蛋白质组学
定量蛋白质组学
等压标记
多路复用
无标记量化
计算机科学
计算生物学
串联质量标签
生物
生物化学
电信
基因
作者
Nishant Pappireddi,Lance Martin,Martin Wühr
出处
期刊:ChemBioChem
[Wiley]
日期:2019-01-04
卷期号:20 (10): 1210-1224
被引量:322
标识
DOI:10.1002/cbic.201800650
摘要
Over the last few decades, mass spectrometry-based proteomics has become an increasingly powerful tool that is now able to routinely detect and quantify thousands of proteins. A major advance for global protein quantification was the introduction of isobaric tags, which, in a single experiment, enabled the global quantification of proteins across multiple samples. Herein, these methods are referred to as multiplexed proteomics. The principles, advantages, and drawbacks of various multiplexed proteomics techniques are discussed and compared with alternative approaches. We also discuss how the emerging combination of multiplexing with targeted proteomics might enable the reliable and high-quality quantification of very low abundance proteins across multiple conditions. Lastly, we suggest that fusing multiplexed proteomics with data-independent acquisition approaches might enable the comparison of hundreds of different samples without missing values, while maintaining the superb measurement precision and accuracy obtainable with isobaric tag quantification.
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