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利用CRISPR-Cas系统构建翻译激活因子

Engineering Translational Activators with CRISPR-Cas System.

作者信息

Du Pei, Miao Chensi, Lou Qiuli, Wang Zefeng, Lou Chunbo

机构信息

CAS Key Laboratory of Microbial Physiological and Metabolic Engineering, Institute of Microbiology, Chinese Academy of Sciences ; Beijing, 100101, China.

College of Life Science, University of Science and Technology of China , Hefei 230027, China.

出版信息

ACS Synth Biol. 2016 Jan 15;5(1):74-80. doi: 10.1021/acssynbio.5b00130. Epub 2015 Oct 8.

Abstract

RNA parts often serve as critical components in genetic engineering. Here we report a design of translational activators which is composed of an RNA endoribonuclease (Csy4) and two exchangeable RNA modules. Csy4, a member of Cas endoribonuclease, cleaves at a specific recognition site; this cleavage releases a cis-repressive RNA module (crRNA) from the masked ribosome binding site (RBS), which subsequently allows the downstream translation initiation. Unlike small RNA as a translational activator, the endoribonuclease-based activator is able to efficiently unfold the perfect RBS-crRNA pairing. As an exchangeable module, the crRNA-RBS duplex was forwardly and reversely engineered to modulate the dynamic range of translational activity. We further showed that Csy4 and its recognition site, together as a module, can also be replaced by orthogonal endoribonuclease-recognition site homologues. These modularly structured, high-performance translational activators would endow the programming of gene expression in the translation level with higher feasibility.

摘要

RNA 组件常常作为基因工程中的关键元件。在此,我们报道了一种翻译激活因子的设计,它由一种 RNA 内切核糖核酸酶(Csy4)和两个可互换的 RNA 模块组成。Csy4 是 Cas 内切核糖核酸酶家族的一员,能在特定识别位点进行切割;这种切割从被掩盖的核糖体结合位点(RBS)释放出一个顺式抑制性 RNA 模块(crRNA),随后使得下游翻译起始。与作为翻译激活因子的小 RNA 不同,基于内切核糖核酸酶的激活因子能够有效地解开完美的 RBS-crRNA 配对。作为一个可互换模块,crRNA-RBS 双链体经过正向和反向工程改造以调节翻译活性的动态范围。我们进一步表明,Csy4 及其识别位点作为一个模块,也可以被正交内切核糖核酸酶-识别位点同源物所取代。这些具有模块化结构的高性能翻译激活因子将赋予在翻译水平上进行基因表达编程更高的可行性。

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