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A chemical-genetic approach for functional analysis of plant protein kinases

机译:化学遗传方法对植物蛋白激酶进行功能分析

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摘要

Plant genomes encode hundreds of protein kinases, yet only for a small fraction of them precise functions and phos-phorylation targets have been identified. Recently, we applied a chemical-genetic approach to sensitize the tomato serine/ threonine kinase Pto to analogs of PP1, an ATP-competitive and cell-permeable small-molecule inhibitor. The Pto kinase confers resistance to Pst bacteria by activating immune responses upon specific recognition of bacterial effectors. By using PP1 analogs in combination with the analog-sensitive Pto, we shed new light on the role of Pto kinase activity in effector recognition and signal transduction. Here we broaden the use of this chemical-genetic approach to another defense-related plant protein kinase, the MAP kinase LeMPK3. In addition, we show that analog-sensitive but not wild-type kinases are able to use unnatural N6-modified ATP analogs as phosphodonors that can be exploited for tagging direct phosphorylation targets of the kinase of interest. Thus, sensitization of kinases to analogs of the small-molecule inhibitor PP1 and ATP can be an effective tool for the discovery of cellular functions and phosphorylation substrates of plant protein kinases.
机译:植物基因组编码数百种蛋白激酶,但仅其中的一小部分就已经确定了精确的功能和磷酸化目标。最近,我们应用化学遗传方法使番茄丝氨酸/苏氨酸激酶Pto对PP1的类似物敏感,PP1是一种具有ATP竞争性和细胞渗透性的小分子抑制剂。 Pto激酶通过特异性识别细菌效应子激活免疫反应,从而赋予对Pst细菌的抗性。通过将PP1类似物与类似物敏感的Pto结合使用,我们对Pto激酶活性在效应子识别和信号转导中的作用有了新的认识。在这里,我们将这种化学遗传方法的应用扩展到另一种与防御相关的植物蛋白激酶MAP激酶LeMPK3。此外,我们表明类似物敏感但不是野生型激酶能够使用非天然的N6修饰的ATP类似物作为供体,可用于标记感兴趣的激酶的直接磷酸化靶标。因此,使激酶对小分子抑制剂PP1和ATP类似物的敏感性可以成为发现植物蛋白激酶的细胞功能和磷酸化底物的有效工具。

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