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  3. Peptide dendrimers transfecting CRISPR/Cas9 plasmid DNA: optimization and mechanism.
 

Peptide dendrimers transfecting CRISPR/Cas9 plasmid DNA: optimization and mechanism.

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BORIS DOI
10.48620/8304
Publisher DOI
10.1039/d4cb00116h
PubMed ID
39211473
Description
Gene editing by CRISPR/Cas9 offers great therapeutic opportunities but requires delivering large plasmid DNA (pDNA) into cells, a task for which transfection reagents are better suited than viral vectors. Here we performed a structure-activity relationship study of Z22, a d-enantiomeric, arginine containing, lipidated peptide dendrimer developed for pDNA transfection of a CRISPR/Cas9 plasmid co-expressing GFP. While all dendrimer analogs tested bound pDNA strongly and internalized their cargo into cells, d-chirality proved essential for transfection by avoiding proteolysis of the dendrimer structure required for endosome escape and possibly crossing of the nuclear envelope. Furthermore, a cysteine residue at the core of Z22 proved non-essential and was removed to yield the more active analog Z34. This dendrimer shows >83% GFP transfection efficiency in HEK cells with no detrimental effect on cell viability and promotes functional CRISPR/Cas9 mediated gene editing. It is accessible by solid-phase peptide synthesis and therefore attractive for further development.
Date of Publication
2024-08-28
Publication Type
Article
Language(s)
en
Contributor(s)
Zamolo, Susanna
Zakharova, Elena
Department of Chemistry, Biochemistry and Pharmaceutical Sciences (DCBP)
Boursinhac, Lise
Hollfelder, Florian
Darbre, Tamis
Reymond, Jean-Louisorcid-logo
DCBP Gruppe Prof. Reymond
Additional Credits
DCBP Gruppe Prof. Reymond
Department of Chemistry, Biochemistry and Pharmaceutical Sciences (DCBP)
Series
RSC chemical biology
ISSN
2633-0679
Access(Rights)
open.access
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