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低密度脂蛋白亚组分的氧化易感性与其泛醇-10和α-生育酚含量有关。

Oxidative susceptibility of low density lipoprotein subfractions is related to their ubiquinol-10 and alpha-tocopherol content.

作者信息

Tribble D L, van den Berg J J, Motchnik P A, Ames B N, Lewis D M, Chait A, Krauss R M

机构信息

Department of Molecular and Nuclear Medicine, Lawrence Berkeley Laboratory, University of California, Berkeley 94720.

出版信息

Proc Natl Acad Sci U S A. 1994 Feb 1;91(3):1183-7. doi: 10.1073/pnas.91.3.1183.

Abstract

The conjugated polyene fatty acid parinaric acid (PnA) undergoes a stoichiometric loss in fluorescence upon oxidation and can be used to directly monitor peroxidative stress within lipid environments. We evaluated the course of potentially atherogenic oxidative changes in low density lipoproteins (LDL) by monitoring the oxidation of PnA following its incorporation into buoyant (p = 1.026-1.032 g/ml) and dense (p = 1.040-1.054 g/ml) LDL subfractions. Copper-induced oxidation of LDL-associated PnA exhibited an initial lag phase followed by an increased rate of loss until depletion. Increased PnA oxidation occurred immediately after the antioxidants ubiquinol-10 and alpha-tocopherol were consumed but before there were marked elevations in conjugated dienes. Despite differences in sensitivity to early oxidation events, PnA oxidation and conjugated diene lag times were correlated (r = 0.582; P = 0.03), and both indicated a greater susceptibility of dense than buoyant LDL in accordance with previous reports. The greater susceptibility of PnA in dense LDL was attributed to reduced levels of ubiquinol-10 and alpha-tocopherol, which were approximately 50% lower than in buoyant LDL (mol of antioxidant/mol of LDL) and together accounted for 80% of the variation in PnA oxidation lag times. These results suggest that PnA is a useful probe of LDL oxidative susceptibility and may be superior to conjugated dienes for monitoring the initial stages of LDL lipid peroxidation. Differences in oxidative susceptibility among LDL density subfractions are detected by the PnA assay and are due in large part to differences in their antioxidant content.

摘要

共轭多烯脂肪酸紫黄质酸(PnA)在氧化时会发生荧光化学计量损失,可用于直接监测脂质环境中的过氧化应激。我们通过监测PnA掺入漂浮(p = 1.026 - 1.032 g/ml)和致密(p = 1.040 - 1.054 g/ml)低密度脂蛋白(LDL)亚组分后的氧化情况,评估了低密度脂蛋白(LDL)中潜在致动脉粥样硬化氧化变化的过程。铜诱导的与LDL相关的PnA氧化呈现出初始延迟期,随后损失速率增加直至耗尽。抗氧化剂泛醇-10和α-生育酚消耗后,PnA氧化立即增加,但共轭二烯显著升高之前。尽管对早期氧化事件的敏感性存在差异,但PnA氧化和共轭二烯延迟时间相关(r = 0.582;P = 0.03),并且两者均表明致密LDL比漂浮LDL更易氧化,这与先前报道一致。致密LDL中PnA更易氧化归因于泛醇-10和α-生育酚水平降低,其比漂浮LDL低约50%(抗氧化剂摩尔数/LDL摩尔数),共同占PnA氧化延迟时间变化的80%。这些结果表明,PnA是LDL氧化敏感性的有用探针,在监测LDL脂质过氧化初始阶段可能优于共轭二烯。通过PnA测定可检测到LDL密度亚组分之间氧化敏感性的差异,这在很大程度上归因于它们抗氧化剂含量的差异。

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