Lys63连锁泛素抗体表位的质谱切除和提取方法鉴定。

IF 1.1 4区 化学 Q4 PHYSICS, ATOMIC, MOLECULAR & CHEMICAL
European Journal of Mass Spectrometry Pub Date : 2023-10-01 Epub Date: 2023-09-19 DOI:10.1177/14690667231199012
Ji Eun Jung, Vanessa Cárdenas, Brîndușa Alina Petre
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引用次数: 0

摘要

泛素是真核细胞中的一种保守蛋白,以单体或多泛素链形式存在,称为异肽连接聚合物。这些链通过泛素中赖氨酸的α-氨基与随后泛素单元c端甘氨酸之间的共价键连接到底物或其他泛素分子上。泛素中特定赖氨酸残基形成泛素-泛素链的选择决定了其生化和生物学功能。需要对各自的多泛素链进行详细的化学结构-功能评估。有趣的是,在严重的人类疾病状态中,特异的赖氨酸连锁多泛素链与许多病理包涵体共价结合,这些包涵体似乎对正常降解具有抗性,因此多泛素链与泛素抗体之间的相互作用是非常有用的。例如,阿尔茨海默病的神经原纤维缠结和帕金森氏病的路易小体是严重泛素化的,可以使用特异性泛素抗体很容易地观察到。本研究利用合成的泛素构建块肽,包含与Gly-Gly二肽连接的各种赖氨酸残基(K6, K11, K33, K48和K63),目的是探索lys63 -多泛素抗体的识别特异性。通过亲和质谱(Affinity-MS)和免疫印迹技术,研究了不同泛素构建块与特异性Lys63-ubiquitin (K63-Ub)抗体之间的相互作用,从而能够以前所未有的选择性从生物材料中直接鉴定蛋白质。亲和质谱和斑点杂交数据证实了K63-Ub抗体与含有Lys6或Lys63残基的泛素肽的特异性结合。在质谱表位鉴定的表位切除中,使用pronase对固定的K63-Ub抗体结合的泛素构建块与Lys63残基进行蛋白水解裂解。所得到的表位和非表位片段进行了基质辅助激光解吸/电离飞行时间分析,显示表位位于泛素序列(60-66)。表位提取-质谱法一致证实了这些发现。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Epitope identification of a Lys63 linkage ubiquitin antibody by mass spectrometric epitope excision and extraction approaches.

Ubiquitin, a conserved protein in eukaryotic cells, exists as a monomer or polyubiquitin chains known as isopeptide-linked polymers. These chains are attached to a substrate or other ubiquitin molecules through a covalent bond between the α-amino group of lysine in ubiquitin and glycine in the C-terminal of the subsequent ubiquitin unit. The choice of the specific lysine residue in ubiquitin for forming ubiquitin-ubiquitin chains determines its biochemical and biological function. A detailed chemical structure-function evaluation of the respective polyubiquitin chain is required. Interestingly, specific lysine linkage polyubiquitin chains become covalently bonded to many pathological inclusions seen in serious human disease states which appear to be resistant to normal degradation, so the interaction between polyubiquitin chains and ubiquitin antibodies is very useful. For example, the neurofibrillary tangles of Alzheimer's disease and the Lewy bodies seen in Parkinson's disease are heavily ubiquitinated and can be readily visualized using specific ubiquitin antibodies. This study utilized synthetic ubiquitin building block peptides that contained various lysine residues (K6, K11, K33, K48, and K63) linked to a Gly-Gly dipeptide, with the aim of exploring the recognition specificity of the Lys63-polyubiquitin antibody. The interaction studies between different ubiquitin building blocks and the specific Lys63-ubiquitin (K63-Ub) antibody were performed by affinity-mass spectrometry (Affinity-MS) and immunoblotting which enables direct protein identification from biological material with unprecedented selectivity. Affinity-MS and dot blot data proved the specific binding of the K63-Ub antibody to the ubiquitin peptides containing Lys6 or Lys63 residues. In epitope excision for mass spectrometric epitope identification, the ubiquitin building block with Lys63 residue bound to the immobilized K63-Ub antibody was proteolytically cleaved using pronase. The resulting epitope and non-epitope fractions were subjected to matrix-assisted laser desorption/ionization-time of flight analysis, revealing that the epitope is located within the sequence ubiquitin(60-66). Epitope extraction-MS consistently confirmed these findings.

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来源期刊
CiteScore
2.40
自引率
7.70%
发文量
16
审稿时长
>12 weeks
期刊介绍: JMS - European Journal of Mass Spectrometry, is a peer-reviewed journal, devoted to the publication of innovative research in mass spectrometry. Articles in the journal come from proteomics, metabolomics, petroleomics and other areas developing under the umbrella of the “omic revolution”.
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