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Transportins 1 and 2 are redundant nuclear import factors for hnRNP A1 and HuR

机译:运输蛋白1和2是hnRNP A1和HuR的多余核输入因子

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Several mRNA-binding proteins, including hnRNP A1 and HuR, contain bidirectional transport signals that mediate both their nuclear import and export. Previously, Transportin 1 (Trn1) was identified as a mediator of hnRNP A1 import, whereas the closely related protein Transportin 2 (Trn2) was shown to interact with HuR. Here we have investigated the subfamily of transportins that consists of Trn1 (or Kap beta2A) and two alternatively spliced Trn2 isoforms (Trn2a and Trn2b), also called Trn2 and Kap beta2B. The sequence differences among these proteins could alter either their cargo specificity or their response to RanGTP and thus their function as import or export receptors. Using in vitro binding assays, we show that hnRNP A1 preferentially binds Trn1 and Trn2b versus Trn2a. HuR interacts with all three transportins, as well as weakly with Imp beta. The hnRNP A1 and HuR shuttling domains, called M9 and HNS, respectively, are sufficient for these interactions. Despite small differences in the binding of HuR and hnRNP A1 to the three transportins, in vitro interaction studies performed in the presence and absence of RanQ69LGTP indicate that all three transportins most likely act as import factors for HuR and hnRNP A1. In digitonin-permeabilized HeLa cells, both M9 and HNS peptides compete for the import of recombinant hnRNP A1 and HuR, indicating that HuR and hnRNP A1 import pathways are at least partially overlapping. Possible nucleocytoplasmic shuttling mechanisms for hnRNP A1 and HuR are discussed. [References: 44]
机译:几个mRNA结合蛋白,包括hnRNP A1和HuR,都包含双向转运信号,介导其核的进出口。以前,运输蛋白1(Trn1)被确定为hnRNP A1进口的媒介,而密切相关的蛋白运输蛋白2(Trn2)被证明与HuR相互作用。在这里,我们研究了运输蛋白亚家族,由Trn1(或Kap beta2A)和两个交替剪接的Trn2同工型(Trn2a和Trn2b)组成,也称为Trn2和Kap beta2B。这些蛋白质之间的序列差异可能会改变其货物特异性或对RanGTP的反应,从而改变其作为进口或出口受体的功能。使用体外结合试验,我们显示hnRNP A1相对于Trn2a优先结合Trn1和Trn2b。 HuR与所有三种转运蛋白相互作用,并且与Imp beta相互作用较弱。分别称为M9和HNS的hnRNP A1和HuR穿梭域足以进行这些相互作用。尽管HuR和hnRNP A1与三种转运蛋白的结合差异很小,但在存在和不存在RanQ69LGTP的情况下进行的体外相互作用研究表明,所有三种转运蛋白最有可能充当HuR和hnRNP A1的进口因子。在洋地黄素透化的HeLa细胞中,M9和HNS肽都竞争进口重组hnRNP A1和HuR的输入,这表明HuR和hnRNP A1的输入途径至少部分重叠。讨论了hnRNP A1和HuR可能的核质穿梭机制。 [参考:44]

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