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A Novel Mitogen-Activated Protein Kinase Docking Site in the N Terminus of MEK5α Organizes the Components of the Extracellular Signal-Regulated Kinase 5 Signaling Pathway

机译:在MEK5αN总站的一个新的丝裂素活化蛋白激酶对接位点组织细胞外信号调节激酶5信号通路的组成部分。

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The alternative splicing of the mek5 gene gives rise to two isoforms. MEK5β lacks an extended N terminus present in MEK5α. Comparison of their activities led us to identify a novel mitogen-activated protein kinase (MAPK) docking site in the N terminus of MEK5α that is distinct from the consensus motif identified in the other MAPK kinases. It consists of a cluster of acidic residues at position 61 and positions 63 to 66. The formation of the MEK5/extracellular signal-regulated kinase 5 (ERK5) complex is critical for MEK5 to activate ERK5, to increase transcription via MEF2, and to enhance cellular survival in response to osmotic stress. Certain mutations in the ERK5 docking site that prevent MEK5/ERK5 interaction also abrogate the ability of MEKK2 to bind and activate MEK5. However, the identification of MEK5α mutants with selective binding defect demonstrates that the MEK5/ERK5 interaction does not rely on the binding of MEK5α to MEKK2 via their respective PB1 domains. Altogether these results establish that the N terminus of MEK5α is critical for the specific organization of the components of the ERK5 signaling pathway.
机译: mek5 基因的可变剪接产生两个同工型。 MEK5β缺少MEK5α中存在的扩展N末端。他们的活动比较导致我们在MEK5α的N末端鉴定了一个新的有丝分裂原活化蛋白激酶(MAPK)停靠位点,该位点不同于在其他MAPK激酶中鉴定出的共有基序。它由位于位置61和位置63至66的酸性残基簇组成。MEK5/细胞外信号调节激酶5(ERK5)复合物的形成对于MEK5激活ERK5,增加通过MEF2的转录并增强应对渗透胁迫的细胞存活。 ERK5停靠位点中某些阻止MEK5 / ERK5相互作用的突变也消除了MEKK2结合并激活MEK5的能力。然而,鉴定具有选择性结合缺陷的MEK5α突变体表明,MEK5 / ERK5相互作用不依赖于MEK5α通过其各自的PB1结构域与MEKK2的结合。总而言之,这些结果确定了MEK5α的N末端对于ERK5信号传导途径的组分的特定组织至关重要。

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