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利用内在荧光探测淀粉样β蛋白组装体的构象动力学

Conformational dynamics of amyloid beta-protein assembly probed using intrinsic fluorescence.

作者信息

Maji Samir K, Amsden Jason J, Rothschild Kenneth J, Condron Margaret M, Teplow David B

机构信息

Department of Neurology, David Geffen School of Medicine at UCLA, Los Angeles, California 90095, USA.

出版信息

Biochemistry. 2005 Oct 11;44(40):13365-76. doi: 10.1021/bi0508284.

DOI:10.1021/bi0508284
PMID:16201761
Abstract

Formation of toxic oligomeric and fibrillar structures by the amyloid beta-protein (Abeta) is linked to Alzheimer's disease (AD). To facilitate the targeting and design of assembly inhibitors, intrinsic fluorescence was used to probe assembly-dependent changes in Abeta conformation. To do so, Tyr was substituted in Abeta40 or Abeta42 at position 1, 10 (wild type), 20, 30, 40, or 42. Fluorescence then was monitored periodically during peptide monomer folding and assembly. Electron microscopy revealed that all peptides assembled readily into amyloid fibrils. Conformational differences between Abeta40 and Abeta42 were observed in the central hydrophobic cluster (CHC) region, Leu17-Ala21. Tyr20 was partially quenched in unassembled Abeta40 but displayed a significant and rapid increase in intensity coincident with the maturation of an oligomeric, alpha-helix-containing intermediate into amyloid fibrils. This process was not observed during Abeta42 assembly, during which small decreases in fluorescence intensity were observed in the CHC. These data suggest that the structure of the CHC in Abeta42 is relatively constant within unassembled peptide and during the self-association process. Solvent accessibility of the Tyr ring was studied using a mixed solvent (dimethyl sulfoxide/water) system. [Tyr40]Abeta40, [Tyr30]Abeta42, and [Tyr42]Abeta42 all were relatively shielded from solvent. Analysis of the assembly dependence of the site-specific intrinsic fluorescence data suggests that the CHC is particularly important in controlling Abeta40 assembly, whereas the C-terminus plays the more significant role in Abeta42 assembly.

摘要

淀粉样β蛋白(Aβ)形成有毒的寡聚体和纤维状结构与阿尔茨海默病(AD)相关。为了便于靶向和设计组装抑制剂,利用内在荧光来探测Aβ构象中与组装相关的变化。为此,在Aβ40或Aβ42的第1、10位(野生型)、20、30、40或42位替换酪氨酸(Tyr)。然后在肽单体折叠和组装过程中定期监测荧光。电子显微镜显示所有肽都能很容易地组装成淀粉样纤维。在中央疏水簇(CHC)区域Leu17 - Ala21观察到Aβ40和Aβ42之间的构象差异。在未组装的Aβ40中Tyr20部分猝灭,但随着含α螺旋的寡聚中间体成熟为淀粉样纤维,其强度显著且迅速增加。在Aβ42组装过程中未观察到这一过程,在此期间CHC中荧光强度有小幅下降。这些数据表明Aβ42中CHC的结构在未组装肽内和自组装过程中相对恒定。使用混合溶剂(二甲亚砜/水)系统研究了Tyr环的溶剂可及性。[Tyr40]Aβ40、[Tyr30]Aβ42和[Tyr42]Aβ42都相对被溶剂屏蔽。对位点特异性内在荧光数据的组装依赖性分析表明,CHC在控制Aβ40组装中特别重要,而C末端在Aβ42组装中起更重要的作用。

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