Incorporation and turnover of eicosapentaenoic and docosahexaenoic acids in human blood platelets in vitro

M Croset; M Lagarde; Y Bayon

摘要

pMass changes in the incorporation of linoleic (C18:2), eicosapentaenoic (C20:5) and docosahexaenoic (C22:6) acids in human blood platelet phospholipids were induced by incubating the cells and these fatty acids complexed to albumin. The remodelling of [14C]C18:2, [14C]C20:5 and [14C]C22:6 in classes, subclasses and molecular species of platelet phospholipids was studied in resting and thrombin-stimulated cells. More than 85% of the incorporation was located in phospholipids, representing 5-fold and 2.5-fold increases in the phospholipid C20:5 and C22:6 endogenous content respectively. Thrombin stimulation induced a 30% degradation of 1-acyl-2-C20:5-glycerophosphocholine (GPC) and 1-acyl-2-C22:6-GPC, but did not induce significant release of C18:2 from 1-acyl-2-C18:2-GPC. There was no change in the [14C]fatty acid composition of 1-alkyl-2-acyl-GPC. Thrombin-dependent increases in 1-alkenyl-2-C20:5-glycerophosphoethanolamine (GPE) and 1-alkenyl-2-C22:6-GPE of 2.1-fold and 2.5-fold respectively accounted for the rise in GPE radioactivity and partly compensated for the loss of these fatty acids from 1,2-diacyl-GPC: transfer to 1-alkenyl-2-acyl-GPE was 0.4 and 1.5 nmol/10(9) platelets for C20:5 and C22:6 respectively. [14C]C20:5 and [14C]C22:6 were incorporated into six different species of 1,2-diacyl-GPC, with acylation in the major endogenous forms (C18:1 +C16:0 and C18:0 species) representing 76% and 66% respectively of the total radioactivity present in 1,2-diacyl-GPC. Stimulation by thrombin induced significant release of these fatty acids from the main molecular species of 1,2-diacyl-GPC, but significantly stimulated the synthesis of alkenyl forms of GPE containing C18:1/C22:6 +C16:0/C22:6, C18:0/C22:6 and C18:0/C20:5. C18:0/C18:2, the major endogenous C18:2 molecular species, represented only 10.5% of the incorporation; none of the [14C]C18:2 molecular species was a substrate for transfer towards 1-alkenyl-2-acyl-GPE. It is concluded that when C20:5 and C22:6, but not C18:2, are acylated in 1,2-diacyl-GPC, they participate in thrombin-dependent phospholipid remodelling, and might compete with the turnover and release of arachidonic acid from platelet phospholipids and the subsequent activation of the cells./p

机译：通过孵育细胞并将这些脂肪酸复合到白蛋白上，诱导亚油酸（C18：2），二十碳五烯酸（C20：5）和二十二碳六烯酸（C22：6）酸在人血小板磷脂中掺入的质量变化。在静止和凝血酶刺激的细胞中研究了[14C] C18：2，[14C] C20：5和[14C] C22：6在血小板磷脂的类，亚类和分子种类中的重塑。超过85％的掺入位于磷脂中，分别代表磷脂C20：5和C22：6内源性含量增加了5倍和2.5倍。凝血酶刺激导致1-酰基-2-C20：5-甘油磷酸胆碱（GPC）和1-酰基-2-C22：6-GPC降解30％，但未诱导C18：2从1-酰基-β的显着释放。 2-C18：2-GPC。 1-烷基-2-酰基-GPC的[14C]脂肪酸组成没有变化。 1-链烯基-2-C20：5-甘油磷酸乙醇胺（GPE）和1-链烯基-2-C22：6-GPE的凝血酶依赖性增加分别为2.1倍和2.5倍，这解释了GPE放射性的增加并部分得到了补偿对于这些脂肪酸从1,2-二酰基-GPC的损失：对于C20：5和C22：6，转移到1-烯基-2-酰基-GPE的血小板分别为0.4和1.5 nmol / 10（9）血小板。将[14C] C20：5和[14C] C22：6掺入六种不同的1,2-二酰基GPC中，其中以主要内源形式（C18：1 + C16：0和C18：0物种）酰化1,2-二酰基-GPC中分别存在总放射性的76％和66％。凝血酶刺激导致这些脂肪酸从1,2-二酰基-GPC的主要分子物质中大量释放，但显着刺激了含有C18：1 / C22：6 + C16：0 / C22：6的GPE烯基形式的合成，C18：0 / C22：6和C18：0 / C20：5。 C18：0 / C18：2是主要的内源性C18：2分子种类，仅占掺入量的10.5％; [14C] C18：2分子种类均不是向1-烯基-2-酰基-GPE转移的底物。结论是，当C20：5和C22：6而不是C18：2在1,2-二酰基GPC中被酰化时，它们参与凝血酶依赖性磷脂重塑，并可能与花生四烯酸的更新和释放竞争从血小板磷脂中提取并随后激活细胞。

Incorporation and turnover of eicosapentaenoic and docosahexaenoic acids in human blood platelets in vitro

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