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Exposure of bipartite hydrophobic signal triggers nuclear quality control of Ndc10 at the endoplasmic reticulumuclear envelope

机译:双向疏水信号的暴露触发内质网/核包膜的Ndc10核质量控制

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摘要

Proper functioning of the protein-folding quality control network depends on the network's ability to discern diverse structural perturbations to the native states of its protein substrates. Despite the centrality of the detection of misfolded states to cell home­ostasis, very little is known about the exact sequence and structural features that mark a protein as being misfolded. To investigate these features, we studied the requirements for the degradation of the yeast kinetochore protein Ndc10p. Mutant Ndc10p is a substrate of a protein-folding quality control pathway mediated by the E3 ubiquitin (Ub) ligase Doa10p at the endoplasmic reticulum (ER)uclear envelope membrane. Analysis of Ndc10p mutant derivatives, employing a reverse genetics approach, identified an autonomous quality control–associated degradation motif near the C-terminus of the protein. This motif is composed of two indispensable hydrophobic elements: a hydrophobic surface of an amphipathic helix and a loosely structured hydrophobic C-terminal tail. Site-specific point mutations expose these elements, triggering ubiquitin-mediated and HSP70 chaperone–dependent degradation of Ndc10p. These findings substantiate the ability of the ER quality control system to recognize subtle perturbation(s) in the native structure of a nuclear protein.
机译:蛋白质折叠质量控制网络的正常运行取决于该网络识别其蛋白质底物天然状态的各种结构扰动的能力。尽管检测错误折叠状态对细胞稳态具有重要意义,但对于将蛋白质标记为错误折叠的确切序列和结构特征了解甚少。为了研究这些特征,我们研究了降解酵母动核蛋白Ndc10p的要求。 Ndc10p突变体是内质网(ER)/核包膜上的E3泛素(Ub)连接酶Doa10p介导的蛋白质折叠质量控制途径的底物。 Ndc10p突变体衍生物的分析,采用反向遗传学方法,在蛋白质C末端附近发现了一个与质量控制相关的自主降解基序。该基序由两个必不可少的疏水元素组成:两亲螺旋的疏水表面和结构松散的疏水C末端尾巴。位点特异性点突变暴露了这些元素,从而触发了泛素介导的和HSP70伴侣依赖性的Ndc10p降解。这些发现证实了ER质量控制系统识别核蛋白天然结构中细微扰动的能力。

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