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突变一个保守残基可增强类似物敏化激酶的敏感性,为研究裂殖酵母有丝分裂提供新方法。

Mutation of a conserved residue enhances the sensitivity of analogue-sensitised kinases to generate a novel approach to the study of mitosis in fission yeast.

机构信息

CRUK Cell Division Group, Paterson Institute for Cancer Research, Wilmslow Road, Manchester M20 4BX, UK.

出版信息

J Cell Sci. 2013 Nov 1;126(Pt 21):5052-61. doi: 10.1242/jcs.135301. Epub 2013 Aug 28.

Abstract

The chemical genetic strategy in which mutational enlargement of the ATP-binding site sensitises of a protein kinase to bulky ATP analogues has proved to be an elegant tool for the generation of conditional analogue-sensitive kinase alleles in a variety of model organisms. Here, we describe a novel substitution mutation in the kinase domain that can enhance the sensitivity of analogue-sensitive kinases. Substitution of a methionine residue to phenylalanine in the +2 position after HRDLKxxN motif of the subdomain VIb within the kinase domain markedly increased the sensitivities of the analogue-sensitive kinases to ATP analogues in three out of five S. pombe kinases (i.e. Plo1, Orb5 and Wee1) that harbor this conserved methionine residue. Kinome alignment established that a methionine residue is found at this site in 5-9% of kinases in key model organisms, suggesting that a broader application of this structural modification may enhance ATP analogue sensitivity of analogue-sensitive kinases in future studies. We also show that the enhanced sensitivity of the wee1.as8 allele in a cdc25.22 background can be exploited to generate highly synchronised mitotic and S phase progression at 36°C. Proof-of-principle experiments show how this novel synchronisation technique will prove of great use in the interrogation of the mitotic or S-phase functions through temperature sensitivity mutation of molecules of interest in fission yeast.

摘要

化学遗传学策略中,通过突变扩大 ATP 结合位点,使蛋白激酶对大体积的 ATP 类似物敏感,这已被证明是在多种模式生物中生成条件性类似物敏感激酶等位基因的一种优雅工具。在这里,我们描述了一种激酶结构域中的新型取代突变,可增强类似物敏感激酶的敏感性。在激酶结构域的亚结构域 VIb 内 HRDLKxxN 基序的+2 位置将甲硫氨酸残基替换为苯丙氨酸,可显著提高五种裂殖酵母激酶(即 Plo1、Orb5 和 Wee1)中三个激酶对 ATP 类似物的敏感性,这些激酶都含有该保守的甲硫氨酸残基。激酶组比对确定,在关键模型生物中的 5-9%的激酶中,该位点存在一个甲硫氨酸残基,这表明这种结构修饰的更广泛应用可能会在未来的研究中提高类似物敏感激酶对 ATP 类似物的敏感性。我们还表明,cdc25.22 背景下 wee1.as8 等位基因的敏感性增强可用于在 36°C 下生成高度同步的有丝分裂和 S 期进程。原理验证实验表明,这种新的同步技术将如何通过在裂殖酵母中对感兴趣分子的温度敏感性突变来研究有丝分裂或 S 期功能,从而非常有用。

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