首页> 外文期刊>Journal of biomolecular screening: The official journal of the Society for Biomolecular Screening >Development of a novel ectonucleotidase assay suitable for high-throughput screening
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Development of a novel ectonucleotidase assay suitable for high-throughput screening

机译:适用于高通量筛选的新型外切核苷酸酶测定方法的开发

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5′-Ectonucleotidase (NT5E) catalyzes the conversion of adenosine monophosphate to adenosine and free phosphate. The role of this ectonucleotidase and its production of adenosine are linked with immune function, angiogenesis, and cancer. NT5E activity is typically assayed either by chromatographic quantification of substrates and products using high-performance liquid chromatography (HPLC) or by quantification of free phosphate using malachite green. These methods are not suitable for robust screening assays of NT5E activity. HPLC is not readily suitable for the rapid and efficient assay of multiple samples and malachite green is highly sensitive to the phosphate-containing buffers common in various media and sample buffers. Here the development and validation of a novel high-throughput ectonucleotidase screening assay are described, which makes use of a luciferase-based assay reagent, the Promega CellTiter-Glo kit, to measure the catabolism of AMP by NT5E. This multiwell plate-based assay facilitates the screening of potential ectonucleotidase antagonists and is unaffected by the presence of contaminating phosphate molecules present in screening samples.
机译:5'-核苷酸核酸酶(NT5E)催化单磷酸腺苷转化为腺苷和游离磷酸。这种外切核苷酸酶的作用及其腺苷的产生与免疫功能,血管生成和癌症有关。 NT5E活性通常通过使用高效液相色谱(HPLC)进行底物和产物的色谱定量或通过孔雀石绿对游离磷酸盐的定量来测定。这些方法不适用于NT5E活性的稳健筛选测定。 HPLC不适合用于快速高效地分析多个样品,而孔雀石绿对各种介质和样品缓冲液中常见的含磷酸盐的缓冲液高度敏感。这里描述了一种新型的高通量胞外核苷酸酶筛选测定法的开发和验证,该测定法利用了基于荧光素酶的测定试剂Promega CellTiter-Glo试剂盒来测定NT5E对AMP的分解代谢。这种基于多孔板的检测方法有助于筛选潜在的胞外核苷酸酶拮抗剂,并且不受筛选样品中存在的污染性磷酸盐分子的影响。

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