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Targeted proteomics reveals compositional dynamics of 60S pre-ribosomes after nuclear export

机译:靶向蛋白质组学揭示核输出后60S前核糖体的组成动态

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摘要

Construction and intracellular targeting of eukaryotic pre-ribosomal particles involve a multitude of diverse transiently associating trans-acting assembly factors, energy-consuming enzymes, and transport factors. The ability to rapidly and reliably measure co-enrichment of multiple factors with maturing pre-ribosomal particles presents a major biochemical bottleneck towards revealing their function and the precise contribution of >50 energy-consuming steps that drive ribosome assembly. Here, we devised a workflow that combines genetic trapping, affinity-capture, and selected reaction monitoring mass spectrometry (SRM-MS), to overcome this deficiency. We exploited this approach to interrogate the dynamic proteome of pre-60S particles after nuclear export. We uncovered assembly factors that travel with pre-60S particles to the cytoplasm, where they are released before initiating translation. Notably, we identified a novel shuttling factor that facilitates nuclear export of pre-60S particles. Capturing and quantitating protein interaction networks of trapped intermediates of macromolecular complexes by our workflow is a reliable discovery tool to unveil dynamic processes that contribute to their in vivo assembly and transport.
机译:真核生物核糖体前颗粒的构建和细胞内靶向涉及多种多样的瞬时关联反式组装因子,耗能酶和转运因子。快速和可靠地测量多个因素与成熟的核糖体颗粒共同富集的能力,对于揭示其功能以及驱动核糖体装配的> 50个耗能步骤的精确贡献,是一个主要的生化瓶颈。在这里,我们设计了一个工作流程,将遗传捕获,亲和捕获和选定的反应监测质谱(SRM-MS)相结合,以克服这一缺陷。我们利用这种方法来询问核输出后60S以前的粒子的动态蛋白质组。我们发现了与60S以前的颗粒一起进入细胞质的组装因子,在启动翻译之前将其释放。值得注意的是,我们确定了一种新的穿梭因子,可促进60S之前颗粒的核出口。通过我们的工作流程捕获和定量捕获的大分子复合物中间体的蛋白质相互作用网络是一种可靠的发现工具,可揭示有助于其体内组装和运输的动态过程。

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