一种亲脂性铝复合物乙酰丙酮铝显著刺激了Fe2+在磷脂脂质体中引发的脂质过氧化。

Biochimica et biophysica acta Pub Date : 1998-01-15
T Ohyashiki, S Suzuki, E Satoh, Y Uemori
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引用次数: 0

摘要

在本研究中,研究了亲脂性Al复合物乙酰丙酮铝在磷脂脂质体中作为Fe2+引发的脂质过氧化刺激剂的效果,并将结果与AlCl3处理的脂质体进行了比较。脂质过氧化程度通过硫代巴比妥酸反应物质(TBARS)的形成来评估。结果表明,在相同条件下,Al复合物对Fe2+引发的磷脂酰胆碱脂质体中脂质过氧化的刺激作用比AlCl3更有效。Al复合物对TBARS产生的浓度依赖性表明,诱导TBARS产生半最大刺激所需的复合物浓度为43微米。相比之下,直到AlCl3浓度增加到300微米以上,才观察到AlCl3的刺激作用。此外,我们发现不同浓度Al复合物PC脂质体脂质过氧化早期(加入Fe2+后2 min内)Fe2+残留量与TBARS值之间存在线性关系,表明Fe2+氧化过程与Al复合物的刺激作用密切相关。用Triton X-100处理Al复合物处理的脂质体后,Al复合物对脂质过氧化的刺激作用完全消失。使用12-(9-羟基硬脂酸)标记的脂质体进行荧光各向异性测量的结果表明,用Al复合物处理脂质体导致其脂质流动性降低。此外,还发现不同浓度Al配合物的脂质体中Fe2+氧化参数与荧光各向异性的程度存在相关性。从这些结果可以看出,Al复合物在脂质体膜中的掺入显著增强了Al对磷脂脂质体中Fe2+引发的脂质过氧化的作用,并且由于脂层中酰基链之间的填料加强而加速了Fe2+的氧化可能是Al复合物对Fe2+引发的脂质过氧化产生显著刺激作用的一个可能机制。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
A marked stimulation of Fe2+-initiated lipid peroxidation in phospholipid liposomes by a lipophilic aluminum complex, aluminum acetylacetonate.

In the present study, the efficacy of a lipophilic Al complex, aluminum acetylacetonate, as a stimulator of Fe2+-initiated lipid peroxidation in phospholipid liposomes was examined, and results were compared with those from the liposomes treated with AlCl3. The extent of lipid peroxidation was assessed by the formation of thiobarbituric acid-reactive substances (TBARS). The results indicated that the stimulatory effect of Al complex on Fe2+-initiated lipid peroxidation in phosphatidylcholine liposomes was more effective than that of AlCl3 under the same conditions. The concentration dependence of Al complex on TBARS production showed that the concentration of the complex required to induce half-maximal stimulation of TBARS production was 43 microM. In contrast, the stimulatory effect of AlCl3 was not observed until the AlCl3 concentration is increased above 300 microM. In addition, it was found that there is a linear relationship between the TBARS values and the residual amounts of Fe2+ at an earlier stage (within 2 min after the addition of Fe2+) of the lipid peroxidation in PC liposomes with different concentrations of Al complex, suggesting that Fe2+ oxidation process is closely related to the stimulatory effect of Al complex. The stimulatory effect of Al complex upon the lipid peroxidation completely disappeared by treatment of Al complex-treated liposomes with Triton X-100. The results of fluorescence anisotropy measurements using 12-(9-anthroyloxy)stearic acid-labeled liposomes suggested that treatment of the liposomes with Al complex caused a decrease in their lipid fluidity. Furthermore, it was found that there is a correlation between the extents of the fluorescence anisotropy and the Fe2+ oxidation parameters in the liposomes with different concentrations of Al complex. From these results, it is suggested that the Al effect on Fe2+-initiated lipid peroxidation in the phospholipid liposomes is markedly enhanced by incorporation of Al complex into the liposomal membranes and that an acceleration of Fe2+ oxidation due to a strengthened packing between the acyl chains in the lipid layer may be one possible mechanism for the occurrence of a marked stimulatory effect of Al complex on Fe2+ initiated lipid peroxidation.

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