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穿梭肽将碱基编辑器核糖核蛋白递送至恒河猴气道上皮细胞

Shuttle Peptide Delivers Base Editor RNPs to Rhesus Monkey Airway Epithelial Cells .

作者信息

Kulhankova Katarina, Traore Soumba, Cheng Xue, Benk-Fortin Hadrien, Hallée Stéphanie, Harvey Mario, Roberge Joannie, Couture Frédéric, Gross Thomas, Newby Gregory, Liu David, Tarantal Alice, Guay David, McCray Paul

机构信息

University of Iowa.

Feldan Therapeutics.

出版信息

Res Sq. 2023 Feb 17:rs.3.rs-2540755. doi: 10.21203/rs.3.rs-2540755/v1.

Abstract

Gene editing strategies for cystic fibrosis are challenged by the complex barrier properties of airway epithelia. We previously reported that the amphiphilic S10 shuttle peptide non-covalently combined with CRISPR-associated (Cas) ribonucleoprotein (RNP) enabled editing of human and mouse airway epithelial cells. Here, to improve base editor RNP delivery, we optimized S10 to derive the S315 peptide. Following intratracheal aerosol of Cy5-labeled peptide cargo in rhesus macaques, we confirmed delivery throughout the respiratory tract. Subsequently, we targeted with co-administration of ABE8e-Cas9 RNP and S315. We achieved editing efficiencies of up to 5.3% in rhesus airway epithelia. Moreover, we documented persistence of edited epithelia for up to 12 months in mice. Finally, delivery of ABE8e-Cas9 targeting the mutation restored anion channel function in cultured human airway epithelial cells. These results demonstrate the therapeutic potential of base editor delivery with S315 to functionally correct the mutation in respiratory epithelia.

摘要

囊性纤维化的基因编辑策略受到气道上皮复杂屏障特性的挑战。我们之前报道过,两亲性S10穿梭肽与CRISPR相关(Cas)核糖核蛋白(RNP)非共价结合能够对人和小鼠气道上皮细胞进行编辑。在此,为了改善碱基编辑器RNP的递送,我们对S10进行了优化以获得S315肽。在恒河猴中进行气管内雾化Cy5标记的肽负载后,我们证实了其在整个呼吸道的递送。随后,我们通过共同施用ABE8e-Cas9 RNP和S315进行靶向。我们在恒河猴气道上皮中实现了高达5.3%的编辑效率。此外,我们记录了在小鼠中编辑后的上皮细胞持续存在长达12个月。最后,递送靶向该突变的ABE8e-Cas9恢复了培养的人气道上皮细胞中的阴离子通道功能。这些结果证明了用S315递送碱基编辑器在功能上纠正呼吸道上皮中该突变的治疗潜力。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2dfc/9949254/5403c968d639/nihpp-rs2540755v1-f0001.jpg

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