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一种基于荧光寿命的阿贝尔森激酶检测方法。

A fluorescence lifetime-based assay for abelson kinase.

作者信息

Pritz Stephan, Meder Gabriele, Doering Klaus, Drueckes Peter, Woelcke Julian, Mayr Lorenz M, Hassiepen Ulrich

机构信息

Biosyntan GmbH, Berlin, Germany.

出版信息

J Biomol Screen. 2011 Jan;16(1):65-72. doi: 10.1177/1087057110385817. Epub 2010 Dec 8.

Abstract

We present a novel homogeneous in vitro assay format and apply it to the quantitative determination of the enzymatic activity of a tyrosine kinase. The assay employs a short peptidic substrate containing a single tyrosine and a single probe attached via a cysteine side chain. The structural flexibility of the peptide allows for the dynamic quenching of the probe by the nonphosphorylated tyrosine side chain. The probe responds with changes in its fluorescence lifetime depending on the phosphorylation state of the tyrosine. We use this effect to directly follow the enzymatic phosphorylation of the substrate, without having to resort to additional assay components such as an antibody against the phosphotyrosine. As an example for the application of this assay principle, we present results from the development of an assay for Abelson kinase (c-Abl) used for compound profiling. Adjustments in the peptide sequence would make this assay format suitable to a wide variety of other tyrosine kinases.

摘要

我们提出了一种新型的均相体外检测方法,并将其应用于酪氨酸激酶酶活性的定量测定。该检测方法采用一种短肽底物,其含有一个酪氨酸和一个通过半胱氨酸侧链连接的单一探针。肽的结构灵活性允许未磷酸化的酪氨酸侧链对探针进行动态猝灭。探针对其荧光寿命的变化做出响应,这取决于酪氨酸的磷酸化状态。我们利用这一效应直接跟踪底物的酶促磷酸化过程,而无需借助诸如抗磷酸酪氨酸抗体等额外的检测成分。作为该检测原理应用的一个例子,我们展示了用于化合物谱分析的阿贝尔森激酶(c-Abl)检测方法开发的结果。对肽序列的调整将使这种检测方法适用于多种其他酪氨酸激酶。

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