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Kinetic determination of the GTPase activity of Ras proteins by means of a luminescent terbium complex

机译:通过发光ter络合物动力学测定Ras蛋白的GTPase活性

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Guanine nucleotide binding proteins, such as Ras proteins, play a pivotal role in maintaining the regular life cycle of cells. The involvement of Ras mutants in the progress of cancer has attracted many efforts to find detection methods for Ras activity. In this study we present a luminescent microwell plate assay for monitoring GTPase activity of Ras proteins. The luminescence intensity of the Tb–norfloxacin complex is influenced by nucleoside phosphates as well as by inorganic phosphates. Real-time kinetics of the GTPase activity of wild-type Ras and Ras mutants can be monitored online. The effect of a GTPase activating protein as well as of a downstream effector (Ras-binding domain of human Raf-1) on the GTPase activity of different Ras mutants is examined. In contrast to other methods, this assay does not require the use of radioactively labeled substrates or chromatographic separation steps. Moreover, the application of fluorescently labeled GTP substrates which often interfere with enzymatic activity can be avoided. This in vitro assay can serve as a model system for the screening of regulators affecting the GTPase activity of Ras proteins.
机译:鸟嘌呤核苷酸结合蛋白,例如Ras蛋白,在维持细胞正常生命周期中起着关键作用。 Ras突变体参与癌症的发展已经吸引了许多努力来寻找Ras活性的检测方法。在这项研究中,我们提出了一种发光微孔板测定法,用于监测Ras蛋白的GTPase活性。 Tb-诺氟沙星复合物的发光强度受核苷磷酸盐和无机磷酸盐的影响。可以在线监测野生型Ras和Ras突变体的GTPase活性的实时动力学。研究了GTPase活化蛋白以及下游效应子(人Raf-1的Ras结合域)对不同Ras突变体GTPase活性的影响。与其他方法相比,此测定法不需要使用放射性标记的底物或色谱分离步骤。而且,可以避免经常干扰酶活性的荧光标记的GTP底物的应用。这种体外测定可以用作筛选影响Ras蛋白GTPase活性的调节剂的模型系统。

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