Simple and Integrated Spintip-Based Technology Applied for Deep Proteome Profiling

化学 蛋白质组学 色谱法 分馏 蛋白质组 计算生物学 样品制备 质谱法 生物化学 生物 基因
作者
Wendong Chen,Shuai Wang,Subash Adhikari,Zongyi Deng,Lingjue Wang,Lan Chen,Mi Ke,Pengyuan Yang,Ruijun Tian
出处
期刊:Analytical Chemistry [American Chemical Society]
卷期号:88 (9): 4864-4871 被引量:104
标识
DOI:10.1021/acs.analchem.6b00631
摘要

Great efforts have been taken for developing high-sensitive mass spectrometry (MS)-based proteomic technologies, among which sample preparation is one of the major focus. Here, a simple and integrated spintip-based proteomics technology (SISPROT) consisting of strong cation exchange beads and C18 disk in one pipet tip was developed. Both proteomics sample preparation steps, including protein preconcentration, reduction, alkylation, and digestion, and reversed phase (RP)-based desalting and high-pH RP-based peptide fractionation can be achieved in a fully integrated manner for the first time. This easy-to-use technology achieved high sensitivity with negligible sample loss. Proteomic analysis of 2000 HEK 293 cells readily identified 1270 proteins within 1.4 h of MS time, while 7826 proteins were identified when 100000 cells were processed and analyzed within only 22 h of MS time. More importantly, the SISPROT can be easily multiplexed on a standard centrifuge with good reproducibility (Pearson correlation coefficient > 0.98) for both single-shot analysis and deep proteome profiling with five-step high-pH RP fractionation. The SISPROT was exemplified by the triplicate analysis of 100000 stem cells from human exfoliated deciduous teeth (SHED). This led to the identification of 9078 proteins containing 3771 annotated membrane proteins, which was the largest proteome data set for dental stem cells reported to date. We expect that the SISPROT will be well suited for deep proteome profiling for fewer than 100000 cells and applied for translational studies where multiplexed technology with good label-free quantification precision is required.
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