Numerous debilitating human disorders result from protein misfolding and amyloid formation. Despite the grave nature of these maladies, our understanding of the structural mechanism of fibril assembly is limited. Of paramount importance is the need to identify and characterize oligomeric species formed early during fibril assembly, so that the nature of the initiating assembly mechanism can be revealed and species that may be toxic to cells identified. However, the transient nature of early oligomeric species, combined with their heterogeneity and instability, has precluded detailed analysis to date. Here, we have used electrospray ionisation mass spectrometry (ESI-MS), complemented by analytical ultracentrifugation (AUC) and measurements of thioflavin-T fluorescence, to monitor the early stages of assembly of amyloid-like fibrils formed from human beta-2-microglobulin (beta2m) in vitro. We show that worm-like fibrils that form with nucleation-independent kinetics assemble by a mechanism consistent with monomer addition, with species ranging from monomer to > or = 13-mer being identified directly and uniquely as transient assembly intermediates. By contrast, only monomers, dimers, trimers and tetramers are observed during nucleated growth, which leads to the formation of long straight fibrils. The results highlight the unique power of non-covalent ESI-MS to identify protein assembly intermediates in complex heterogeneous systems and demonstrate its great potential to identify and characterise individual species formed early during amyloid assembly.

译文

:许多使人衰弱的疾病源于蛋白质错误折叠和淀粉样蛋白形成。尽管这些疾病具有严重的性质,但是我们对原纤维组装的结构机理的理解是有限的。最重要的是需要鉴定和表征在原纤维组装过程中早期形成的寡聚物种,以便可以揭示起始组装机制的性质并鉴定可能对细胞有毒的物种。然而,迄今为止,早期寡聚物种的短暂性质,加上其异质性和不稳定性,已使详细分析无法进行。在这里,我们使用了电喷雾电离质谱(ESI-MS),并通过分析超速离心(AUC)和硫代黄素-T荧光的测量,来监测由人β-2-微球蛋白形成的淀粉样蛋白原纤维组装的早期阶段。 (beta2m)体外。我们显示,与成核无关的动力学形式形成的蠕虫状原纤维通过与单体加成一致的机制组装,从单体到>或= 13-mer的物质被直接和唯一地识别为瞬态组装中间体。相反,在成核生长期间仅观察到单体,二聚体,三聚体和四聚体,这导致长直原纤维的形成。结果突出了非共价ESI-MS识别复杂异质系统中蛋白质装配中间体的独特能力,并证明了其鉴定和表征淀粉样蛋白装配早期形成的单个物种的巨大潜力。

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