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铜胁迫下藻类 V-ATPase 大亚基 A(VHA-A)的动态 RNA 编辑事件的细胞内定位及诱导

Intracellular localization and induction of a dynamic RNA-editing event of macro-algal V-ATPase subunit A (VHA-A) in response to copper.

机构信息

School of Biosciences, Cardiff University, Cardiff, CF10 3AT, Wales, UK.

出版信息

Plant Cell Environ. 2014 Jan;37(1):189-203. doi: 10.1111/pce.12145. Epub 2013 Jun 30.

Abstract

A V-ATPase subunit A protein (VHA-A) transcript together with a variant (C793 to U), which introduces a stop codon truncating the subunit immediately downstream of its ATP binding site, was identified within a Fucus vesiculosus cDNA from a heavy metal contaminated site. This is intriguing because the VHA-A subunit is the crucial catalytic subunit responsible for the hydrolysis of ATP that drives ion transport underlying heavy metal detoxification pathways. We employed a chemiluminescent hybridization protection assay to quantify the proportion of both variants directly from mRNA while performing quantification of total transcript using Q-PCR. Polyclonal antisera raised against recombinant VHA-A facilitated simultaneous detection of parent and truncated VHA-A and revealed its cellular and subcellular localization. By exploiting laboratory exposures and samples from an environmental copper gradient, we showed that total VHA-A transcript and protein, together with levels of the truncated variant, were induced by copper. The absence of a genomic sequence representing the truncated variant suggests a RNA editing event causing the production of the truncated VHA-A. Based on these observations, we propose RNA editing as a novel molecular process underpinning VHA trafficking and intracellular sequestration of heavy metals under stress.

摘要

在一个来自重金属污染地区的泡叶藻 cDNA 中,鉴定到一种 V-ATPase 亚基 A 蛋白 (VHA-A) 的转录本,以及一种变体 (C793 突变为 U),该变体引入了一个终止密码子,从而截断了其 ATP 结合位点下游的亚基。这很有趣,因为 VHA-A 亚基是负责 ATP 水解的关键催化亚基,该水解反应驱动重金属解毒途径中的离子转运。我们采用化学发光杂交保护测定法,直接从 mRNA 中定量两种变体的比例,同时使用 Q-PCR 对总转录本进行定量。针对重组 VHA-A 制备的多克隆抗血清促进了亲本和截断的 VHA-A 的同时检测,并揭示了其细胞和亚细胞定位。通过利用实验室暴露和环境铜梯度的样本,我们表明,铜诱导了总 VHA-A 转录本和蛋白以及截断变体的水平。不存在代表截断变体的基因组序列表明发生了 RNA 编辑事件,导致产生截断的 VHA-A。基于这些观察结果,我们提出 RNA 编辑是一种新的分子过程,为应激下 VHA 转运和重金属的细胞内隔离提供了基础。

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