Fully integrated on-line strategy for highly sensitive proteome profiling of 10–500 mammalian cells

蛋白质组 蛋白质组学 化学 可扩展性 纳米技术 色谱法 计算机科学 计算生物学 材料科学 生物 生物化学 数据库 基因
作者
Yun Yang,Shuangwen Sun,Shunji He,Chengmin Liu,Changying Fu,Min Tang,Chao Liu,Ying Sun,Henry H N Lam,Yong Li,Ruijun Tian
出处
期刊:Analyst [The Royal Society of Chemistry]
卷期号:148 (1): 120-127 被引量:1
标识
DOI:10.1039/d2an01508k
摘要

Recent development in proteomic sample preparation using nanofluidic devices has made single-cell proteome profiling possible. However, these nanofluidic devices require special expertise and costly nanopipetting instruments. They are also specially designed for single cells, are not well-suited for profiling rare samples consisting of a few hundred mammalian cells, arguably a more common need that remains a great challenge. Herein, we developed an easy-to-use and scalable device for processing low-input samples, which combined the merits of previously reported rare cell proteomic reactor (RCPR) and mixed-mode simple and integrated spintip-based proteomics technology, as an alternative to nanofluidic devices. All steps of proteomics sample preparation, including protein preconcentration, impurity removal, reduction, alkylation, digestion, and desalting, were fully integrated in our workflow, and the device can be directly connected to online nanoLC-MS system after processing the rare samples. Using the developed 3-frit mixed-mode RCPR, we identified on average 946 ± 158, 2 998 ± 106, and 3 934 ± 85 protein groups in data-dependent acquisition (DDA) mode from 10, 100, and 500 fluorescence-activated cell sorting (FACS)-sorted 293T cells, respectively. As an illustrative application of this technology, we performed a label-free proteome comparison of 500 FACS-sorted mouse cochlear hair cells of two different ages. On average, 2 595 ± 230 and 2 042 ± 120 protein groups were quantified in the juvenile and the adult samples in DDA mode, respectively, achieving dynamic ranges of over 6 orders of magnitude for both.
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