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首页> 美国卫生研究院文献>The Journal of Biological Chemistry >Endothelial Surface N-Glycans Mediate Monocyte Adhesion and Are Targets for Anti-inflammatory Effects of Peroxisome Proliferator-activated Receptor γ Ligands
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Endothelial Surface N-Glycans Mediate Monocyte Adhesion and Are Targets for Anti-inflammatory Effects of Peroxisome Proliferator-activated Receptor γ Ligands

机译:内皮表面N-聚糖介导单核细胞粘附是过氧化物酶体增殖物激活受体γ配体抗炎作用的目标。

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Endothelial-monocyte interactions are regulated by adhesion molecules and key in the development of vascular inflammatory disease. Peroxisome proliferator-activated receptor (PPAR) γ activation in endothelial cells is recognized to mediate anti-inflammatory effects that inhibit monocyte rolling and adhesion. Herein, evidence is provided for a novel mechanism for the anti-inflammatory effects of PPARγ ligand action that involves inhibition of proinflammatory cytokine-dependent up-regulation of endothelial N-glycans. TNFα treatment of human umbilical vein endothelial cells increased surface expression of high mannose/hybrid N-glycans. A role for these sugars in mediating THP-1 or primary human monocyte rolling and adhesion was indicated by competition studies in which addition of α-methylmannose, but not α-methylglucose, inhibited monocyte rolling and adhesion during flow, but not under static conditions. This result supports the notion that adhesion molecules provide scaffolds for sugar epitopes to mediate adhesion with cognate receptors. A panel of structurally distinct PPARγ agonists all decreased TNFα-dependent expression of endothelial high mannose/hybrid N-glycans. Using rosiglitazone as a model PPARγ agonist, which decreased TNFα-induced high mannose N-glycan expression, we demonstrate a role for these carbohydrate residues in THP-1 rolling and adhesion that is independent of endothelial surface adhesion molecule expression (ICAM-1 and E-selectin). Data from N-glycan processing gene arrays identified α-mannosidases (MAN1A2 and MAN1C1) as targets for down-regulation by TNFα, which was reversed by rosiglitazone, a result consistent with altered high mannose/hybrid N-glycan epitopes. Taken together we propose a novel anti-inflammatory mechanism of endothelial PPARγ activation that involves targeting protein post-translational modification of adhesion molecules, specifically N-glycosylation.
机译:内皮-单核细胞的相互作用受粘附分子的调节,是血管炎性疾病发展的关键。内皮细胞中的过氧化物酶体增殖物激活受体(PPAR)γ激活被认为可介导抑制单核细胞滚动和粘附的抗炎作用。在本文中,提供了关于PPARγ配体作用的抗炎作用的新机制的证据,该机制涉及抑制促炎细胞因子依赖性内皮N-聚糖的上调。 TNFα处理人脐静脉内皮细胞可增加高甘露糖/杂交N-聚糖的表面表达。这些竞争性研究表明了这些糖在介导THP-1或人类原代单核细胞滚动和粘附中的作用,其中加入α-甲基甘露糖而不是α-甲基葡萄糖抑制了流动过程中单核细胞的滚动和粘附,但在静态条件下却没有。该结果支持以下观点:粘附分子为糖表位提供支架以介导与同源受体的粘附。一组结构上不同的PPARγ激动剂均降低了内皮高甘露糖/杂合N-聚糖的TNFα依赖性表达。使用罗格列酮作为模型PPARγ激动剂,可降低TNFα诱导的高甘露糖N-聚糖表达,我们证明了这些碳水化合物残基在THP-1滚动和粘附中的作用独立于内皮表面粘附分子的表达(ICAM-1和E -selectin)。来自N-聚糖加工基因阵列的数据确定α-甘露糖苷酶(MAN1A2和MAN1C1)为TNFα下调的靶标,罗格列酮逆转了这一结果,这一结果与高甘露糖/杂合N-聚糖表位的改变一致。总之,我们提出了内皮PPARγ激活的新型抗炎机制,该机制涉及靶向粘附分子的蛋白质翻译后修饰,特别是N-糖基化。

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