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工程化的 pegRNA 可提高 Prime 编辑效率。

Engineered pegRNAs improve prime editing efficiency.

机构信息

Merkin Institute of Transformative Technologies in Healthcare, Broad Institute of MIT and Harvard, Cambridge, MA, USA.

Howard Hughes Medical Institute, Harvard University, Cambridge, MA, USA.

出版信息

Nat Biotechnol. 2022 Mar;40(3):402-410. doi: 10.1038/s41587-021-01039-7. Epub 2021 Oct 4.

Abstract

Prime editing enables the installation of virtually any combination of point mutations, small insertions or small deletions in the DNA of living cells. A prime editing guide RNA (pegRNA) directs the prime editor protein to the targeted locus and also encodes the desired edit. Here we show that degradation of the 3' region of the pegRNA that contains the reverse transcriptase template and the primer binding site can poison the activity of prime editing systems, impeding editing efficiency. We incorporated structured RNA motifs to the 3' terminus of pegRNAs that enhance their stability and prevent degradation of the 3' extension. The resulting engineered pegRNAs (epegRNAs) improve prime editing efficiency 3-4-fold in HeLa, U2OS and K562 cells and in primary human fibroblasts without increasing off-target editing activity. We optimized the choice of 3' structural motif and developed pegLIT, a computational tool to identify non-interfering nucleotide linkers between pegRNAs and 3' motifs. Finally, we showed that epegRNAs enhance the efficiency of the installation or correction of disease-relevant mutations.

摘要

引发编辑技术可在活细胞的 DNA 中几乎任意组合地点突变、小片段插入或缺失。引发编辑向导 RNA(pegRNA)指导引发编辑蛋白到达靶向基因座,并且还编码所需的编辑。本文中,我们发现,pegRNA 3' 区域(包含逆转录酶模板和引物结合位点)的降解会使引发编辑系统失活,从而阻碍编辑效率。我们在 pegRNA 的 3' 末端加入了结构 RNA 基序,从而提高了它们的稳定性并防止 3' 延伸的降解。由此产生的工程化 pegRNA(epegRNA)可将 HeLa、U2OS 和 K562 细胞以及原代人成纤维细胞中的引发编辑效率提高 3-4 倍,而不会增加脱靶编辑活性。我们优化了 3' 结构基序的选择,并开发了 pegLIT,这是一种用于识别 pegRNA 和 3' 基序之间非干扰核苷酸接头的计算工具。最后,我们证明了 epegRNA 可提高与疾病相关的突变的安装或校正效率。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/6722/8930418/ad2e17e5620b/nihms-1729173-f0001.jpg

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