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A comprehensive platform for the analysis of ubiquitin-like protein modifications using in vivo biotinylation

机译:使用体内生物素化分析泛素样蛋白质修饰的综合平台

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Post-translational modification by ubiquitin and ubiquitin-like proteins (UbLs) is fundamental for maintaining protein homeostasis. Efficient isolation of UbL conjugates is hampered by multiple factors, including cost and specificity of reagents, removal of UbLs by proteases, distinguishing UbL conjugates from interactors, and low quantities of modified substrates. Here we describe bioUbLs, a comprehensive set of tools for studying modifications in Drosophila and mammals, based on multicistronic expression and in vivo biotinylation using the E. coli biotin protein ligase BirA. While the bioUbLs allow rapid validation of UbL conjugation for exogenous or endogenous proteins, the single vector approach can facilitate biotinylation of most proteins of interest. Purification under denaturing conditions inactivates deconjugating enzymes and stringent washes remove UbL interactors and non-specific background. We demonstrate the utility of the method in Drosophila cells and transgenic flies, identifying an extensive set of putative SUMOylated proteins in both cases. For mammalian cells, we show conjugation and localization for many different UbLs, with the identification of novel potential substrates for UFM1. Ease of use and the flexibility to modify existing vectors will make the bioUbL system a powerful complement to existing strategies for studying this important mode of protein regulation.
机译:通过泛素和泛素样蛋白(UBLS)的翻译后修饰是维持蛋白质稳态的基础。 UBL缀合物的有效分离受到多种因素的阻碍,包括试剂的成本和特异性,通过蛋白酶去除UBLS,从交流器中区分UBL缀合物,以及低量的改性基板。在这里,我们描述了一套全面的一组工具,用于研究果蝇和哺乳动物的修饰,基于多时钟表达和使用大肠杆菌生物素蛋白连接酶Bira的体内生物素化。虽然BioubLs允许快速验证外源或内源蛋白的UBL缀合,但单载体方法可以促进大多数感兴趣的蛋白质的生物素化。在变性条件下纯化灭活去杂交酶和严格的洗涤去除UBL交互式和非特异性背景。我们证明了果蝇细胞和转基因苍蝇中该方法的效用,在这两种情况下识别出广泛推定的雄性蛋白质。对于哺乳动物细胞,我们对许多不同的UBL表示缀合和定位,具有用于UFM1的新型潜在基材。易于使用和改变现有载体的灵活性将使BioubL系统成为研究这种重要蛋白质调节模式的现有策略的强大补充。

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