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在线纳流反相-强阴离子交换-反相液相色谱-串联质谱平台,用于高效和深入分析复杂生物的蛋白质组序列。

Online nanoflow reversed phase-strong anion exchange-reversed phase liquid chromatography-tandem mass spectrometry platform for efficient and in-depth proteome sequence analysis of complex organisms.

机构信息

Department of Cancer Biology, Dana-Farber Cancer Institute, Boston, Massachusetts 02215-5450, United States.

出版信息

Anal Chem. 2011 Sep 15;83(18):6996-7005. doi: 10.1021/ac200639v. Epub 2011 Aug 18.

DOI:10.1021/ac200639v
PMID:21851055
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3196608/
Abstract

The dynamic range of protein expression in complex organisms coupled with the stochastic nature of discovery-driven tandem mass spectrometry (MS/MS) analysis continues to impede comprehensive sequence analysis and often provides only limited information for low-abundance proteins. High-performance fractionation of proteins or peptides prior to mass spectrometry analysis can mitigate these effects, though achieving an optimal combination of automation, reproducibility, separation peak capacity, and sample yield remains a significant challenge. Here we demonstrate an automated nanoflow 3-D liquid chromatography (LC)-MS/MS platform based on high-pH reversed phase (RP), strong anion exchange (SAX), and low-pH reversed phase (RP) separation stages for analysis of complex proteomes. We observed that RP-SAX-RP outperformed RP-RP for analysis of tryptic peptides derived from Escherichia coli and enabled identification of proteins present at a level of 50 copies per cell in Saccharomyces cerevisiae, corresponding to an estimated detection limit of 500 amol, from 40 μg of total lysate on a low-resolution 3-D ion trap mass spectrometer. A similar study performed on a LTQ-Orbitrap yielded over 4000 unique proteins from 5 μg of total yeast lysate analyzed in a single, 101 fraction RP-SAX-RP LC-MS/MS acquisition, providing an estimated detection limit of 65 amol for proteins expressed at 50 copies per cell.

摘要

复杂生物中蛋白质表达的动态范围加上发现驱动的串联质谱(MS/MS)分析的随机性,继续阻碍了全面的序列分析,并且通常仅为低丰度蛋白质提供有限的信息。在进行质谱分析之前,对蛋白质或肽进行高性能分级可以减轻这些影响,但实现自动化、重现性、分离峰容量和样品产量的最佳组合仍然是一个重大挑战。在这里,我们展示了一种基于高 pH 反相(RP)、强阴离子交换(SAX)和低 pH 反相(RP)分离阶段的自动化纳流 3D 液相色谱(LC)-MS/MS 平台,用于分析复杂的蛋白质组。我们观察到,RP-SAX-RP 比 RP-RP 更适合于分析来自大肠杆菌的胰蛋白酶肽,并且能够鉴定出在酿酒酵母中每个细胞存在 50 个拷贝的蛋白质,相当于在低分辨率 3D 离子阱质谱仪上从 40 μg 总裂解物中检测到 500 amol 的估计检测限。在 LTQ-Orbitrap 上进行的类似研究,从 5 μg 总酵母裂解物中分析了超过 4000 个独特蛋白质,在单个 101 级 RP-SAX-RP LC-MS/MS 采集,为每个细胞表达 50 个拷贝的蛋白质提供了 65 amol 的估计检测限。

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