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通过蛋白质工程和蛋白质递送提高碱基编辑的 DNA 特异性和适用性。

Improving the DNA specificity and applicability of base editing through protein engineering and protein delivery.

机构信息

Department of Chemistry and Chemical Biology, Harvard University, Cambridge, Massachusetts 02138, USA.

Howard Hughes Medical Institute, Harvard University, Cambridge, Massachusetts 02138, USA.

出版信息

Nat Commun. 2017 Jun 6;8:15790. doi: 10.1038/ncomms15790.

Abstract

We recently developed base editing, a genome-editing approach that enables the programmable conversion of one base pair into another without double-stranded DNA cleavage, excess stochastic insertions and deletions, or dependence on homology-directed repair. The application of base editing is limited by off-target activity and reliance on intracellular DNA delivery. Here we describe two advances that address these limitations. First, we greatly reduce off-target base editing by installing mutations into our third-generation base editor (BE3) to generate a high-fidelity base editor (HF-BE3). Next, we purify and deliver BE3 and HF-BE3 as ribonucleoprotein (RNP) complexes into mammalian cells, establishing DNA-free base editing. RNP delivery of BE3 confers higher specificity even than plasmid transfection of HF-BE3, while maintaining comparable on-target editing levels. Finally, we apply these advances to deliver BE3 RNPs into both zebrafish embryos and the inner ear of live mice to achieve specific, DNA-free base editing in vivo.

摘要

我们最近开发了碱基编辑技术,这是一种基因组编辑方法,可在不进行双链 DNA 切割、过多随机插入和缺失或不依赖同源定向修复的情况下,将一个碱基对可编程地转换为另一个碱基对。碱基编辑的应用受到脱靶活性和对细胞内 DNA 递送的依赖的限制。在这里,我们描述了两项可解决这些限制的进展。首先,我们通过在第三代碱基编辑器(BE3)中安装突变来大大减少脱靶碱基编辑,从而生成高保真碱基编辑器(HF-BE3)。接下来,我们将 BE3 和 HF-BE3 纯化并作为核糖核蛋白(RNP)复合物递送至哺乳动物细胞中,从而实现无 DNA 的碱基编辑。RNP 递送的 BE3 甚至比 HF-BE3 的质粒转染具有更高的特异性,同时保持可比的靶向编辑水平。最后,我们将这些进展应用于将 BE3 RNP 递送至斑马鱼胚胎和活体小鼠内耳中,以在体内实现特定的、无 DNA 的碱基编辑。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f56b/5467206/cc35fd094e3a/ncomms15790-f1.jpg

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