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免疫亲和富集和检测的优化:通过液相色谱-质谱法全面表征 K562 细胞的磷酸酪氨酸蛋白质组。

Optimization of immunoaffinity enrichment and detection: toward a comprehensive characterization of the phosphotyrosine proteome of K562 cells by liquid chromatography-mass spectrometry.

机构信息

Department of Physical and Analytical Chemistry, Uppsala University, SE-751 24 Uppsala, Sweden.

出版信息

Analyst. 2011 May 7;136(9):1971-8. doi: 10.1039/c0an00649a. Epub 2011 Mar 14.

DOI:10.1039/c0an00649a
PMID:21403953
Abstract

Phosphorylation of protein tyrosine residues regulates many cell functions and has also been proved to be involved in oncogenesis. Thus, the identification of the phosphotyrosine (pTyr) proteome of cells is a very important task. Since tyrosine phosphorylation represents only around 1% of the total human phosphoproteome, the study of pTyr proteins is rather challenging. Here we report the optimization study of the phosphotyrosine proteome using K562 cells as a model system. A substantial segment of the phosphotyrosine proteome of K562 cells was characterized by immunoaffinity enrichment with 4G10 and PYKD1 antibodies followed by LC-MS/MS analysis. 480 non-redundant pTyr peptides corresponding to 342 pTyr proteins were found. 141 pTyr peptides were not described elsewhere. The mass spectrometry approach involving high-resolving FTMS analysis of precursor ions and subsequent detection of CID fragments in a linear ion trap was considered as optimal. For detection of low abundant pTyr peptides pooling of individual immunoaffinity enrichments for one LC-MS/MS analysis was crucial. The enrichment properties of the monoclonal PYKD1 antibody were presented for the first time, also in comparison to the 4G10 antibody. PYKD1 was found to be more effective for protein enrichment (1.2 and 5% efficiency at peptide and protein level correspondingly), while 4G10 showed better results when peptide enrichment was performed (15% efficiency versus 3.6% at protein level). Substantially different subsets of the phosphoproteome were enriched by these antibodies. This finding together with previous studies demonstrates that comprehensive pTyr proteome characterization by immunoprecipitation requires multiple antibodies to be used for the affinity enrichment.

摘要

磷酸化的酪氨酸残基调节许多细胞功能,并且已经被证明参与了致癌作用。因此,鉴定细胞的磷酸酪氨酸(pTyr)蛋白质组是一项非常重要的任务。由于酪氨酸磷酸化仅占人类磷酸蛋白质组的约 1%,因此研究 pTyr 蛋白质具有相当大的挑战性。在这里,我们报告了使用 K562 细胞作为模型系统优化磷酸酪氨酸蛋白质组研究的结果。使用 4G10 和 PYKD1 抗体进行免疫亲和富集,然后进行 LC-MS/MS 分析,鉴定了 K562 细胞中相当大一部分的磷酸酪氨酸蛋白质组。发现了 480 个非冗余的 pTyr 肽,对应于 342 个 pTyr 蛋白质。有 141 个 pTyr 肽在其他地方没有描述过。涉及高分辨率 FTMS 分析前体离子和随后在线性离子阱中检测 CID 片段的质谱方法被认为是最佳的。为了检测低丰度的 pTyr 肽,将单个免疫亲和富集物汇集到一个 LC-MS/MS 分析中是至关重要的。首次提出了单克隆 PYKD1 抗体的富集特性,也与 4G10 抗体进行了比较。PYKD1 被发现对蛋白质富集更有效(肽和蛋白质水平的效率分别为 1.2%和 5%),而 4G10 则在进行肽富集时表现出更好的效果(肽水平的效率为 15%,而蛋白质水平的效率为 3.6%)。这些抗体富集了磷酸蛋白质组的大量不同子集。这一发现与以前的研究一起表明,通过免疫沉淀进行全面的 pTyr 蛋白质组特征描述需要使用多种抗体进行亲和富集。

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