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利用真核逆转录元件蛋白将转基因插入人类安全位点。

Harnessing eukaryotic retroelement proteins for transgene insertion into human safe-harbor loci.

作者信息

Zhang Xiaozhu, Van Treeck Briana, Horton Connor A, McIntyre Jeremy J R, Palm Sarah M, Shumate Justin L, Collins Kathleen

机构信息

Department of Molecular and Cell Biology, University of California at Berkeley, Berkeley, CA, USA.

出版信息

Nat Biotechnol. 2025 Jan;43(1):42-51. doi: 10.1038/s41587-024-02137-y. Epub 2024 Feb 20.

Abstract

Current approaches for inserting autonomous transgenes into the genome, such as CRISPR-Cas9 or virus-based strategies, have limitations including low efficiency and high risk of untargeted genome mutagenesis. Here, we describe precise RNA-mediated insertion of transgenes (PRINT), an approach for site-specifically primed reverse transcription that directs transgene synthesis directly into the genome at a multicopy safe-harbor locus. PRINT uses delivery of two in vitro transcribed RNAs: messenger RNA encoding avian R2 retroelement-protein and template RNA encoding a transgene of length validated up to 4 kb. The R2 protein coordinately recognizes the target site, nicks one strand at a precise location and primes complementary DNA synthesis for stable transgene insertion. With a cultured human primary cell line, over 50% of cells can gain several 2 kb transgenes, of which more than 50% are full-length. PRINT advantages include no extragenomic DNA, limiting risk of deleterious mutagenesis and innate immune responses, and the relatively low cost, rapid production and scalability of RNA-only delivery.

摘要

目前将自主转基因插入基因组的方法,如CRISPR-Cas9或基于病毒的策略,存在效率低和非靶向基因组诱变风险高的局限性。在此,我们描述了转基因的精确RNA介导插入(PRINT),这是一种位点特异性引发逆转录的方法,可将转基因合成直接定向到多拷贝安全港位点的基因组中。PRINT使用两种体外转录RNA的递送:编码禽R2反转录元件蛋白的信使RNA和编码长度经验证可达4 kb的转基因的模板RNA。R2蛋白协同识别靶位点,在精确位置切割一条链,并引发互补DNA合成以实现稳定的转基因插入。在一种培养的人类原代细胞系中,超过50%的细胞可获得多个2 kb的转基因,其中超过50%是全长的。PRINT的优点包括无基因组外DNA,限制了有害诱变和先天免疫反应的风险,以及仅RNA递送相对低成本、快速生产和可扩展性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7f52/11738989/c8db774da324/41587_2024_2137_Fig1_HTML.jpg

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