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A light-inducible organelle-targeting system for dynamically activating and inactivating signaling in budding yeast

机译:光诱导细胞器靶向系统用于动态激活和失活酵母中的信号传导

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摘要

Protein localization plays a central role in cell biology. Although powerful tools exist to assay the spatial and temporal dynamics of proteins in living cells, our ability to control these dynamics has been much more limited. We previously used the phytochrome B– phytochrome-interacting factor light-gated dimerization system to recruit proteins to the plasma membrane, enabling us to control the activation of intracellular signals in mammalian cells. Here we extend this approach to achieve rapid, reversible, and titratable control of protein localization for eight different organelles/positions in budding yeast. By tagging genes at the endogenous locus, we can recruit proteins to or away from their normal sites of action. This system provides a general strategy for dynamically activating or inactivating proteins of interest by controlling their localization and therefore their availability to binding partners and substrates, as we demonstrate for galactose signaling. More importantly, the temporal and spatial precision of the system make it possible to identify when and where a given protein's activity is necessary for function, as we demonstrate for the mitotic cyclin Clb2 in nuclear fission and spindle stabilization. Our light-inducible organelle-targeting system represents a powerful approach for achieving a better understanding of complex biological systems.
机译:蛋白质定位在细胞生物学中起着核心作用。尽管存在强大的工具来分析活细胞中蛋白质的时空动态,但是我们控制这些动态的能力却受到很大限制。我们以前使用植物色素B–植物色素相互作用因子光门二聚系统将蛋白募集到质膜上,从而使我们能够控制哺乳动物细胞内细胞内信号的激活。在这里,我们扩展了该方法,以实现快速,可逆和可滴定控制萌芽酵母中八个不同细胞器/位置的蛋白质定位。通过在内源基因座处标记基因,我们可以募集蛋白质至其正常作用位点或远离其正常作用位点。该系统提供了一种一般策略,可通过控制目标蛋白的定位并因此控制其对结合配偶体和底物的可用性来动态激活或失活目标蛋白,正如我们对半乳糖信号传导所证明的那样。更重要的是,系统的时间和空间精度使我们有可能确定何时以及何地需要给定蛋白质的功能来发挥功能,正如我们在核裂变和纺锤体稳定中证明有丝分裂细胞周期蛋白Clb2所证明的那样。我们的光诱导细胞器靶向系统代表了一种强大的方法,可以更好地了解复杂的生物系统。

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