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Nuclear Import of Zinc Binuclear Cluster Proteins Proceeds through Multiple, Overlapping Transport Pathways

机译:锌双核簇蛋白的核输入通过多种重叠的运输途径进行。

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In Aspergillus nidulans, the high transcriptional level of the ethanol utilization pathway genes (alc) is regulated by the specific activator AlcR. Here we have analyzed the mechanism of the nuclear import of AlcR, as well as that of other proteins belonging to the Zn2Cys6 binuclear cluster family. The nuclear localization signal of AlcR maps within the N-terminal 75 amino acid residues and overlaps with its DNA-binding domain. It consists of five clusters rich in basic residues. Four of them are necessary and sufficient for nuclear targeting. The first two basic regions are crucial for both nuclear localization and recognition of AlcR-specific DNA targets. This nuclear localization signal (NLS) motif is recognized by the nuclear transport machinery of Saccharomyces cerevisiae and requires both Ran/Gsp1p activity and specific transport receptors. AlcR can be imported into nuclei via multiple transport pathways mediated by a distinct set of karyopherins composed of Kap104p, Sxm1p, and Nmd5p transport receptors. The two former karyopherins interact with the NLS of AlcR directly. Other Zn binuclear cluster proteins from S. cerevisiae, such as Gal4p and Pdr3p, also appear to be transported to the nuclei in a nonclassical, importin-α-independent manner and can share common importin β receptors.
机译:构巢曲霉中,乙醇利用途径基因( alc )的高转录水平受特定激活因子AlcR调控。在这里,我们分析了AlcR以及其他Zn 2 Cys 6 双核簇家族蛋白的核输入机制。 AlcR的核定位信号在N末端75个氨基酸残基内定位,并与其DNA结合结构域重叠。它由五个富含基本残基的簇组成。其中四个对于核目标是必要和充分的。前两个基本区域对于核定位和AlcR特异性DNA靶标的识别都至关重要。酿酒酵母(Saccharomyces cerevisiae)的核转运机制可以识别这种核定位信号(NLS)基序,它既需要Ran / Gsp1p活性,又需要特定的转运受体。 AlcR可以通过由Kap104p,Sxm1p和Nmd5p转运受体组成的一组独特的核蛋白介导的多种转运途径导入细胞核。前两个核蛋白直接与AlcR的NLS相互作用。来自 S的其他Zn双核簇蛋白。酿酒酵母,例如Gal4p和Pdr3p,也似乎以非经典的,不依赖importin-α的方式转运至细胞核,并且可以共享常见的importinβ受体。

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