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LaF3 nanoparticle-assisted sensitive detection of protein kinase activity

机译:LaF3纳米粒子辅助检测蛋白激酶活性

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摘要

A fluorescent protein kinase assay is developed based on the selective recognition ability of LaF3 nanoparticles (LaF3 NPs) towards a phosphorylated peptide substrate. In this study, protein kinase can catalyze the phosphorylation of the fluorescently labeled substrate peptide, which may then bind specifically on the surface of LaF3 NPs through the strong interaction between La~(3+) and the phosphate group while the unphosphorylated peptide will not. Therefore, fluorescent phosphopeptides are enriched on the LaF3 NP surfaces in correlation with the kinase activity. After isolation of the unbound peptides via centrifugation, the fluorophore-anchored LaF3 NPs can be easily re-dispersed in aqueous buffer to form a stable colloid solution. By monitoring the fluorescence signal of such colloid solution, the activity of protein kinase A (PKA), a proof-of-concept protein kinase, can be easily determined from 0.0006 U μL~(-1) to 0.2 U uL~(-1) with a detection limit of 0.0002 U μL~(-1). By combining with the synchronous fluorescence technique, the proposed assay is feasible for simultaneous detection of multiple protein kinases. Furthermore, this simple method is also successfully applied to the PKA inhibition assay, showing great potential in the study of cellular signal transduction and drug discovery.
机译:基于LaF3纳米颗粒(LaF3 NPs)对磷酸化肽底物的选择性识别能力,开发了一种荧光蛋白激酶测定法。在这项研究中,蛋白激酶可以催化荧光标记的底物肽的磷酸化,然后可以通过La〜(3+)与磷酸基团之间的强相互作用特异性地结合在LaF3 NP的表面上,而未磷酸化的肽则不会。因此,与激酶活性相关,荧光磷酸肽富集在LaF3 NP表面上。通过离心分离未结合的肽后,荧光团锚定的LaF3 NP可以轻松地重新分散在水性缓冲液中以形成稳定的胶体溶液。通过监测这种胶体溶液的荧光信号,可以很容易地从0.0006 UμL〜(-1)到0.2 U uL〜(-1)确定蛋白激酶A(PKA)的活性,这是一种概念验证蛋白激酶。的检测限为0.0002 UμL〜(-1)。通过与同步荧光技术结合,所提出的测定法对于同时检测多种蛋白激酶是可行的。此外,这种简单的方法也成功地应用于PKA抑制测定,在细胞信号转导和药物发现的研究中显示出巨大的潜力。

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