Large-scale single-molecule analysis of tau proteoforms.

bioRxiv : the preprint server for biology Pub Date : 2025-07-21 DOI:10.1101/2025.06.26.660445

J Joly, V Budamagunta, Z Zhang, B Nortman, M Jouzi, R Bhatnagar, J D Egertson, M E Flaster, R Grothe, S Guha, K Kaneshige, K McVey, N Nelson, R T Perera, S J Tan, T Trinh, D Arnott, J Lipka, N J Pandya, L Rougé, T J Wendorff, D S Kirkpatrick, A Rohou, D C Butler, S Lotz, A Forton, E R Sartori, J E Schwarz, P S Brereton, K Chen, M A Darcy, H R Golnabi, R Hartley, P F Indermuhl, C E Inman, K M Jin, S Katsyuk, R Kota, B Lowry, J C Menger, D A Miller, M R Newman, A Ogunyemi, J K Robinson, N Steiner, J Sun, S Tabakman, L Wang, Z Wang, S K Wilcox, G T Kapp, S Patel, S Temple, T Bertucci, J Blanchard, A Huhmer, S Sankar, K Juneau, P Mallick

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Abstract

Proteins exist as diverse proteoforms resulting from a combination of genetic variation, alternative splicing, and post-translational modifications. Current methods struggle to capture this complexity at the single-molecule level. Here we introduce Iterative Ma pping of P roteoforms (IMaP), a method that enables the massively-parallel interrogation of millions to billions of single-protein molecules through iterative probing with fluorescently labeled antibodies. Using 12 site-specific antibodies, the method is capable of measuring 2 ¹² (4,096) potential proteoform groups. We used IMaP to measure proteoform group profiles of the tau protein, a key player in neurodegenerative diseases, using two pan anti-tau antibodies (Tau-13, Tau-216), three isoform-specific antibodies (Anti-0N, Anti-2N, Anti-4R), and seven phosphosite-specific antibodies (Anti-pT181, Anti-pS202+pT205, Anti-pT205, Anti-pS214, Anti-pT217, Anti-pT231, and Anti-pS396). The method demonstrates high sensitivity (detecting proteoforms at 0.1% abundance), high reproducibility (median CV <5.5%), and broad dynamic range (>3 orders of magnitude), outperforming conventional techniques in resolving closely related proteoform groups. We demonstrated that the method can be used on relevant biological samples by examining various neuronal models (iNeuron cells, organoids, MiBrains, and mouse brains) and human samples. This examination revealed 130 distinct tau proteoform groups with as many as six phosphorylation events. The non-random distribution of these phosphorylation events suggests ordered and site-specific modification processes rather than random, stochastic accumulation. Certain combinations of phosphorylation events were more abundant than others; for example, pT217 preferentially co-occurred with pT181. In validating the applicability of the assay to human disease samples, we noted a specific pattern of multiple phosphorylation events in an advanced Alzheimer's disease patient that suggests a sequential pathway of pathological tau modification. Iterative Mapping of Proteoforms provides insights into proteoform complexity at the single-molecule level, with significant implications for understanding protein regulation in neurodegenerative diseases and beyond.

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开发一种大规模单分子分析tau蛋白的方法。

由于遗传变异、选择性剪接和翻译后修饰的结合，蛋白质以多种蛋白质形式存在。目前的方法很难在单分子水平上捕捉这种复杂性。在这里，我们介绍了P原形的迭代映射（IMaP），这是一种通过荧光标记抗体的迭代探测，能够对数百万到数十亿个单蛋白分子进行大规模并行探测的方法。使用12个位点特异性抗体，该方法能够测量12（4,096）个潜在的蛋白类群。我们使用IMaP测量tau蛋白的蛋白质类群特征，tau蛋白是神经退行性疾病的关键参与者，使用两种泛抗tau抗体（tau -13, tau -216），三种异构体特异性抗体（Anti-0N, Anti-2N, Anti-4R）和七种磷酸基特异性抗体（Anti-pT181, Anti-pS202+pT205, Anti-pT205, Anti-pS214, Anti-pT217， Anti-pT231和Anti-pS396）。该方法具有高灵敏度（检测到0.1%丰度的变形）、高重现性（中位CV 3数量级），在解析密切相关的变形类群方面优于传统技术。我们通过检测各种神经元模型（神经元细胞、类器官、miBrains和小鼠大脑）和人类样本，证明了该方法可以用于相关的生物样本。这项检查发现了130个不同的tau蛋白类群，有多达6个磷酸化事件。这些磷酸化事件的非随机分布表明是有序的和特定位点的修饰过程，而不是随机的、随机的积累。某些磷酸化事件的组合比其他的更丰富；例如，pT217优先与pT181共存。在验证该检测方法对人类疾病样本的适用性时，我们注意到在一名晚期阿尔茨海默病患者中出现了多种磷酸化事件的特定模式，这表明病理性tau修饰的顺序途径。蛋白质形式的迭代映射提供了单分子水平上对蛋白质形式复杂性的见解，对理解神经退行性疾病及其他疾病的蛋白质调控具有重要意义。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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