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A single promoter system co-expressing RNA sensor with fluorescent proteins for quantitative mRNA imaging in living tumor cells

机译:单启动子系统与荧光蛋白共表达RNA传感器用于在活体肿瘤细胞中定量mRNA成像

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摘要

Genetically encoded light-up RNA aptamers afford a valuable platform for developing RNA sensors toward live cell imaging. However, quantitative imaging of intracellular RNAs remains a grand challenge. Here we reported a novel genetically encoded RNA sensor strategy using a plasmid that expresses a splittable fusion of the RNA sensor and the GFP mRNA in an individual transcript using a single promoter system. This splittable fusion design enables synchronous co-expression of the RNA sensor with GFP mRNA while alleviates the interference with correct folding of RNA aptamers due to intramolecular hybridization. This single-promoter system is applied to ratiometric imaging of survivin mRNA in tumor cells. The results reveal that the ratiometric images dynamically correlated with survivin mRNA concentrations and allow quantitative imaging of survivin mRNA in different tumor cells. The RNA sensor strategy may provide a new paradigm for developing a robust imaging platform for quantitative mRNA studies in living cells.
机译:遗传编码的点亮RNA适体为开发用于活细胞成像的RNA传感器提供了宝贵的平台。然而,细胞内RNA的定量成像仍然是一个巨大的挑战。在这里,我们报告了一种新的遗传编码的RNA传感器策略,该策略使用的质粒使用单个启动子系统在单个转录物中表达RNA传感器和GFP mRNA的可拆分融合。这种可拆分融合设计使RNA传感器与GFP mRNA同步共表达,同时减轻了由于分子内杂交对RNA适体正确折叠的干扰。该单启动子系统应用于肿瘤细胞中survivin mRNA的比例成像。结果显示,比例图像与survivin mRNA浓度动态相关,并可以对不同肿瘤细胞中survivin mRNA进行定量成像。 RNA传感器策略可能为开发用于活细胞定量mRNA研究的强大成像平台提供新的范例。

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