Limitations of the Plasmid-Based Cas9-Zinc Finger Fusion System for Homology-Directed Knock-In in Chinese Hamster Ovary Cells

The clustered regularly interspaced short palindromic repeat (CRISPR)/CRISPR-associated protein 9 (Cas9) system has been used for the insertion of large transgenes into Chinese hamster ovary cells via co-transfection of a Cas9/guide RNA expression vector and donor plasmid. The Cas9 protein includes...

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Bibliographic Details
Published inBiotechnology and bioprocess engineering Vol. 28; no. 2; pp. 289 - 299
Main Authors Kim, Dongwoo, Lee, Jae Seong
Format Journal Article
LanguageEnglish
Published Seoul The Korean Society for Biotechnology and Bioengineering 01.04.2023
Springer Nature B.V
한국생물공학회
Subjects
Biotechnology
Chemistry
Chemistry and Materials Science
Cricetulus griseus
CRISPR
CRISPR-associated endonuclease 9
CRISPR-Cas systems
DNA damage
Efficiency
gene editing
Gene expression
Genetic modification
genetic vectors
Genome editing
Homology
Imports
Industrial and Production Engineering
Localization
Nuclei (cytology)
Ovaries
peptides
Plasmids
Proteins
Research Paper
RNA
Tethering
Transfection
Transgenes
Translocation
Zinc
zinc finger motif
Zinc finger proteins
생물공학
Chinese hamster ovary
donor plasmid
CRISPR/Cas9
homology-directed repair
zinc finger
knock-in
Online AccessGet full text
ISSN1226-8372
1976-3816
DOI10.1007/s12257-022-0348-6

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Summary:The clustered regularly interspaced short palindromic repeat (CRISPR)/CRISPR-associated protein 9 (Cas9) system has been used for the insertion of large transgenes into Chinese hamster ovary cells via co-transfection of a Cas9/guide RNA expression vector and donor plasmid. The Cas9 protein includes nuclear localization sequences that are used as peptide tags for the import of Cas9 into the nucleus. However, the import of a donor plasmid into the nucleus is passive because of the absence of such localization signals; thus, the delivery of Cas9 and the donor plasmid is not synchronized, resulting in low knock-in (KI) efficiency. Here, we modified the Cas9 expression vector expressing a Cas9 protein fused to a zinc finger (ZF) domain, Cas9-ZF, to expedite the translocation of the donor plasmid into the nucleus and the co-localization of the donor plasmid with a CRISPR/Cas9-mediated DNA double-strand break site by tethering Cas9-ZF and the donor plasmid. Compared to the typical donor plasmid and wild-type Cas9, the donor plasmid harboring the ZF-binding motif showed increased homology-mediated KI efficiency, while the engineered Cas9 protein showed decreased expression and gene-editing efficiency. Moreover, the pair of Cas9-ZF and the donor plasmid with the ZF motif did not improve KI efficiency, but rather negated the positive effect of the donor plasmid with the ZF motif. This study demonstrates the importance of the transport of donor plasmids and the limitations of using the plasmid-based Cas9-ZF fusion system to improve KI efficiency.
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ISSN:1226-8372
1976-3816
DOI:10.1007/s12257-022-0348-6