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Optimizing the protein switch: altering nuclear import and export signals and ligand binding domain

机译:优化蛋白质转换:改变核的进出口信号和配体结合结构域

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摘要

Ligand regulated localization controllable protein constructs were optimized in this study. Several constructs were made from a classical nuclear export signal (HIV-rev, MAPKK, or progesterone receptor) in combination with a SV40 T-antigen type nuclear import signal. Different ligand binding domains (LBDs from glucocorticoid receptor or progesterone receptor) were also tested for their ability to impart control over localization of proteins. This study was designed to create constructs which are cytoplasmic in the absence of ligand and nuclear in the presence of ligand, and also to regulate the amount of protein translocating to the nucleus on ligand induction. The balance between the strengths of import and export signals was critical for overall localization of proteins. The amount of protein entering the nucleus was also affected by the dose of ligand (10-100nM). However, the overall import characteristics were determined by the strengths of localization signals and the inherent localization properties of the LBD used. This study established that the amount of protein present in a particular compartment can be regulated by the use of localization signals of various strengths. These optimized localization controllable protein constructs can be used to correct for diseases due to aberrant localization of proteins.
机译:在这项研究中优化了配体调控的定位可控蛋白构建体。由经典的核输出信号(HIV-rev,MAPKK或孕激素受体)与SV40 T抗原型核输入信号结合制成了几种构建体。还测试了不同的配体结合域(来自糖皮质激素受体或孕激素受体的LBD)赋予蛋白质定位控制的能力。设计该研究的目的是创建在不存在配体的情况下为细胞质而在存在配体的情况下为核的构建体,并在配体诱导时调节转运到细胞核的蛋白质的量。进出口信号强度之间的平衡对于蛋白质的整体定位至关重要。进入细胞核的蛋白质量也受到配体剂量(10-100nM)的影响。但是,总体进口特征取决于定位信号的强度和所使用的LBD的固有定位特性。这项研究表明,可以通过使用各种强度的定位信号来调节特定隔室中存在的蛋白质量。这些优化的定位可控蛋白质构建体可用于纠正由于蛋白质异常定位引起的疾病。

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