Automated High-Throughput Affinity Capture-Mass Spectrometry Platform with Data-Independent Acquisition

吞吐量 质谱法 化学 计算机科学 计算生物学 色谱法 生物 操作系统 无线
作者
Hui Jing,Paul L. Richardson,Gregory K. Potts,Sameera Senaweera,Violeta L. Marin,Ryan A. McClure,Adam Banlasan,Hua Tang,James E. Kath,Shitalben Patel,Maricel Torrent,Renze Ma,Jon D. Williams
出处
期刊:Journal of Proteome Research [American Chemical Society]
标识
DOI:10.1021/acs.jproteome.4c00696
摘要

Affinity capture (AC) combined with mass spectrometry (MS)-based proteomics is highly utilized throughout the drug discovery pipeline to determine small-molecule target selectivity and engagement. However, the tedious sample preparation steps and time-consuming MS acquisition process have limited its use in a high-throughput format. Here, we report an automated workflow employing biotinylated probes and streptavidin magnetic beads for small-molecule target enrichment in the 96-well plate format, ending with direct sampling from EvoSep Solid Phase Extraction tips for liquid chromatography (LC)-tandem mass spectrometry (MS/MS) analysis. The streamlined process significantly reduced both the overall and hands-on time needed for sample preparation. Additionally, we developed a data-independent acquisition-mass spectrometry (DIA-MS) method to establish an efficient label-free quantitative chemical proteomic kinome profiling workflow. DIA-MS yielded a coverage of ∼380 kinases, a > 60% increase compared to using a data-dependent acquisition (DDA)-MS method, and provided reproducible target profiling of the kinase inhibitor dasatinib. We further showcased the applicability of this AC-MS workflow for assessing the selectivity of two clinical-stage CDK9 inhibitors against ∼250 probe-enriched kinases. Our study here provides a roadmap for efficient target engagement and selectivity profiling in native cell or tissue lysates using AC-MS.
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