Rostagno Agueda, Neubert Thomas A, Ghiso Jorge
Department of Pathology, New York University School of Medicine, New York, NY, USA.
Department of Biochemistry and Molecular Pharmacology, New York University School of Medicine, New York, NY, USA.
Methods Mol Biol. 2018;1779:23-43. doi: 10.1007/978-1-4939-7816-8_3.
Amyloid β (Aβ) is the major constituent of the brain deposits found in parenchymal plaques and cerebral blood vessels of patients with Alzheimer's disease (AD). Besides classic full-length peptides, biochemical analyses of brain deposits have revealed high degree of Aβ heterogeneity likely resulting from the action of multiple proteolytic enzymes. This chapter describes a sequential extraction protocol allowing the differential fractionation of soluble and deposited Aβ species taking advantage of their differential solubility properties. Soluble Aβ is extracted by water-based buffers like phosphate-buffered saline-PBS-whereas pre-fibrillar and fibrillar deposits, usually poorly soluble in PBS, are extractable in detergent containing solutions or more stringent conditions as formic acid. The extraction procedure is followed by the biochemical identification of the extracted Aβ species using Western blot and a targeted proteomic analysis which combines immunoprecipitation with MALDI-ToF mass spectrometry. This approach revealed the presence of numerous C- and N-terminal truncated Aβ species in addition to Aβ1-40/42. Notably, the more soluble C-terminal cleaved fragments constitute a main part of PBS homogenates. On the contrary, N-terminal truncated species typically require more stringent conditions for the extraction in agreement with their lower solubility and enhanced aggregability. Detailed assessment of the molecular diversity of Aβ species composing interstitial fluid and amyloid deposits at different disease stages, as well as the evaluation of the truncation profile during various pharmacologic approaches will provide a comprehensive understanding of the still undefined contribution of Aβ truncations to AD pathogenesis and their potential as novel therapeutic targets.
淀粉样β蛋白(Aβ)是在阿尔茨海默病(AD)患者脑实质斑块和脑血管中发现的脑沉积物的主要成分。除了经典的全长肽外,对脑沉积物的生化分析显示,Aβ具有高度的异质性,这可能是多种蛋白水解酶作用的结果。本章描述了一种顺序提取方案,利用可溶性和沉积性Aβ物种的不同溶解性,对其进行差异分级分离。可溶性Aβ用基于水的缓冲液(如磷酸盐缓冲盐水 - PBS)提取,而预纤维状和纤维状沉积物通常在PBS中溶解性较差,可在含洗涤剂的溶液或更严格的条件(如甲酸)下提取。提取过程之后,使用蛋白质印迹法和将免疫沉淀与基质辅助激光解吸电离飞行时间质谱联用的靶向蛋白质组学分析对提取的Aβ物种进行生化鉴定。该方法揭示了除Aβ1-40/42之外还存在大量C端和N端截短的Aβ物种。值得注意的是,溶解性更强的C端裂解片段构成了PBS匀浆的主要部分。相反,N端截短的物种通常需要更严格的提取条件,这与其较低的溶解性和增强的聚集性一致。详细评估不同疾病阶段构成间质液和淀粉样沉积物的Aβ物种的分子多样性,以及评估各种药理方法中的截短情况,将全面了解Aβ截短对AD发病机制尚未明确的贡献及其作为新型治疗靶点的潜力。