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内溶酶体肽可实现肽核酸的细胞递送。

Endosomolytic peptides enable the cellular delivery of peptide nucleic acids.

作者信息

Giancola JoLynn B, Raines Ronald T

机构信息

Department of Chemistry, Massachusetts institute of Technology, 77 Massachusetts Avenue, Cambridge, MA 02139, USA.

出版信息

Chem Commun (Camb). 2024 Dec 12;60(100):15019-15022. doi: 10.1039/d4cc05214e.

Abstract

Precision genetic medicine enlists antisense oligonucleotides (ASOs) to bind to nucleic acid targets important for human disease. Peptide nucleic acids (PNAs) have many desirable attributes as ASOs but lack cellular permeability. Here, we use an assay based on the corrective splicing of an mRNA to assess the ability of synthetic peptides to deliver a functional PNA into a human cell. We find that the endosomolytic peptides L17E and L17ER are highly efficacious delivery vehicles. Co-treatment of a PNA with low micromolar L17E or L17ER enables robust corrective splicing in nearly all treated cells. Peptide-PNA conjugates are even more effective. These results enhance the utility of PNAs as research tools and potential therapeutic agents.

摘要

精准基因医学利用反义寡核苷酸(ASO)与对人类疾病至关重要的核酸靶点结合。肽核酸(PNA)作为ASO具有许多理想特性,但缺乏细胞通透性。在此,我们使用一种基于mRNA校正剪接的检测方法来评估合成肽将功能性PNA递送至人类细胞的能力。我们发现溶酶体溶解肽L17E和L17ER是高效的递送载体。将PNA与低微摩尔浓度的L17E或L17ER共同处理可使几乎所有处理过的细胞实现强大的校正剪接。肽-PNA缀合物甚至更有效。这些结果提高了PNA作为研究工具和潜在治疗剂的效用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/16bd/11600723/56d38e246554/d4cc05214e-s1.jpg

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