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Ure2p 纤维的淀粉样成核与分级组装。朊病毒结构域中天冬酰胺/谷氨酰胺重复序列和非重复区域的作用。

Amyloid nucleation and hierarchical assembly of Ure2p fibrils. Role of asparagine/glutamine repeat and nonrepeat regions of the prion domains.

作者信息

Jiang Yi, Li Hui, Zhu Li, Zhou Jun-Mei, Perrett Sarah

机构信息

National Laboratory of Biomacromolecules, Institute of Biophysics, Chinese Academy of Sciences, 15 Datun Road, Chaoyang District, Beijing 100101, China.

出版信息

J Biol Chem. 2004 Jan 30;279(5):3361-9. doi: 10.1074/jbc.M310494200. Epub 2003 Nov 10.

DOI:10.1074/jbc.M310494200
PMID:14610069
Abstract

The yeast prion protein Ure2 forms amyloid-like filaments in vivo and in vitro. This ability depends on the N-terminal prion domain, which contains Asn/Gln repeats, a motif thought to cause human disease by forming stable protein aggregates. The Asn/Gln region of the Ure2p prion domain extends to residue 89, but residues 15-42 represent an island of "normal" random sequence, which is highly conserved in related species and is relatively hydrophobic. We compare the time course of structural changes monitored by thioflavin T (ThT) binding fluorescence and atomic force microscopy for Ure2 and a series of prion domain mutants under a range of conditions. Atomic force microscopy height images at successive time points during a single growth experiment showed the sequential appearance of at least four fibril types that could be readily differentiated by height (5, 8, 12, or 9 nm), morphology (twisted or smooth), and/or time of appearance (early or late in the plateau phase of ThT binding). The Ure2 dimer (h = 2.6 +/- 0.5 nm) and granular particles corresponding to higher order oligomers (h = 4-12 nm) could also be detected. The mutants 15Ure2 and Delta 15-42Ure2 showed the same time-dependent variation in fibril types but with an increased lag time detected by ThT binding compared with wild-type Ure2. In addition, Delta 15-42Ure2 showed reduced binding to ThT. The results imply a role of the conserved region in both amyloid nucleation and formation of the binding surface recognized by ThT. Further, Ure2 amyloid formation is a multistep process via a series of fibrillar intermediates.

摘要

酵母朊病毒蛋白Ure2在体内和体外均能形成淀粉样细丝。这种能力取决于N端朊病毒结构域,该结构域包含Asn/Gln重复序列,这是一种被认为通过形成稳定的蛋白质聚集体而导致人类疾病的基序。Ure2p朊病毒结构域的Asn/Gln区域延伸至第89位残基,但第15 - 42位残基代表一个“正常”随机序列岛,在相关物种中高度保守且相对疏水。我们比较了在一系列条件下,通过硫黄素T(ThT)结合荧光和原子力显微镜监测的Ure2及一系列朊病毒结构域突变体结构变化的时间进程。在单个生长实验中连续时间点的原子力显微镜高度图像显示,至少有四种不同类型的纤维依次出现,这些纤维可以通过高度(5、8、12或9 nm)、形态(扭曲或光滑)和/或出现时间(ThT结合平台期的早期或晚期)轻易区分。还能检测到Ure2二聚体(h = 2.6 +/- 0.5 nm)和对应于高阶寡聚体的颗粒(h = 4 - 12 nm)。突变体15Ure2和Δ15 - 42Ure2在纤维类型上表现出相同的时间依赖性变化,但与野生型Ure2相比,通过ThT结合检测到的滞后时间增加。此外,Δ15 - 42Ure2与ThT的结合减少。结果表明保守区域在淀粉样成核和ThT识别的结合表面形成中均起作用。此外,Ure2淀粉样形成是一个通过一系列纤维状中间体的多步骤过程。

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