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Large-Scale Comparative Phosphoproteomics Identifies Conserved Phosphorylation Sites in Plants1[W][OA]

机译:大规模比较性磷酸化蛋白质组学鉴定了植物中保守的磷酸化位点[W] [OA]

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摘要

Knowledge of phosphorylation events and their regulation is crucial to understand the functional biology of plants. Here, we report a large-scale phosphoproteome analysis in the model monocot rice (Oryza sativa japonica ‘Nipponbare’), an economically important crop. Using unfractionated whole-cell lysates of rice cells, we identified 6,919 phosphopeptides from 3,393 proteins. To investigate the conservation of phosphoproteomes between plant species, we developed a novel phosphorylation-site evaluation method and performed a comparative analysis of rice and Arabidopsis (Arabidopsis thaliana). The ratio of tyrosine phosphorylation in the phosphoresidues of rice was equivalent to those in Arabidopsis and human. Furthermore, despite the phylogenetic distance and the use of different cell types, more than 50% of the phosphoproteins identified in rice and Arabidopsis, which possessed ortholog(s), had an orthologous phosphoprotein in the other species. Moreover, nearly half of the phosphorylated orthologous pairs were phosphorylated at equivalent sites. Further comparative analyses against the Medicago phosphoproteome also showed similar results. These data provide direct evidence for conserved regulatory mechanisms based on phosphorylation in plants. We also assessed the phosphorylation sites on nucleotide-binding leucine-rich repeat proteins and identified novel conserved phosphorylation sites that may regulate this class of proteins.
机译:磷酸化事件及其调控的知识对于理解植物的功能生物学至关重要。在这里,我们报告了一种具有重要经济意义的单子叶水稻模型(Oryza sativa japonica的“ Nipponbare”)的大规模磷酸化蛋白质组分析。使用未分离的水稻细胞全细胞裂解物,我们从3,393个蛋白质中鉴定出6,919个磷酸肽。为了研究植物物种之间磷酸化蛋白质组的保守性,我们开发了一种新型的磷酸化位点评估方法,并对水稻和拟南芥(Arabidopsis thaliana)进行了比较分析。水稻的磷酸化残基中酪氨酸磷酸化的比例与拟南芥和人类中的相同。此外,尽管系统发育距离远并且使用了不同的细胞类型,但在水稻和拟南芥中鉴定出的具有直系同源物的磷蛋白中,有超过50%的磷蛋白在其他物种中具有直系同源的磷蛋白。此外,近一半的磷酸化直系同源物对在等效位点被磷酸化。针对Medicago磷酸化蛋白质组的进一步比较分析也显示了相似的结果。这些数据提供了基于植物磷酸化的保守调节机制的直接证据。我们还评估了核苷酸结合的富含亮氨酸的重复蛋白上的磷酸化位点,并鉴定了可能调节此类蛋白质的新型保守的磷酸化位点。

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