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由含GM1的筏样膜介导的β-淀粉样蛋白聚集抑制剂。

Inhibitors of amyloid beta-protein aggregation mediated by GM1-containing raft-like membranes.

作者信息

Matsuzaki Katsumi, Noguch Taeko, Wakabayashi Masaki, Ikeda Keisuke, Okada Takuma, Ohashi Yumiko, Hoshino Masaru, Naiki Hironobu

机构信息

Graduate School of Pharmaceutical Sciences, Kyoto University, Sakyo-ku, Kyoto 606-8501, Japan.

出版信息

Biochim Biophys Acta. 2007 Jan;1768(1):122-30. doi: 10.1016/j.bbamem.2006.09.014. Epub 2006 Sep 23.

DOI:10.1016/j.bbamem.2006.09.014
PMID:17069749
Abstract

The aggregation (fibril formation) of amyloid beta-protein (Abeta) is considered to be a crucial step in the etiology of Alzheimer's disease (AD). The inhibition of Abeta aggregation and/or decomposition of fibrils formed in aqueous solution by small compounds have been studied extensively for the prevention and treatment of AD. However, recent studies suggest that Abeta aggregation also occurs in lipid rafts mediated by a cluster of monosialoganglioside GM1. This study examined the effects of representative compounds on Abeta aggregation and fibril destabilization in the presence of GM1-containing raft-like liposomes. Among the compounds tested, nordihydroguaiaretic acid (NDGA), rifampicin (RIF), tannic acid (TA), and quercetin (QUE) showed strong fibrillization inhibitory activity. NDGA and RIF inhibited the binding of Abeta to GM1 liposomes by competitively binding to the membranes and/or direct interaction with Abeta in solution, thus at least partly preventing fibrils from forming. Coincubation of Abeta with NDGA, RIF, and QUE in the presence of GM1 liposomes resulted in elongate particles, whereas the presence of TA yielded protofibrillar structures. TA and RIF also destabilized fibrils. The most potent NDGA prevented Abeta-induced toxicity in PC12 cells by inhibiting Abeta accumulation. Furthermore, a comparison of the inhibitory effects of various compounds between aqueous-phase and GM1-mediated aggregation of Abeta suggested that the two aggregation processes are not identical.

摘要

β-淀粉样蛋白(Aβ)的聚集(原纤维形成)被认为是阿尔茨海默病(AD)病因学中的关键步骤。小分子化合物对Aβ聚集的抑制和/或对水溶液中形成的原纤维的分解作用已被广泛研究用于AD的预防和治疗。然而,最近的研究表明,Aβ聚集也发生在由单唾液酸神经节苷脂GM1簇介导的脂筏中。本研究检测了代表性化合物在含GM1的筏样脂质体存在下对Aβ聚集和原纤维去稳定化的影响。在所测试的化合物中,去甲二氢愈创木酸(NDGA)、利福平(RIF)、单宁酸(TA)和槲皮素(QUE)表现出很强的原纤维化抑制活性。NDGA和RIF通过竞争性结合膜和/或与溶液中的Aβ直接相互作用,抑制Aβ与GM1脂质体的结合,从而至少部分地阻止原纤维形成。在GM1脂质体存在下,将Aβ与NDGA、RIF和QUE共同孵育会产生细长颗粒,而TA的存在则产生原纤维状结构。TA和RIF也会使原纤维去稳定化。最有效的NDGA通过抑制Aβ积累来预防Aβ诱导的PC12细胞毒性。此外,比较各种化合物在水相和GM1介导的Aβ聚集之间的抑制作用表明,这两种聚集过程并不相同。

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