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Molecular recordings by directed CRISPR spacer acquisition

机译:通过定向CRISPR间隔子采集进行分子记录

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摘要

The ability to write a stable record of identified molecular events into a specific genomic locus would enable the examination of long cellular histories and have many applications, ranging from developmental biology to synthetic devices. We show that the type I-E CRISPR-Cas system of E. coli can mediate acquisition of defined pieces of synthetic DNA. We harnessed this feature to generate records of specific DNA sequences into a population of bacterial genomes. We then applied directed evolution to alter the recognition of a protospacer adjacent motif by the Cas1-Cas2 complex, which enabled recording in two modes simultaneously. We used this system to reveal aspects of spacer acquisition, fundamental to the CRISPR-Cas adaptation process. These results lay the foundations of a multimodal intracellular recording device.
机译:将已鉴定的分子事件的稳定记录写入特定基因组基因座的能力将能够检查较长的细胞历史,并具有许多用途,从发育生物学到合成装置。我们显示,大肠杆菌的I-E型CRISPR-Cas系统可以介导合成DNA定义片段的获取。我们利用此功能将特定DNA序列的记录生成细菌基因组。然后,我们应用定向进化来改变Cas1-Cas2复合体对原间隔子相邻基序的识别,从而可以同时以两种模式进行记录。我们使用该系统揭示了间隔捕获的各个方面,这是CRISPR-Cas适应过程的基础。这些结果奠定了多模式细胞内记录设备的基础。

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