Depletion of Abundant Plasma Proteins and Limitations of Plasma Proteomics

猎枪 化学 等电聚焦 血液蛋白质类 鸟枪蛋白质组学 蛋白质组学 蛋白质组 串联质谱法 色谱法 分馏 人血浆 质谱法 生物化学 基因
作者
Chengjian Tu,Paul A. Rudnick,Misti Y. Martinez,Kristin L. Cheek,Stephen E. Stein,Robbert J.C. Slebos,D.C. Liebler
出处
期刊:Journal of Proteome Research [American Chemical Society]
卷期号:9 (10): 4982-4991 被引量:351
标识
DOI:10.1021/pr100646w
摘要

Immunoaffinity depletion with antibodies to the top 7 or top 14 high-abundance plasma proteins is used to enhance detection of lower abundance proteins in both shotgun and targeted proteomic analyses. We evaluated the effects of top 7/top 14 immunodepletion on the shotgun proteomic analysis of human plasma. Our goal was to evaluate the impact of immunodepletion on detection of proteins across detectable ranges of abundance. The depletion columns afforded highly repeatable and efficient plasma protein fractionation. Relatively few nontargeted proteins were captured by the depletion columns. Analyses of unfractionated and immunodepleted plasma by peptide isoelectric focusing (IEF), followed by liquid chromatography−tandem mass spectrometry (LC−MS/MS), demonstrated enrichment of nontargeted plasma proteins by an average of 4-fold, as assessed by MS/MS spectral counting. Either top 7 or top 14 immunodepletion resulted in a 25% increase in identified proteins compared to unfractionated plasma. Although 23 low-abundance (<10 ng mL−1) plasma proteins were detected, they accounted for only 5−6% of total protein identifications in immunodepleted plasma. In both unfractionated and immunodepleted plasma, the 50 most abundant plasma proteins accounted for 90% of cumulative spectral counts and precursor ion intensities, leaving little capacity to sample lower abundance proteins. Untargeted proteomic analyses using current LC−MS/MS platforms—even with immunodepletion—cannot be expected to efficiently discover low-abundance, disease-specific biomarkers in plasma.
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