首页> 美国卫生研究院文献>The Journal of Experimental Medicine >Leukotriene production in human neutrophils primed by recombinant human granulocyte/macrophage colony-stimulating factor and stimulated with the complement component C5A and FMLP as second signals
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Leukotriene production in human neutrophils primed by recombinant human granulocyte/macrophage colony-stimulating factor and stimulated with the complement component C5A and FMLP as second signals

机译:重组人粒细胞/巨噬细胞集落刺激因子启动并以补体成分C5A和FMLP作为第二信号刺激的人类嗜中性白细胞白三烯生产

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摘要

Neutrophils (PMN) preincubated with recombinant human granulocyte/macrophage colony-stimulating factor (rhGM-CSF) for 2 h and then stimulated with the chemotactic factors, C5a or FMLP, produce substantial amounts of the lipoxygenase products 5-Hete, LTB4, and omega-oxidised LTB4 metabolites (4.36 +/- 0.95 (SEM) pM (n = 21) LTB4 and LTB4 metabolites/10(6) PMN). No lipoxygenase metabolites are detected by HPLC and RIA if purified PMN are stimulated by either GM- CSF or chemotactic factors in the absence of exogenous arachidonate. The priming effect of GM-CSF upon chemotactic factor induced generation of lipid mediators is a relatively slow process, clearly evident after 1 h and optimal after 2 h. Leukotriene generation is measurable with 0.8 U GM-CSF/10(6) PMN and is maximal with 80 U (10(-11)-10(-9) M). Upon activation of primed PMN with chemotactic factors, leukotriene synthesis is induced very rapidly. Already 2.5 min after activation the major lipoxygenase metabolites present are 20-OH LTB4 and 20-COOH LTB4. Our study shows that the synthesis of lipoxygenase metabolites from endogeneous AA can be initiated in PMN through receptor mediated processes by the appropriately timed combination of biological soluble inflammatory mediator peptides. Furthermore, these results indicate that GM-CSF not only enhances effector cell functions but can qualitatively change the mediator profile formed after activation with a second triggering signal. Such a mechanism might be important in amplifying inflammatory responses. Alternatively, lipid mediators formed might also have an intracellular or autocoid role and be responsible for the enhancement of other PMN functions like oxygen radical release.
机译:中性粒细胞(PMN)与重组人粒细胞/巨噬细胞集落刺激因子(rhGM-CSF)预孵育2 h,然后用趋化因子C5a或FMLP刺激,产生大量的脂氧合酶产物5-Hete,LTB4和omega -氧化的LTB4代谢产物(4.36 +/- 0.95(SEM)pM(n = 21)LTB4和LTB4代谢产物/ 10(6)PMN)。如果在不存在外源花生四烯酸酯的情况下,GM-CSF或趋化因子刺激了纯化的PMN,则HPLC和RIA均未检测到脂氧合酶代谢物。 GM-CSF对趋化因子诱导的脂质介体生成的引发作用是一个相对缓慢的过程,在1 h后清晰可见,在2 h后达到最佳。用0.8 U GM-CSF / 10(6)PMN可以测量白三烯的生成,最大80 U(10(-11)-10(-9)M)可以测量。在用化学趋化因子激活引发的PMN时,白三烯合成很快被诱导。活化后约2.5分钟,主要的脂氧合酶代谢产物为20-OH LTB4和20-COOH LTB4。我们的研究表明,内源性AA合成脂氧合酶代谢物可以通过适当地定时组合生物可溶性炎症介质肽,通过受体介导的过程在PMN中启动。此外,这些结果表明,GM-CSF不仅增强了效应细胞的功能,而且可以定性地改变在用第二触发信号激活后形成的介体分布。这种机制在放大炎症反应中可能很重要。或者,形成的脂质介体也可能具有细胞内或自体体的作用,并负责增强其他PMN功能(如氧自由基的释放)。

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