Luscinskas F W, Nicolaou K C, Webber S E, Veale C A, Gimbrone M A, Serhan C N
Department of Medicine, Brigham and Women's Hospital, Boston, MA 02115.
Biochem Pharmacol. 1990 Jan 15;39(2):355-65. doi: 10.1016/0006-2952(90)90035-j.
The biosynthesis of leukotrienes and lipoxins involves epoxide-containing intermediates which may be subject to several routes of transcellular metabolism. We have examined the capacity of leukotriene A4 (LTA4) and 15S-hydroxy-5,6-oxido-7,9,13-trans-11-cis-eicosatetraenoic acid [5(6)-epoxytetraene] to stimulate the mobilization of free cytosolic calcium [( Ca2+]i) in human blood neutrophils. To gain insight into structure-activity relationships, a putative intermediate in lipoxin biosynthesis, 5S-hydroxy-14,15-oxido-6,10,12-trans-8-cis-eicosatetraenoic acid [14(15)-epoxytetraene], was prepared by total synthesis. When added to fura-2 loaded neutrophils, each of these compounds provoked a rapid and transient increase in [Ca2+]i (maximum by 8 sec) which returned to baseline within 60-90 sec. Ca2+ mobilization with LTA4 was dose dependent and, at 1 microM, the efficacies of LTA4 and LTB4 were quantitatively similar. The 5(6)-epoxytetraene and 14(15)-epoxytetraene were less potent than LTA4. Prior exposure of the cells to ethyleneglycolbis(aminoethylether)tetra-acetate (EGTA) (60 sec, 3 mM) did not diminish either the amplitude or the extent of [Ca2+]i elicited by LTA4. Methyl esters of LTA4 and 5(6)-epoxytetraene were less potent than their corresponding free acids, whereas the free acid of 14(15)-epoxytetraene and its methyl ester were quantitatively similar. Results from alcohol trapping studies showed that these epoxides were intact during the initial phase of Ca2+i mobilization (t0-10 sec) stimulated by LTA4, 5(6)-epoxytetraene, and 14(15)-epoxytetraene. In addition, the individual mixtures of products formed upon aqueous hydrolysis of each of the epoxides did not stimulate changes in [Ca2+]i. In each case, the products formed were identified by physical methods including reverse phase high pressure liquid chromatography, ultraviolet spectroscopy and gas liquid chromatography-mass spectrometry. These results indicate that, when added to human neutrophils, LTA4, 5(6)-epoxytetraene and 14(15)-epoxytetraene each stimulate a rapid mobilization of [Ca2+]i. Moreover, they suggest that intermediates in the biosynthesis of leukotrienes and lipoxins possess intrinsic activities that may serve to amplify cellular responses within their cell of origin or act on adjacent cells during their transcellular metabolism.
白三烯和脂氧素的生物合成涉及含环氧化物的中间体,这些中间体可能会经历几种跨细胞代谢途径。我们研究了白三烯A4(LTA4)和15S-羟基-5,6-环氧-7,9,13-反式-11-顺式-二十碳四烯酸[5(6)-环氧四烯]刺激人血中性粒细胞中游离胞质钙([Ca2+]i)动员的能力。为了深入了解结构-活性关系,通过全合成制备了脂氧素生物合成中的一个假定中间体,5S-羟基-14,15-环氧-6,10,12-反式-8-顺式-二十碳四烯酸[14(15)-环氧四烯]。当添加到用fura-2负载的中性粒细胞中时,这些化合物中的每一种都会引起[Ca2+]i的快速和短暂增加(8秒时达到最大值),并在60-90秒内恢复到基线水平。LTA4引起的Ca2+动员呈剂量依赖性,在1 microM时,LTA4和LTB4的效力在数量上相似。[5(6)-环氧四烯和14(15)-环氧四烯的效力低于LTA4。细胞预先暴露于乙二醇双(氨基乙基醚)四乙酸(EGTA)(60秒,3 mM)不会降低LTA4引起的[Ca2+]i的幅度或程度。LTA4和[5(6)-环氧四烯的甲酯效力低于其相应的游离酸,而14(15)-环氧四烯的游离酸及其甲酯在数量上相似。醇捕获研究的结果表明,在LTA4、[5(6)-环氧四烯和14(15)-环氧四烯刺激的Ca2+i动员的初始阶段(t0-10秒),这些环氧化物是完整的。此外,每种环氧化物在水水解后形成的产物的单独混合物不会刺激[Ca2+]i的变化。在每种情况下,通过包括反相高压液相色谱、紫外光谱和气-液色谱-质谱在内的物理方法鉴定形成的产物。这些结果表明,当添加到人中性粒细胞中时,LTA4、[5(6)-环氧四烯和14(15)-环氧四烯各自刺激[Ca2+]i的快速动员。此外,它们表明白三烯和脂氧素生物合成中的中间体具有内在活性,这些活性可能有助于在其起源细胞内放大细胞反应,或在其跨细胞代谢过程中作用于相邻细胞。
