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输出蛋白t的稳态核定位涉及RanGTP结合和两个不同的核孔复合体相互作用结构域。

Steady-state nuclear localization of exportin-t involves RanGTP binding and two distinct nuclear pore complex interaction domains.

作者信息

Kuersten Scott, Arts Gert-Jan, Walther Tobias C, Englmeier Ludwig, Mattaj Iain W

机构信息

Gene Expression Programme, European Molecular Biology Laboratory, D-69117 Heidelberg, Germany.

出版信息

Mol Cell Biol. 2002 Aug;22(16):5708-20. doi: 10.1128/MCB.22.16.5708-5720.2002.

Abstract

Vertebrate tRNA export receptor exportin-t (Xpo-t) binds to RanGTP and mature tRNAs cooperatively to form a nuclear export complex. Xpo-t shuttles bidirectionally through nuclear pore complexes (NPCs) but is mainly nuclear at steady state. The steady-state distribution of Xpo-t is shown to depend on its interaction with RanGTP. Two distinct Xpo-t NPC interaction domains that bind differentially to peripherally localized nucleoporins in vitro are identified. The N terminus binds to both Nup153 and RanBP2/Nup358 in a RanGTP-dependent manner, while the C terminus binds to CAN/Nup214 independently of Ran. We propose that these interactions increase the concentration of tRNA export complexes and of empty Xpo-t in the vicinity of NPCs and thus increase the efficiency of the Xpo-t transport cycle.

摘要

脊椎动物的tRNA输出受体输出蛋白t(Xpo-t)与RanGTP和成熟tRNA协同结合,形成核输出复合物。Xpo-t通过核孔复合体(NPC)进行双向穿梭,但在稳态时主要位于细胞核内。研究表明,Xpo-t的稳态分布取决于其与RanGTP的相互作用。已鉴定出两个不同的Xpo-t NPC相互作用结构域,它们在体外与外周定位的核孔蛋白的结合方式不同。N端以RanGTP依赖的方式与Nup153和RanBP2/Nup358结合,而C端独立于Ran与CAN/Nup214结合。我们认为,这些相互作用增加了NPC附近tRNA输出复合物和空载Xpo-t的浓度,从而提高了Xpo-t运输循环的效率。

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