattractant(s). We hypothesized that the fifth component of complement (C5) on the cell surface may be required for activation of the alveolar macrophage to release neutrophil chemotactic activity. C5 was identified on guinea pig alveolar macrophages by epifluorescent microscopy, flow cytometry, and enzyme-linked immunoabsorbent assay of eluted macrophages. When cultured for 4 h with stimuli that induce the release of chemotactic activity or for 24 h without added stimuli, purified Fab' fragments of a goat anti-C5 antibody significantly inhibited the ability of macrophages to release chemotactic activity as determined by a blindwell chamber method (p less than 0.001, all comparisons). This inhibition of chemotactic activity was not detected when anti-C5 antibody was added after the culture period. In contrast, anti-C3 antibody had no inhibitory effect at 4 h or at 24 h (p greater than 0.2, all comparisons). Partial characterization of released chemotactic activity revealed it was of low molecular weight, partially lipid soluble, and not inhibited by C5a chemotactic factor inactivator. These studies suggest that C5 may have a regulatory role in the release of chemotactic activity by alveolar macrophages.

摘要

通过刺激肺部常驻吞噬细胞——肺泡巨噬细胞释放一种有效的中性粒细胞趋化因子,可诱导中性粒细胞流入肺泡结构。我们推测,细胞表面的补体第五成分(C5)可能是激活肺泡巨噬细胞以释放中性粒细胞趋化活性所必需的。通过落射荧光显微镜、流式细胞术以及对洗脱巨噬细胞进行酶联免疫吸附测定,在豚鼠肺泡巨噬细胞上鉴定出了C5。当用诱导趋化活性释放的刺激物培养4小时或在不添加刺激物的情况下培养24小时时,山羊抗C5抗体的纯化Fab'片段显著抑制了巨噬细胞释放趋化活性的能力,这是通过盲孔室法测定的(所有比较中p均小于0.001)。在培养期后添加抗C5抗体时,未检测到对趋化活性的这种抑制作用。相比之下,抗C3抗体在4小时或24小时时均无抑制作用(所有比较中p均大于0.2)。对释放的趋化活性的部分特性分析表明,其分子量低,部分脂溶性,且不受C5a趋化因子灭活剂的抑制。这些研究表明,C5可能在肺泡巨噬细胞释放趋化活性方面具有调节作用。

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