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A general approach to high-yield biosynthesis of chimeric RNAs bearing various types of functional small RNAs for broad applications

机译:带有各种功能的小RNA的嵌合RNA高产量生物合成的通用方法

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RNA research and therapy relies primarily on synthetic RNAs. We employed recombinant RNA technology toward large-scale production of pre-miRNA agents in bacteria, but found the majority of target RNAs were not or negligibly expressed. We thus developed a novel strategy to achieve consistent high-yield biosynthesis of chimeric RNAs carrying various small RNAs (e.g. miRNAs, siRNAs and RNA aptamers), which was based upon an optimal noncoding RNA scaffold (OnRS) derived from tRNA fusion pre-miR-34a (tRNA/mir-34a). Multi-milligrams of chimeric RNAs (e.g. OnRS/miR-124, OnRS/GFP-siRNA, OnRS/Neg (scrambled RNA) and OnRS/MGA (malachite green aptamer)) were readily obtained from 1 I bacterial culture. Deep sequencing analyses revealed that mature miR-124 and target GFP-siRNA were selectively released from chimeric RNAs in human cells. Consequently, OnRS/miR124 was active in suppressing miR-124 target gene expression and controlling cellular processes, and OnRS/GFP-siRNA was effective in knocking down GFP mRNA levels and fluorescent intensity in ES-2/GFP cells and GFP-transgenic mice. Furthermore, the OnRS/MGA sensor offered a specific strong fluorescence upon binding MG, which was utilized as label-free substrate to accurately determine serum RNase activities in pancreatic cancer patients. These results demonstrate that OnRS-based bioengineering is a common, robust and versatile strategy to assemble various types of small RNAs for broad applications.
机译:RNA研究和治疗主要依靠合成RNA。我们将重组RNA技术用于细菌中pre-miRNA试剂的大规模生产,但是发现大多数目标RNA并未表达或可以忽略不计。因此,我们基于从tRNA融合pre-miR-衍生的最佳非编码RNA支架(OnRS)的基础上,开发了一种新颖的策略,以实现携带各种小RNA(例如miRNA,siRNA和RNA适体)的嵌合RNA的一致高产生物合成。 34a(tRNA / mir-34a)。容易从1 I细菌培养物中获得数毫克的嵌合RNA(例如OnRS / miR-124,OnRS / GFP-siRNA,OnRS / Neg(加扰的RNA)和OnRS / MGA(孔雀石绿适体))。深度测序分析表明,成熟的miR-124和目标GFP-siRNA是从人细胞中的嵌合RNA中选择性释放的。因此,OnRS / miR124在抑制miR-124靶基因表达和控制细胞过程中具有活性,而OnRS / GFP-siRNA可以有效地降低ES-2 / GFP细胞和GFP转基因小鼠中的GFP mRNA水平和荧光强度。此外,OnRS / MGA传感器在与MG结合后可提供特定的强荧光,可将其用作无标记底物,以准确测定胰腺癌患者的血清RNase活性。这些结果表明,基于OnRS的生物工程是组装各种类型的小RNA的广泛应用的通用,健壮和通用策略。

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