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甘蓝型油菜根质膜水通道蛋白的分析:翻译后修饰、从头测序和高分辨质谱法检测同工型。

Analysis of root plasma membrane aquaporins from Brassica oleracea: post-translational modifications, de novo sequencing and detection of isoforms by high resolution mass spectrometry.

机构信息

Plataforma de Proteómica, CIC bioGUNE, CIBERehd, ProteoRed, Parque Tecnológico de Bizkaia, 48160, Bizkaia, Spain.

出版信息

J Proteome Res. 2010 Jul 2;9(7):3479-94. doi: 10.1021/pr901150g.

DOI:10.1021/pr901150g
PMID:20462273
Abstract

Plasma membrane Intrinsic Proteins (PIPs), a subfamily of aquaporins, are ubiquitous membrane channel proteins that play a crucial role in water uptake in plants. The use of high-performance liquid chromatography coupled to tandem mass spectrometry (HPLC-MS/MS) analysis of peptides has previously shown to be a valuable tool to differentiate among PIP homologues sharing a high sequence homology and also to characterize their post-translational modifications (PTMs). The recent introduction of mass spectrometers able to measure peptide mass with high mass accuracy, together with new alternative ways of peptide fragmentation allows the identification and characterization of proteins from nonsequenced organisms, such as broccoli. In this study, we combined three endoproteases (trypsin, Glu-C and Lys-C) with HPLC-MS/MS analysis and two types of peptide fragmentations, CID (collision induced dissociation) and HCD (higher-energy C-trap dissociation), to identify PIP isoforms and PTMs from broccoli roots. After de novo sequencing analysis, eight peptides showing homology to Arabidopsis thaliana PIPs were identified. Although Arabidopsis nomenclature of PIP isoforms has not been defined for broccoli, our results agree with the occurrence of seven AtPIP isoforms (PIP 1;1, PIP 1;2, PIP 1;3 and PIP2;2, PIP 2;3, PIP2;1 and PIP2;7) in broccoli roots, as compared to the plant model A. thaliana. To our knowledge, these results represent the deepest characterization of the PIPs isolated from the roots of broccoli, a crop with increasing agronomical interest.

摘要

质膜内在蛋白(PIPs)是水通道蛋白家族的一个亚家族,是植物中吸水的普遍存在的膜通道蛋白。先前的研究表明,使用高效液相色谱-串联质谱(HPLC-MS/MS)分析肽是区分具有高度序列同源性的 PIP 同源物并表征其翻译后修饰(PTM)的有效工具。最近,能够以高精度测量肽质量的质谱仪的引入,以及肽碎片化的新替代方法,使得能够鉴定和表征来自非测序生物体(如西兰花)的蛋白质。在这项研究中,我们将三种内切酶(胰蛋白酶、Glu-C 和 Lys-C)与 HPLC-MS/MS 分析以及两种类型的肽碎片化(CID(碰撞诱导解离)和 HCD(高能 C 阱解离))相结合,从西兰花根中鉴定 PIP 同工型和 PTM。在从头测序分析后,鉴定出 8 个与拟南芥 PIP 具有同源性的肽。尽管尚未为西兰花定义 PIP 同工型的拟南芥命名法,但我们的结果与在西兰花根中存在 7 种 AtPIP 同工型(PIP 1;1、PIP 1;2、PIP 1;3 和 PIP2;2、PIP 2;3、PIP2;1 和 PIP2;7)一致,与植物模型 A.thaliana 相比。据我们所知,这些结果代表了从西兰花根中分离出的 PIPs 的最深入表征,西兰花是一种具有越来越大农艺学兴趣的作物。

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