Magnetic Bead-Based Workflow for Sensitive and Streamlined Cell Surface Proteomics

链霉亲和素 溶解 化学 蛋白质组学 生物素化 免疫磁选 色谱法 生物化学 生物素 计算生物学 生物 基因
作者
Dylan Z. Dieters‐Castator,Paolo Manzanillo,Han-Yin Yang,Rucha V. Modak,Matthew J. Rardin,Bradford W. Gibson
出处
期刊:Journal of Proteome Research [American Chemical Society]
卷期号:23 (2): 618-632 被引量:7
标识
DOI:10.1021/acs.jproteome.3c00432
摘要

Cell surface proteins represent an important class of molecules for therapeutic targeting and cellular phenotyping. However, their enrichment and detection via mass spectrometry-based proteomics remains challenging due to low abundance, post-translational modifications, hydrophobic regions, and processing requirements. To improve their identification, we optimized a Cell-Surface Capture (CSC) workflow that incorporates magnetic bead-based processing. Using this approach, we evaluated labeling conditions (biotin tags and catalysts), enrichment specificity (streptavidin beads), missed cleavages (lysis buffers), nonenzymatic deamidation (digestion and deglycosylation buffers), and data acquisition methods (DDA, DIA, and TMT). Our findings support the use of alkoxyamine-PEG4-biotin plus 5-methoxy-anthranilic acid, SDS/urea-based lysis buffers, single-pot solid-phased-enhanced sample-preparation (SP3), and streptavidin magnetic beads for maximal surfaceome coverage. Notably, with semiautomated processing, sample handling was simplified and between ∼600 and 900 cell surface N-glycoproteins were identified from only 25–200 μg of HeLa protein. CSC also revealed significant differences between in vitro monolayer cultures and in vivo tumor xenografts of murine CT26 colon adenocarcinoma samples that may aid in target identification for drug development. Overall, the improved efficiency of the magnetic-based CSC workflow identified both previously reported and novel N-glycosites with less material and high reproducibility that should help advance the field of surfaceomics by providing insight in cellular phenotypes not previously documented.
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