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触珠蛋白与载脂蛋白A-I结合可防止羟自由基对其卵磷脂胆固醇酰基转移酶刺激活性的损害。

Haptoglobin binding to apolipoprotein A-I prevents damage from hydroxyl radicals on its stimulatory activity of the enzyme lecithin-cholesterol acyl-transferase.

作者信息

Salvatore Alfonso, Cigliano Luisa, Bucci Enrico M, Corpillo Davide, Velasco Silvia, Carlucci Alessandro, Pedone Carlo, Abrescia Paolo

机构信息

Dipartimento delle Scienze Biologiche, Università di Napoli Federico II, via Mezzocannone 8, 80134 Napoli, Italy.

出版信息

Biochemistry. 2007 Oct 2;46(39):11158-68. doi: 10.1021/bi7006349. Epub 2007 Sep 7.

DOI:10.1021/bi7006349
PMID:17824618
Abstract

Apolipoprotein A-I (ApoA-I), a major component of HDL, binds haptoglobin, a plasma protein transporting to liver or macrophages free Hb for preventing hydroxyl radical production. This work aimed to assess whether haptoglobin protects ApoA-I against this radical. Human ApoA-I structure, as analyzed by electrophoresis and MS, was found severely altered by hydroxyl radicals in vitro. Lower alteration of ApoA-I was found when HDL was oxidized in the presence of haptoglobin. ApoA-I oxidation was limited also when the complex of haptoglobin with both high-density lipoprotein and Hb, immobilized on resin beads, was exposed to hydroxyl radicals. ApoA-I function to stimulate cholesterol esterification was assayed in vitro by using ApoA-I-containing liposomes. Decreased stimulation was observed when liposomes oxidized without haptoglobin were used. Conversely, after oxidative stress in the presence of haptoglobin (0.5 microM monomer), the liposome activity did not change. Plasma of carrageenan-treated mice was analyzed by ELISA for the levels of haptoglobin and ApoA-I, and used to isolate HDL for MS analysis. Hydroxyproline-containing fragments of ApoA-I were found associated with low levels of haptoglobin (18 microM monomer), whereas they were not detected when the haptoglobin level increased (34-70 microM monomer). Therefore haptoglobin, when circulating at enhanced levels with free Hb during the acute phase of inflammation, might protect ApoA-I structure and function against hydroxyl radicals.

摘要

载脂蛋白A-I(ApoA-I)是高密度脂蛋白(HDL)的主要成分,它与触珠蛋白结合,触珠蛋白是一种将游离血红蛋白转运至肝脏或巨噬细胞的血浆蛋白,可防止羟自由基的产生。这项研究旨在评估触珠蛋白是否能保护ApoA-I免受这种自由基的损伤。通过电泳和质谱分析发现,体外羟自由基会严重改变人ApoA-I的结构。当在触珠蛋白存在的情况下氧化HDL时,发现ApoA-I的改变较小。当固定在树脂珠上的触珠蛋白与高密度脂蛋白和血红蛋白的复合物暴露于羟自由基时,ApoA-I的氧化也受到限制。通过使用含ApoA-I的脂质体在体外测定ApoA-I刺激胆固醇酯化的功能。当使用在没有触珠蛋白的情况下氧化的脂质体时,观察到刺激作用降低。相反,在触珠蛋白(0.5微摩尔单体)存在的情况下进行氧化应激后,脂质体活性没有变化。通过酶联免疫吸附测定(ELISA)分析角叉菜胶处理小鼠的血浆中触珠蛋白和ApoA-I的水平,并用于分离HDL进行质谱分析。发现含羟脯氨酸的ApoA-I片段与低水平的触珠蛋白(18微摩尔单体)有关,而当触珠蛋白水平升高(34 - 70微摩尔单体)时未检测到这些片段。因此,在炎症急性期,当触珠蛋白与游离血红蛋白一起以升高的水平循环时,可能会保护ApoA-I的结构和功能免受羟自由基的损伤。

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