首页> 外文期刊>Journal of enzyme inhibition and medicinal chemistry. >Microplate-based method to screen inhibitors of isozymes of cyclic nucleotide phosphodiesterase fused to SUMO
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Microplate-based method to screen inhibitors of isozymes of cyclic nucleotide phosphodiesterase fused to SUMO

机译:基于微孔板的方法筛选与SUMO融合的环状核苷酸磷酸二酯酶同工酶抑制剂

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The feasibility for microplate-based screening of inhibitors of isozymes of cyclic nucleotide phosphodiesterase (PDE) was tested via the coupled action of a phosphatase on adenosine-5′-monophosphate and an improved malachite green assay of phosphate. Human full-length PDE4B2 and truncated mutant (152–528aa) were expressed in Escherichia coli via fusion to SUMO, which after purification through Ni-NTA column exhibited specific activities >0.017?U?mg?1. In the presence of proteins ?1, absorbance for 10?μΜ phosphate was measurable; a PDE isozyme of specific activity over 0.008?U?mg?1 after reaction for 20?min thus suited for microplate-based screening of inhibitors. By using Biotek ELX 800 microplate reader, affinities of two forms of PEDE4B2 for cAMP, rolipram and papaverine varied over three magnitudes and were consistent with those by routine assay, respectively. Hence, the proposed method was promising for high-throughput-screening of inhibitors of phosphate-releasing enzymes bearing specific activities over 0.008?U?mg?1.
机译:通过磷酸酶对5'-腺苷单磷酸的偶联作用和改进的孔雀绿磷酸盐检测法,测试了基于微孔板筛选环状核苷酸磷酸二酯酶(PDE)同工酶抑制剂的可行性。人全长PDE4B2和截短的突变体(152-528aa)通过与SUMO融合在大肠杆菌中表达,通过Ni-NTA柱纯化​​后,其比活度> 0.017?U?mg ?1 。在存在蛋白质α1的情况下,可测量10μμM磷酸盐的吸光度。反应20?min后,比活度超过0.008?U?mg ?1 的PDE同工酶适用于基于微孔板的抑制剂筛选。通过使用Biotek ELX 800酶标仪,两种形式的PEDE4B2对cAMP,咯利普兰和罂粟碱的亲和力在三个数量级上变化,并且分别与常规测定的亲和力一致。因此,该方法有望用于高通量筛选比活度超过0.008?U?mg ?1 的磷酸释放酶抑制剂。

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