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Multiple pathways regulate intracellular shuttling of MoKA, a co-activator of transcription factor KLF7

机译:多种途径可调节MoKA(转录因子KLF7的共激活物)的细胞内穿梭运动

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摘要

MoKA is a novel F-box containing protein that interacts with and stimulates the activity of transcription factor KLF7, a regulator of neuronal differentiation. MoKA accumulates throughout the cell and predominantly in the cytosol, consistent with the presence of several putative nuclear localization and export signals (NLSs and NESs). The present study was designed to refine the identity and location of the sequences responsible for MoKA intracellular shuttling and transcriptional activity. Forced expression of fusion proteins in mammalian cells demonstrated that only one of three putative NLSs potentially recognized by karyopherin receptors is involved in nuclear localization of MoKA. By contrast, three distinct sequences were found to participate in mediating cytoplasmic accumulation. One of them is structurally and functionally related to the leucine-rich export signal that interacts with the exportin 1 (CRM1) receptor. The other two export signals instead display either a novel leucine-rich sequence or an undefined peptide motif, and both appear to act through CRM1-independent pathways. Finally, transcriptional analyses using the chimeric GAL4 system mapped the major activation domain of MoKA to a highly acidic sequence that resides between the NLS and NES clusters.
机译:MoKA是一种新型的F盒蛋白,它与神经元分化的调节因子转录因子KLF7相互作用并刺激其活动。 MoKA会在整个细胞中积累,并主要在胞质溶胶中积累,这与几种假定的核定位和输出信号(NLS和NES)的存在相一致。本研究旨在完善负责MoKA细胞内穿梭和转录活性的序列的身份和位置。融合蛋白在哺乳动物细胞中的强迫表达表明,可能被核卵磷脂受体识别的三种推定的NLS中只有一种与MoKA的核定位有关。相比之下,发现三个不同的序列参与介导细胞质积累。其中之一与与出口蛋白1(CRM1)受体相互作用的富含亮氨酸的出口信号在结构和功能上相关。相反,其他两个输出信号显示新的富含亮氨酸的序列或未定义的肽基序,并且两者似乎都通过不依赖CRM1的途径起作用。最后,使用嵌合GAL4系统进行的转录分析将MoKA的主要激活域映射到位于NLS和NES簇之间的高酸性序列。

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