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A new robust and nonradioactive approach for exploring N-myristoylation

机译:探索N-肉豆蔻酰化的一种新的健壮的非放射性的方法

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摘要

Myristoyl-CoA (CoA):protein N-myristoyltransferase (NMT) catalyzes protein modification through covalent attachment of a C14 fatty acid (myristic acid) to the N-terminal glycine of proteins, thus promoting protein-protein and protein-membrane interactions. NMT is essential for the viability of numerous human pathogens and is also up-regulated in several tumors. Here we describe a new, nonradioactive, ELISA-based method for measuring NMT activity. After the NMT-catalyzed reaction between a FLAG-tagged peptide and azido-dodecanoyl-CoA (analog of myristoyl-CoA), the resulting azido-dodecanoyl-peptide-FLAG was coupled to phosphine-biotin by Staudinger ligation, captured by plate-bound anti-FLAG antibodies and detected by streptavidin-peroxidase. The assay was validated with negative controls (including inhibitors), corroborated by HPLC analysis, and demonstrated to function with fresh or frozen tissues. Recombinant murine NMT1 and NMT2 were characterized using this new method. This versatile assay is applicable for exploring recombinant NMTs with regard to their activity, substrate specificity, and possible inhibitors as well as for measuring NMT-activity in tissues.
机译:肉豆蔻酰基辅酶A(CoA):蛋白质N-肉豆蔻酰基转移酶(NMT)通过C14脂肪酸(肉豆蔻酸)与蛋白质N端甘氨酸共价连接来催化蛋白质修饰,从而促进蛋白质-蛋白质和蛋白质-膜相互作用。 NMT对于许多人类病原体的生存至关重要,并且在几种肿瘤中也被上调。在这里,我们描述了一种新的非放射性,基于ELISA的方法来测量NMT活性。在FLAG标记的肽和叠氮基十二烷酰基-CoA(肉豆蔻酰基-CoA的类似物)之间的NMT催化反应后,所得的叠氮基十二烷酰基-肽-FLAG通过Staudinger连接与膦-生物素偶联,并通过板结合捕获抗FLAG抗体,并通过链霉亲和素过氧化物酶检测。该测定已通过阴性对照(包括抑制剂)进行了验证,并通过HPLC分析得到证实,并证明可与新鲜或冷冻组织一起发挥作用。重组鼠NMT1和NMT2使用此新方法进行了表征。这种多功能的测定方法可用于研究重组NMT的活性,底物特异性和可能的​​抑制剂,以及用于测量组织中的NMT活性。

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