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Multistep Mass Tagging Coupled with 2D LC-MS—An Approach to Increasing the Number of Identified Proteins

机译:多步质量标记与二维LC-MS结合使用—一种增加鉴定蛋白质数量的方法

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摘要

Identification of large numbers of proteins from complex biological samples is a continuing challenge in the area of quantitative proteomics. We introduce here a simple and reliable multistep mass tagging technique using our recently developed solid phase mass tagging reagents. When coupled with two-dimensional liquid chromatographyano-electrospray ionization ion trap mass spectrometry (2D-LCano-ESI-MS), this method allows enhanced protein identification when tested on samples from prokaryotic and eukaryotic sources. The proteome of Escherichia coli D21 grown to either mid-exponential or stationary phase, and the membrane proteome from established breast cancer cell lines BT474 and MCF7 were used as model systems in these experiments. In both experiments, the numbers of total identified proteins are at least twice the numbers identified from a single tagging cycle. The sample complexity can be effectively reduced with corresponding increases in protein identification using the multistep method. The strategy described here represents a potentially powerful technique for large-scale qualitative and quantitative proteome research.
机译:从复杂的生物样品中鉴定大量蛋白质是定量蛋白质组学领域的持续挑战。我们在这里介绍一种使用我们最近开发的固相质量标记试剂的简单可靠的多步质量标记技术。与二维液相色谱/纳米电喷雾电离离子阱质谱法(2D-LC /纳米ESI-MS)结合使用时,此方法在对原核和真核来源的样品进行测试时,可以增强蛋白质的鉴定。在这些实验中,将大肠杆菌D21的蛋白质组生长到指数中期或固定期,并将已建立的乳腺癌细胞系BT474和MCF7的膜蛋白质组用作模型系统。在两个实验中,总鉴定出的蛋白质数量至少是从单个标记周期鉴定出的蛋白质数量的两倍。使用多步方法可以有效地降低样品的复杂性,同时增加相应的蛋白质鉴定。此处描述的策略代表了大规模定性和定量蛋白质组研究的潜在强大技术。

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