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拟南芥中假定的CPK5底物的体内鉴定。

In vivo identification of putative CPK5 substrates in Arabidopsis thaliana.

作者信息

Yip Delormel Tiffany, Avila-Ospina Liliana, Davanture Marlène, Zivy Michel, Lang Julien, Valentin Nicolas, Rayapuram Naganand, Hirt Heribert, Colcombet Jean, Boudsocq Marie

机构信息

Université Paris-Saclay, CNRS, INRAE, Univ Evry, Institute of Plant Sciences Paris-Saclay (IPS2), 91405, Orsay, France; Université de Paris, Institute of Plant Sciences Paris-Saclay (IPS2), 91405, Orsay, France.

Université Paris-Saclay, INRAE, CNRS, AgroParisTech, Génétique Quantitative et Évolution (GQE) - Le Moulon, 91190, Gif-sur-Yvette, France.

出版信息

Plant Sci. 2022 Jan;314:111121. doi: 10.1016/j.plantsci.2021.111121. Epub 2021 Nov 17.

DOI:10.1016/j.plantsci.2021.111121
PMID:34895550
Abstract

Calcium signaling mediates most developmental processes and stress responses in plants. Among plant calcium sensors, the calcium-dependent protein kinases display a unique structure harboring both calcium sensing and kinase responding activities. AtCPK5 is an essential member of this family in Arabidopsis that regulates immunity and abiotic stress tolerance. To understand the underlying molecular mechanisms, we implemented a biochemical approach to identify in vivo substrates of AtCPK5. We generated transgenic lines expressing a constitutively active form of AtCPK5 under the control of a dexamethasone-inducible promoter. Lines expressing a kinase-dead version were used as a negative control. By comparing the phosphoproteome of the kinase-active and kinase-dead lines upon dexamethasone treatment, we identified 5 phosphopeptides whose abundance increased specifically in the kinase-active lines. Importantly, we showed that all 5 proteins were phosphorylated in vitro by AtCPK5 in a calcium-dependent manner, suggesting that they are direct targets of AtCPK5. We also detected several interaction patterns between the kinase and the candidates in the cytosol, membranes or nucleus, consistent with the ubiquitous localization of AtCPK5. Finally, we further validated the two phosphosites S245 and S280 targeted by AtCPK5 in the E3 ubiquitin ligase ATL31. Altogether, those results open new perspectives to decipher AtCPK5 biological functions.

摘要

钙信号传导介导植物中的大多数发育过程和应激反应。在植物钙传感器中,钙依赖性蛋白激酶具有独特的结构,兼具钙传感和激酶反应活性。AtCPK5是拟南芥中该家族的一个重要成员,它调节免疫和非生物胁迫耐受性。为了了解其潜在的分子机制,我们采用生化方法来鉴定AtCPK5在体内的底物。我们构建了在地塞米松诱导型启动子控制下表达组成型活性形式AtCPK5的转基因株系。表达激酶失活版本的株系用作阴性对照。通过比较地塞米松处理后激酶活性株系和激酶失活株系的磷酸化蛋白质组,我们鉴定出5种磷酸肽,其丰度在激酶活性株系中特异性增加。重要的是,我们表明所有这5种蛋白质在体外都能被AtCPK5以钙依赖性方式磷酸化,这表明它们是AtCPK5的直接靶标。我们还在细胞质、膜或细胞核中检测到了激酶与候选蛋白之间的几种相互作用模式,这与AtCPK5的普遍定位一致。最后,我们进一步验证了E3泛素连接酶ATL31中AtCPK5靶向的两个磷酸化位点S245和S280。总之,这些结果为解读AtCPK5的生物学功能开辟了新的视角。

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