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利用表面增强激光解吸电离飞行时间质谱法同时监测多种激酶活性

Simultaneous monitoring of multiple kinase activities by SELDI-TOF mass spectrometry.

作者信息

Thulasiraman Vanitha, Wang Zheng, Katrekar Anjali, Lomas Lee, Yip Tai-Tung

机构信息

Department of Biological Research, Ciphergen Biosystems, Inc, Fremont, CA, USA.

出版信息

Methods Mol Biol. 2004;264:205-14. doi: 10.1385/1-59259-759-9:205.

Abstract

Cellular response to the external environment is often controlled by one or more protein kinases. We report a methodology for simultaneously monitoring multiple kinase activities across multiple signal-transduction pathways using ProteinChip Array technology. Based on the addition of specific peptide reporters, kinase activity is detected by the presence of a mass shift of 80 Da (or multiple thereof) corresponding to the addition of one or more phosphate groups. These phosphorylated peptide substrates are then enriched using an immobilized metal affinity capture (IMAC)-Ga array and detected directly by surface-enhanced laser desorption/ionization time-of-flight mass spectrometry (SELDI-TOF MS). SELDI-TOF MS is sensitive, tagless (nonradioactive, nonfluorescent), can be easily multiplexed for the analysis of several different kinases in a single reaction mixture (limited only by the specificity of the kinase for its substrate peptides), and is directly scalable through the use of robotic sample processing. By multiplexing kinase assays, one can dramatically increase the amount of information obtained from rare or volume-limited samples. More important, results reflect closely the complex interrelationships between kinases and show high correlation with in vivo assays.

摘要

细胞对外界环境的反应通常由一种或多种蛋白激酶控制。我们报告了一种使用蛋白质芯片阵列技术同时监测多个信号转导途径中多种激酶活性的方法。基于添加特定的肽报告分子,通过对应于添加一个或多个磷酸基团的80 Da(或其倍数)的质量位移来检测激酶活性。然后使用固定化金属亲和捕获(IMAC)-镓阵列富集这些磷酸化的肽底物,并通过表面增强激光解吸/电离飞行时间质谱(SELDI-TOF MS)直接检测。SELDI-TOF MS灵敏、无标记(非放射性、非荧光性),可以很容易地进行多重分析,用于在单一反应混合物中分析几种不同的激酶(仅受激酶对其底物肽的特异性限制),并且通过使用机器人样品处理可直接扩展。通过多重激酶测定,可以显著增加从稀有或体积有限的样品中获得的信息量。更重要的是,结果紧密反映了激酶之间复杂的相互关系,并与体内测定显示出高度相关性。

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