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A microscopy-based screen employing multiplex genome sequencing identifies cargo-specific requirements for dynein velocity

机译:基于显微镜的屏幕,采用多重基因组测序,可确定货物对达因速度的特定要求

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The timely delivery of membranous organelles and macromolecules to specific locations within the majority of eukaryotic cells depends on microtubule-based transport. Here we describe a screening method to identify mutations that have a critical effect on intracellular transport and its regulation using mutagenesis, multicolor-fluorescence microscopy, and multiplex genome sequencing. This screen exploits the filamentous fungus Aspergillus nidulans , which has many of the advantages of yeast molecular genetics but uses long-range microtubule-based transport in a manner more similar to metazoan cells. Using this method, we identified seven mutants that represent novel alleles of components of the intracellular transport machinery: specifically, kinesin-1, cytoplasmic dynein, and the dynein regulators Lis1 and dynactin. The two dynein mutations identified in our screen map to dynein's AAA+ catalytic core. Single-molecule studies reveal that both mutations reduce dynein's velocity in vitro. In vivo these mutants severely impair the distribution and velocity of endosomes, a known dynein cargo. In contrast, another dynein cargo, the nucleus, is positioned normally in these mutants. These results reveal that different dynein functions have distinct stringencies for motor performance.
机译:将膜细胞器和大分子及时递送到大多数真核细胞内的特定位置取决于基于微管的转运。在这里,我们描述了一种筛选方法,以使用诱变,多色荧光显微镜和多重基因组测序来鉴定对细胞内运输及其调控具有关键作用的突变。该筛选利用丝状真菌构巢曲霉(Aspergillus nidulans),它具有酵母分子遗传学的许多优势,但以与子生细胞更相似的方式使用基于微管的远程运输。使用这种方法,我们确定了七个代表细胞内转运机制成分的新等位基因的突变体:具体而言,驱动蛋白1,胞质动力蛋白和动力蛋白调节剂Lis1和动力蛋白。在我们的筛选中鉴定出的两个动力蛋白突变映射到动力蛋白的AAA +催化核心。单分子研究表明,这两种突变都会降低体外动力蛋白的速度。在体内,这些突变体严重损害了内体(一种已知的动力蛋白)的分布和速度。相比之下,另一种动力蛋白的核心,通常位于这些突变体中。这些结果表明,不同的达因功能对电机性能具有不同的严格性。

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