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Comparison of mRNA localization and regulation during endoplasmic reticulum stress in Drosophila cells

机译:果蝇内质网应激过程中mRNA定位与调控的比较

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Ire1 is an endoplasmic reticulum (ER) transmembrane protein that senses disturbances in protein folding homeostasis and contributes to a multifaceted response to stress. The nuclease activity of Ire1, in addition to splicing the mRNA encoding the transcription factor Xbp1, mediates mRNA degradation in response to ER stress through a pathway termed regulated Ire1-dependent decay (RIDD). We previously showed that ER targeting of substrates is necessary for RIDD; in this paper, we show that ER localization is also sufficient to induce decay in a normally unaffected mRNA. Using microarrays, we also measured relative mRNA degradation in the presence and absence of ER stress in Drosophila S2 cells, and determined mRNA membrane association using detergent fractionation. The vast majority of mRNAs that were strongly associated with the ER were degraded faster during ER stress in an Ire1-dependent manner, suggesting that RIDD is the default pathway for ER-localized mRNAs during stress. We also show that the mRNA encoding plexin A remains highly polysome associated during stress and escapes degradation by RIDD, and that its 5′ untranslated region can protect a strong RIDD target from degradation. These results suggest that while translation is generally attenuated during ER stress, continued translation of certain messages can protect them from degradation by RIDD.
机译:Ire1是一种内质网(ER)跨膜蛋白,可感知蛋白折叠动态平衡的紊乱并有助于对压力的多方面反应。 Ire1的核酸酶活性,除了剪接编码转录因子Xbp1的mRNA外,还通过称为Ire1依赖性衰变(RIDD)的途径介导对ER应激的mRNA降解。我们之前表明,ERD对底物的靶向对于RIDD是必需的。在本文中,我们表明ER定位也足以诱导正常情况下不受影响的mRNA的衰变。使用微阵列,我们还测量了果蝇S2细胞中存在和不存在内质网应激时的相对mRNA降解,并使用去垢剂分馏确定了mRNA膜缔合。与ER紧密相关的绝大多数mRNA在ER应激过程中以Ire1依赖的方式降解得更快,这表明RIDD是应激过程中ER定位mRNA的默认途径。我们还显示编码plexin A的mRNA在压力下仍保持高度多聚体相关性,并逃脱了RIDD的降解,并且其5'非翻译区可以保护强大的RIDD目标免于降解。这些结果表明,虽然在ER压力下翻译通常会减弱,但是某些消息的继续翻译可以保护它们免受RIDD的降解。

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