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Ciliary entry of the kinesin-2 motor KIF17 is regulated by importin-beta2 and RanGTP

机译:驱动蛋白-2电机KIF17的睫状进入受importin-beta2和RanGTp调节

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摘要

The biogenesis, maintenance and function of primary cilia are controlled through intraflagellar transport (IFT) driven by two kinesin-2 family members, the heterotrimeric KIF3A/KIF3B/KAP complex and the homodimeric KIF17 motor. How these motors and their cargoes gain access to the ciliary compartment is poorly understood. Here, we identify a ciliary localization signal (CLS) in the KIF17 tail domain that is necessary and sufficient for ciliary targeting. Similarities between the CLS and classic nuclear localization signals (NLSs) suggest that similar mechanisms regulate nuclear and ciliary import. We hypothesize that ciliary targeting of KIF17 is regulated by a ciliary-cytoplasmic gradient of the small GTPase Ran, with high levels of GTP-bound Ran (RanGTP) in the cilium. Consistent with this, cytoplasmic expression of GTP-locked Ran(G19V) disrupts the gradient and abolishes ciliary entry of KIF17. Furthermore, KIF17 interacts with the nuclear import protein importin-beta2 in a manner dependent on the CLS and inhibited by RanGTP. We propose that Ran has a global role in regulating cellular compartmentalization by controlling the shuttling of cytoplasmic proteins into nuclear and ciliary compartments.
机译:原发纤毛的生物发生,维持和功能是由两个驱动蛋白2家族成员(异源三聚体KIF3A / KIF3B / KAP复合体和同二聚体KIF17马达)驱动的鞭毛内转运(IFT)控制的。这些电动机及其货物如何进入睫状体室了解甚少。在这里,我们确定在KIF17尾部域中的睫状定位信号(CLS)对于睫状靶向是必要和充分的。 CLS和经典核定位信号(NLS)之间的相似之处表明,类似的机制调节着核和纤毛的输入。我们假设KIF17的纤毛靶向受纤毛状小GTPase Ran的纤毛细胞质梯度调控,纤毛中GTP结合的Ran(RanGTP)含量高。与此相一致,GTP锁定Ran(G19V)的细胞质表达破坏了梯度并取消了KIF17的纤毛进入。此外,KIF17以依赖CLS并受RanGTP抑制的方式与核输入蛋白importin-beta2相互作用。我们建议冉通过控制细胞质蛋白穿梭入核和睫状区室在调节细胞区室化中具有全球性的作用。

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