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Multiplexed promoterless gene expression with CRISPReader

机译:用脆性仪器多重启动子基因表达

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Abstract BackgroundGenes are comprised of DNA codes and contain promoters and other control elements for reading these codes. The rapid development of clustered regularly interspaced short palindromic repeats (CRISPR) technology has made possible the construction of a novel code-reading system with low dependency on the native control elements.ResultsWe develop CRISPReader, a technology for controlling promoterless gene expression in a robust fashion. We demonstrate that this tool is highly efficient in controlling transcription and translation initiation of a targeted transgene. A notable feature of CRISPReader is the ability to “read” the open reading frames of a cluster of gene without traditional regulatory elements or other cofactors. In particular, we use this strategy to construct an all-in-one AAV-CRISPR-Cas9 system by removing promoter-like elements from the expression cassette to resolve the existing AAV packaging size problem. The compact AAV-CRISPR-Cas9 is also more efficient in transactivation, DNA cleavage, and gene editing than the dual-AAV vector encoding two separate Cas9 elements, shown by targeting both reporter and endogenous genes in vitro and in vivo.ConclusionsCRISPReader represents a novel approach for gene regulation that enables minimal gene constructs to be expressed and can be used in potential biomedical applications.
机译:摘要背景由DNA代码组成,并包含用于读取这些代码的启动子和其他控制元件。集群经常间隙的短语重复(CISRPR)技术的快速发展使得具有低依赖性的新型码头读取系统的构建成为原生控制元素。培养污垢普通的技术,一种用于以强大的方式控制启动者基因表达的技术。我们证明该工具在控制靶向转基因的转录和翻译引发方面具有高效。脆性师的一个值得注意的特征是能够“读取”没有传统的监管元素或其他辅助因子的基因集群的开放阅读帧。特别是,我们使用这种策略来通过从表达式盒中移除启动子样元件来构造一体化AAV-CRAAP-CAS9系统,以解决现有的AAV包装尺寸问题。 Compact Aav-CRISPR-CAS9在转移,DNA裂解和基因编辑中也比编码两个单独的CAS9元素的双AAV载体更有效,通过靶向报道和体内和体内的内源基因来显示.Clucluscrispreader代表一种新颖基因调控方法,其能够表达最小基因构建体,可用于潜在的生物医学应用。

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