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Identifying post-translational modifications of NEMO by tandem mass spectrometry after high affinity purification

机译:高亲和力纯化后通过串联质谱鉴定NEMO的翻译后修饰

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摘要

An integral component of NF-κB signalling is NEMO, NF-κB essential modulator, a regulatory protein of the IκB kinase (IKK) complex. Post-translational modifications of NEMO, including phosphorylation, SUMOylation, and ubiquitination are critical events during stimuli induced NF-κB activation. Here we demonstrate a method to detect post-translational modifications of NEMO using cells stably expressing polyhistidine tagged NEMO which allows for high-affinity purification of NEMO following rapid denaturing lysis and characterization by MS/MS. We identified a previously uncharacterized basal phosphorylation of NEMO at Serine 387 and tested the biological significance of this phosphorylation through a somatic genetic complementation analysis using the NEMO mutants S387A, S388D, and P388I in 1.3E2 NEMO-deficient murine pre-B cells. NF-κB signalling induced by bacterial lipopolysaccharide, Interleukin-1ß or the DNA damaging agent etoposide was not perturbed by these mutations of NEMO. Thus, S387 phosphorylation of NEMO is not a general requirement to mediate efficient NF-κB signalling and therefore may have cell type and/or stimulus-specific activity in vivo.
机译:NF-κB信号的组成部分是NEMO,NF-κB必需的调节剂,IκB激酶(IKK)复合物的调节蛋白。 NEMO的翻译后修饰(包括磷酸化,SUMO酰化和泛素化)是刺激诱导的NF-κB活化过程中的关键事件。在这里,我们展示了一种使用稳定表达多组氨酸标记的NEMO的细胞检测NEMO的翻译后修饰的方法,该方法可在MS / MS快速变性裂解和表征后实现NEMO的高亲和力纯化。我们鉴定出丝氨酸387处NEMO先前未鉴定的基础磷酸化,并通过在1.3E2 NEMO缺陷型鼠前B细胞中使用NEMO突变体S387A,S388D和P388I进行体细胞遗传互补分析,测试了该磷酸化的生物学意义。 NEMO的这些突变不会干扰细菌脂多糖,白介素-1ß或DNA破坏剂依托泊苷诱导的NF-κB信号传导。因此,NEMO的S387磷酸化不是介导有效NF-κB信号传导的一般要求,因此在体内可能具有细胞类型和/或刺激特异性活性。

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