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40LoVe interacts with Vg1RBP/Vera and hnRNP I in binding the Vg1-Localization Element

机译:40LoVe与Vg1RBP / Vera和hnRNP I相互作用,结合Vg1-Localization元素

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摘要

Localizing mRNAs within the cytoplasm gives cells the ability to spatially restrict protein production, a powerful means to regulate gene expression. Localized mRNA is often visible in microscopically observable particles or granules, and the association of mRNA localization with these structures is an indication that particles or granules may be essential to the localization process. Understanding how such structures form will therefore be important for understanding the function of localization RNPs (L-RNPs). We previously identified a novel component of an L-RNP from the Vg1 mRNA from Xenopus oocytes called 40LoVe. 40LoVe interaction with the Vg1-localization element (Vg1LE) was previously shown to be dependent on the VM1 and E2 sequence motifs within the Vg1LE that cross-link to hnRNP I and Vg1RBP/Vera, respectively. We report interaction of these motif-binding proteins with 40LoVe and identify a 40LoVe-Xenopus hnRNP D/AUF1 interaction. We further demonstrate that titration of VM1 and E2 motif binding activity in vivo surprisingly suggests that the motif binding proteins have differing roles during Vg1LE-dependent mRNA localization.
机译:在细胞质内定位mRNA使细胞能够在空间上限制蛋白质的产生,这是调节基因表达的有力手段。在显微镜下可观察到的颗粒或颗粒中通常可以看到局部的mRNA,并且mRNA的定位与这些结构的关联表明颗粒或颗粒对于定位过程必不可少。因此,了解这种结构的形成方式对于理解本地化RNP(L-RNP)的功能至关重要。我们先前从非洲爪蟾卵母细胞Vg1 mRNA中鉴定出一种L-RNP的新型成分,称为40LoVe。先前已显示与Vg1定位元件(Vg1LE)的40LoVe相互作用取决于Vg1LE中分别与hnRNP I和Vg1RBP / Vera交联的VM1和E2序列基序。我们报告这些动机结合蛋白与40LoVe的相互作用,并确定40LoVe-非洲爪蟾hnRNP D / AUF1相互作用。我们进一步证明,在体内对VM1和E2基序结合活性进行滴定令人惊讶地表明,在Vg1LE依赖性mRNA定位过程中,基序结合蛋白具有不同的作用。

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