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Unraveling self-assembly pathways of the 468-kDa proteolytic machine TET2

机译:揭示468 kDa蛋白水解机TET2的自组装途径

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The spontaneous formation of biological higher-order structures from smaller building blocks, called self-assembly, is a fundamental attribute of life. Although the protein self-assembly is a time-dependent process that occurs at the molecular level, its current understanding originates either from static structures of trapped intermediates or from modeling. Nuclear magnetic resonance (NMR) spectroscopy has the unique ability to monitor structural changes in real time; however, its size limitation and time-resolution constraints remain a challenge when studying the self-assembly of large biological particles. We report the application of methyl-specific isotopic labeling combined with relaxation-optimized NMR spectroscopy to overcome both size- and time-scale limitations. We report for the first time the self-assembly process of a half-megadalton protein complex that was monitored at the structural level, including the characterization of intermediate states, using a mutagenesis-free strategy. NMR was used to obtain individual kinetics data on the different transient intermediates and the formation of final native particle. In addition, complementary time-resolved electron microscopy and native mass spectrometry were used to characterize the low-resolution structures of oligomerization intermediates.
机译:由较小的构件自发形成生物高阶结构的过程称为自组装,是生命的基本属性。尽管蛋白质的自组装是在分子水平上发生的随时间变化的过程,但其目前的了解要么源自所捕获中间体的静态结构,要么源自建模。核磁共振(NMR)光谱具有实时监控结构变化的独特能力;然而,当研究大型生物颗粒的自组装时,其尺寸限制和时间分辨率限制仍然是一个挑战。我们报告了甲基特异性同位素标记结合弛豫优化的NMR光谱技术的应用,以克服尺寸和时间尺度的局限性。我们第一次报告了半兆道尔顿蛋白复合物的自组装过程,该过程使用无诱变策略在结构水平上进行了监测,包括中间状态的表征。 NMR用于获得有关不同瞬态中间体和最终天然颗粒形成的单个动力学数据。此外,互补的时间分辨电子显微镜和天然质谱用于表征低聚中间体的低分辨率结构。

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