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外文期刊>The biochemical journal
>Delayed oxidative degradation of polyunsaturated diacyl phospholipids in the presence of plasmalogen phospholipids in vitro
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Delayed oxidative degradation of polyunsaturated diacyl phospholipids in the presence of plasmalogen phospholipids in vitro
pThe oxidative degradation of plasmalogen (alkenylacyl) phospholipids was analysed in the absence and the presence of polyunsaturated ester phospholipids by sup1/supH-NMR and by chemical determination. Brain lysoplasmenylethanolamine (lyso-P-PE), brain P-PE and erythrocyte P-PE, containing an increasing number of intrachain double bonds at isn/isub2/sub, were oxidized with 2,2′-azobis-(2-amidinopropane hydrochloride) (AAPH; 2 or 10 mM) in Triton X-100 micelles (detergent/phospholipid 1:5, mol/mol). The formation of two peroxyl radicals was accompanied by the degradation of approx. one molecule of brain lyso-P-PE. On oxidation of brain P-PE or erythrocyte P-PE (320 nmol) with 2 mM AAPH, the (α-vinyl) methine sup1/supH signal of the enol ether decreased more rapidly than the methine proton peak of intrachain double bonds. The rate of enol ether degradation increased in the order: erythrocyte P-PE & brain P-PE & brain lyso-P-PE. The disappearance of the polyunsaturated ester phospholipids 1-palmitoyl-2-arachidonoyl phosphatidylcholine (16:0/20:4-PC) and 1-palmitoyl-2-linoleoyl phosphatidylcholine (16:0/18:2-PC) (100 nmol), as induced by 10 mM AAPH, was nearly completely inhibited by the plasmalogens (25 nmol) in the first 30 and 60 min of incubation respectively, and was delayed at later time points. Plasmalogens and vitamin E (4–25 nmol) mitigated the decreases in 16:0/[sup3/supH]20:4-PC (100 nmol) induced by 2 mM AAPH in a similar manner. The initial rate of degradation of intrachain double bonds of 16:0/20:4-PC and 16:0/18:2-PC (320 nmol; 2 mM AAPH) was decreased by 59% and 81% respectively in the presence of 80 nmol of brain lyso-P-PE. In conclusion, plasmalogens markedly delay the oxidative degradation of intrachain double bonds under iin vitro/i conditions. Interactions of enol ether double bonds with initiating peroxyl radicals as well as with products generated by prior oxidation of polyunsaturated fatty acids are proposed to be responsible for this capacity of plasmalogens. Furthermore, the products of enol ether oxidation apparently do not propagate the oxidation of polyunsaturated fatty acids./p
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机译:>通过 1 1 H-NMR和化学测定,分析在不存在和存在多不饱和酯磷脂的情况下缩醛磷脂(烯基酰基)磷脂的氧化降解。脑溶酶原乙醇胺(lyso-P-PE),脑P-PE和红细胞P-PE在 sn 2 处具有越来越多的链内双键,被2氧化。 Triton X-100胶束中的,2'-偶氮双(2-ami基丙烷盐酸盐)(AAPH; 2或10 mM)(洗涤剂/磷脂1:5,mol / mol)。两个过氧自由基的形成伴随着大约10%的降解。一分子的脑溶血素-P-PE。用2 mM AAPH氧化脑P-PE或红细胞P-PE(320 nmol)时,烯醇醚的(α-乙烯基)次甲基 1 H信号下降的速度比次甲基质子峰更快链内双键。烯醇醚的降解速率依次增加:红细胞P-PE> 1。脑P-PE脑溶血素-P-PE。多不饱和酯磷脂1-palmitoyl-2-arachidonoyl磷脂酰胆碱(16:0/20:4-PC)和1-palmitoyl-2-linoleoyl磷脂酰胆碱(16:0/18:2-PC)(100 nmol)的消失由10 mM AAPH诱导的,在孵育的前30分钟和60分钟分别被缩醛磷脂(25 nmol)几乎完全抑制,并在随后的时间点延迟。纤溶酶原和维生素E(4-25 nmol)以类似的方式缓解了2 mM AAPH诱导的16:0 / [ 3 H] 20:4-PC(100 nmol)的降低。在存在以下条件的情况下,16:0/20:4-PC和16:0/18:2-PC(320 nmol; 2 mM AAPH)的链内双键的初始降解速率分别降低了59%和81%。大脑溶血素-P-PE为80 nmol。总之,缩醛磷脂显着延迟了体外条件下链内双键的氧化降解。烯醇醚双键与引发的过氧自由基以及由多不饱和脂肪酸的预先氧化产生的产物的相互作用被认为是造成缩醛磷脂的这种能力的原因。此外,烯醇醚氧化产物显然不传播多不饱和脂肪酸的氧化。
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