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Ultrasensitive and absolute quantification of the phosphoinositide 3-kinase/Akt signal transduction pathway by mass spectrometry

机译:质谱法对磷酸肌醇3-激酶/ Akt信号转导途径的超灵敏和绝对定量

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摘要

The phosphoinositide 3-kinase (P13K)/Akt pathway controls a vast array of normal physiological processes and is frequently aberrantly activated in cancer, thus identifying P13K/Akt-signaling components as promising drug targets in oncology. However, implementation of rational cancer therapies for this pathway needs robust and simple tools to stratify patients according to P13K pathway activation and to validate and measure the impact of targeted inhibition on primary cancer tissues. Herein we present a technique for the quantification of the P13K/Akt-signaling pathway based on the mass spectrometric measurement of P13K-dependent protein kinase activity in cell lysates. The concept of this application of MS is to exploit enzymatic activity to amplify the signal of the enzyme under study analogous to the PCR used to amplify nucleic acid sequences. We show that this approach allows quantitative analysis of a cell-signaling pathway with high sensitivity, precision of quantification, and specificity. Due to its special analytical capabilities and potential for multiplexing, this approach could contribute significantly to cell-signaling studies and to the development and implementation of personalized cancer therapies.
机译:磷酸肌醇3-激酶(P13K)/ Akt通路控制着许多正常的生理过程,并且经常在癌症中异常激活,因此将P13K / Akt信号转导成分鉴定为肿瘤学中有希望的药物靶标。但是,为此途径实施合理的癌症治疗需要强大而简单的工具,以根据P13K途径激活对患者进行分层,并验证和衡量靶向抑制对原发癌组织的影响。本文中,我们基于细胞裂解物中P13K依赖性蛋白激酶活性的质谱测量,提出了一种定量P13K / Akt信号通路的技术。 MS的这种应用的概念是利用酶活性来扩增所研究的酶的信号,类似于用于扩增核酸序列的PCR。我们表明,这种方法可以对细胞信号通路进行高灵敏度,定量精确和特异性的定量分析。由于其特殊的分析能力和潜在的多重性,这种方法可以极大地促进细胞信号研究以及个性化癌症治疗方法的开发和实施。

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