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基于数字微流控的等压肽标记用于低细胞数定量蛋白质组学

Isobaric Peptide Labeling on Digital Microfluidics for Quantitative Low Cell Number Proteomics.

作者信息

Leipert Jan, Steinbach Max K, Tholey Andreas

机构信息

Systematic Proteome Research & Bioanalytics, Institute for Experimental Medicine, Christian-Albrechts-Universität zu Kiel, Kiel 24105, Germany.

出版信息

Anal Chem. 2021 Apr 20;93(15):6278-6286. doi: 10.1021/acs.analchem.1c01205. Epub 2021 Apr 6.

DOI:10.1021/acs.analchem.1c01205
PMID:33823593
Abstract

Digital microfluidics (DMF) is a technology suitable for bioanalytical applications requiring miniaturized, automated, and multiplexed liquid handling. Its use in LC-MS-based proteomics, however, has so far been limited to qualitative proteome analyses. This is mainly due to the need for detergents that enable facile, reproducible droplet movement, which are compatible with organic solvents commonly used in targeted chemical modifications of peptides. Aiming to implement isobaric peptide labeling, a widely applied technique allowing multiplexed quantitative proteome studies, on DMF devices, we tested different commercially available detergents. We identified the maltoside-based detergent 3-dodecyloxypropyl-1-β-d-maltopyranoside (DDOPM) to enable facile droplet movement and show micelle formation even in the presence of organic solvent, which is necessary for isobaric tandem mass tag (TMT) labeling. The detergent is fully compatible with reversed phase LC-MS, not interfering with peptide identification. Tryptic digestion in the presence of DDOPM was more efficient than without detergent, resulting in more protein identifications. Using this detergent, we report the first on-DMF chip isobaric labeling strategy, with TMT-labeling efficiency comparable to conventional protocols. The newly developed labeling protocol was evaluated in the multiplexed analyses of a protein standard digest spiked into 25 cells. Finally, using only 75 cells per biological replicate, we were able to identify 39 proteins being differentially abundant after treatment of Jurkat T cells with the anticancer drug doxorubicin. In summary, we demonstrate an important step toward multiplexed quantitative proteomics on DMF, which, in combination with larger chip arrays and optimized hardware, could enable high throughput low cell number proteomics.

摘要

数字微流控(DMF)是一种适用于生物分析应用的技术,这些应用需要小型化、自动化和多重液体处理。然而,其在基于液相色谱-质谱联用(LC-MS)的蛋白质组学中的应用目前仅限于定性蛋白质组分析。这主要是因为需要使用能够实现便捷、可重复的液滴移动的洗涤剂,这些洗涤剂要与肽段靶向化学修饰中常用的有机溶剂兼容。为了在DMF设备上实现等压肽标记(一种广泛应用于多重定量蛋白质组研究的技术),我们测试了不同的市售洗涤剂。我们发现基于麦芽糖苷的洗涤剂3-十二烷氧基丙基-1-β-D-麦芽糖苷(DDOPM)能够实现便捷的液滴移动,并且即使在存在有机溶剂的情况下也能形成胶束,这对于等压串联质谱标签(TMT)标记是必要的。这种洗涤剂与反相LC-MS完全兼容,不会干扰肽段鉴定。在DDOPM存在下进行胰蛋白酶消化比不使用洗涤剂时更有效,从而鉴定出更多的蛋白质。使用这种洗涤剂,我们报告了首个基于DMF芯片的等压标记策略,其TMT标记效率与传统方案相当。在掺入25个细胞的蛋白质标准消化物的多重分析中评估了新开发的标记方案。最后,每个生物学重复仅使用75个细胞,我们就能够鉴定出用抗癌药物阿霉素处理Jurkat T细胞后差异丰富的39种蛋白质。总之,我们展示了在DMF上进行多重定量蛋白质组学的重要一步,这与更大的芯片阵列和优化的硬件相结合,可以实现高通量低细胞数蛋白质组学。

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