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Golgi export of the Kir2.1 channel is driven by a trafficking signal located within its tertiary structure

机译:高尔基(Kir2.1)通道的出口受到位于其三级结构内的贩运信号的驱动

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摘要

Mechanisms that are responsible for sorting newly synthesized proteins for traffic to the cell surface from the Golgi are poorly understood. Here, we show that the potassium channel Kir2.1, mutations in which are associated with Andersen-Tawil syndrome, is selected as cargo into Golgi export carriers in an unusual signal-dependent manner. Unlike conventional trafficking signals, which are typically comprised of short linear peptide sequences, Golgi exit of Kir2.1 is dictated by residues that are embedded within the confluence of two separate domains. This signal patch forms a recognition site for interaction with the AP1 adaptor complex, thereby marking Kir2.1 for incorporation into clathrin-coated vesicles at the trans-Golgi. The identification of a trafficking signal in the tertiary structure of Kir2.1 reveals a quality control step that couples protein conformation to Golgi export and provides molecular insight into how mutations in Kir2.1 arrest the channels at the Golgi.
机译:人们对负责对新合成的蛋白质进行分类的机制了解甚少,这些蛋白质用于从高尔基体运输到细胞表面。在这里,我们表明钾通道Kir2.1,其中与安徒生-塔维尔综合症相关的突变,被选择作为货物以一种不寻常的信号依赖方式送入高尔基岛出口载体。与通常由短线性肽序列组成的常规运输信号不同,Kir2.1的高尔基体出口由嵌入两个独立结构域汇合的残基决定。该信号补丁形成一个识别位点,用于与AP1接头复合体相互作用,从而标记Kir2.1并入反式高尔基体的网格蛋白涂层囊泡中。在Kir2.1的三级结构中识别出一个运输信号,揭示了一个质量控制步骤,该步骤将蛋白质构象与高尔基体输出耦合,并提供了分子洞察力,以了解Kir2.1中的突变如何阻止高尔基体中的通道。

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