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一种新型三重等压末端标记定量方法,可同时提供三种定量来源。

A novel triplex isobaric termini labeling quantitative approach for simultaneously supplying three quantitative sources.

机构信息

Shanghai Cancer Centre and Institutes of Biomedical Sciences, Fudan University, Shanghai 200032, PR China; Department of Chemistry, Fudan University, Shanghai 200433, PR China.

Shanghai Cancer Centre and Institutes of Biomedical Sciences, Fudan University, Shanghai 200032, PR China.

出版信息

Anal Chim Acta. 2018 Feb 25;1001:70-77. doi: 10.1016/j.aca.2017.11.004. Epub 2017 Nov 9.

DOI:10.1016/j.aca.2017.11.004
PMID:29291808
Abstract

Benefiting from high sensitivity and great ability to measure multiple samples simultaneously, isobaric tandem Mass spectrometry (MS2) quantification has been widely applied for protein biomarker screening. Here, a newly developed isobaric MS2 quantification method named triplex quantification by isobaric termini labeling (Triplex-QITL) was established. This method enables the accurate comparison of various fragment ions (reporter ions, amino acid fragments and N-/C-terminal fragments) based quantification to be operated in a single run. To our knowledge, this is the first time that this kind of comparison is achieved. In Triplex-QITL, proteins were first digested with Lys-C to produce peptides with lysine (K) at the C-termini, then dimethylation reagents and mTRAQ reagents were used to label the N-termini and C-termini of the peptides respectively. N- and C-terminal fragment ion pairs, reporter ions from mTRAQ (113,117,121) and a ion pairs were simultaneously generated in MS2 spectra. In simple sample experiment, not much difference in using various fragment ions for quantification was observed. When analyzing SW480 cell lysate, comparing with a1 ions, about two times of reproducible quantification results were achieved by reporter ions and N- and C-terminal ions. Meanwhile the measured quantification results were much closer to the expected results even in large ratios (1:10:10) using N- and C-terminal ions. Finally, Triplex-QITL was successfully applied to profile metastatic differences of three hepatocellular carcinoma (HCC) cell lines. In all, Triplex-QITL shows a promising future in quantitative proteomics.

摘要

得益于高灵敏度和同时测量多个样本的强大能力,等压串联质谱(MS2)定量已广泛应用于蛋白质生物标志物筛选。在这里,建立了一种新的等压 MS2 定量方法,命名为等压末端标记三重定量(Triplex-QITL)。该方法能够在单次运行中对各种片段离子(报告离子、氨基酸片段和 N-/C-末端片段)进行准确的比较定量。据我们所知,这是第一次实现这种比较。在 Triplex-QITL 中,首先用 Lys-C 消化蛋白质以产生赖氨酸(K)在 C 末端的肽,然后用二甲基化试剂和 mTRAQ 试剂分别标记肽的 N-末端和 C-末端。在 MS2 谱中同时产生 N-和 C-末端片段离子对、mTRAQ 的报告离子(113、117、121)和 a1 离子对。在简单的样品实验中,使用各种片段离子进行定量时,差异不大。当分析 SW480 细胞裂解物时,与 a1 离子相比,报告离子和 N-和 C-末端离子的重复性定量结果约增加两倍。同时,即使使用 N-和 C-末端离子的比例很大(1:10:10),测量的定量结果也更接近预期结果。最后,Triplex-QITL 成功应用于三种肝癌(HCC)细胞系的转移差异分析。总之,Triplex-QITL 在定量蛋白质组学中具有广阔的应用前景。

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