Safe Harbor Targeted CRISPR-Cas9 Tools for Molecular-Genetic Imaging of Cells in Living Subjects.

Autor: Dubois VP; 1 Department of Medical Biophysics, Western University , London, Ontario, Canada.; 2 Imaging Research Laboratories, Robarts Research Institute , London, Ontario, Canada., Zotova D; 2 Imaging Research Laboratories, Robarts Research Institute , London, Ontario, Canada., Parkins KM; 1 Department of Medical Biophysics, Western University , London, Ontario, Canada., Swick C; 2 Imaging Research Laboratories, Robarts Research Institute , London, Ontario, Canada., Hamilton AM; 2 Imaging Research Laboratories, Robarts Research Institute , London, Ontario, Canada., Kelly JJ; 2 Imaging Research Laboratories, Robarts Research Institute , London, Ontario, Canada., Ronald JA; 1 Department of Medical Biophysics, Western University , London, Ontario, Canada.; 2 Imaging Research Laboratories, Robarts Research Institute , London, Ontario, Canada.; 3 Lawson Health Research Institute, London, Ontario, Canada .
Jazyk: angličtina
Zdroj: The CRISPR journal [CRISPR J] 2018 Dec; Vol. 1, pp. 440-449.
DOI: 10.1089/crispr.2018.0030
Abstrakt: Noninvasive molecular-genetic imaging of cells expressing imaging reporter genes is an invaluable approach for longitudinal monitoring of the biodistribution and viability of cancer cells and cell-based therapies in preclinical models and patients. However, labeling cells with reporter genes often relies on using gene transfer methods that randomly integrate the reporter genes into the genome, which may cause unwanted and serious detrimental effects. To overcome this, we have developed CRISPR-Cas9 tools to edit cells at the adeno-associated virus site 1 (AAVS1) safe harbour with a large donor construct (∼6.3 kilobases) encoding an antibiotic resistance gene and reporter genes for bioluminescence (BLI) and fluorescence imaging. HEK293T cells were transfected with a dual plasmid system encoding the Cas9 endonuclease and an AAVS1-targeted guide RNA in one plasmid, and a donor plasmid encoding a puromycin resistance gene, tdTomato and firefly luciferase flanked by AAVS1 homology arms. Puromycin-resistant clonal cells were isolated and AAVS1 integration was confirmed via PCR and sequencing of the PCR product. In vitro BLI signal correlated well to cell number ( R 2  = 0.9988; p  < 0.05) and was stable over multiple passages. Engineered cells (2.5 × 10 6 ) were injected into the left hind flank of nude mice and in vivo BLI was performed on days 0, 7, 14, 21, and 28. BLI signal trended down from day 0 to day 7, but significantly increased by day 28 due to cell growth ( p  < 0.05). This describes the first CRISPR-Cas9 system for AAVS1 integration of large gene constructs for molecular-genetic imaging of cells in vivo . With further development, including improving editing efficiency, use of clinically relevant reporters, and evaluation in other cell populations that can be readily expanded in culture (e.g., immortalized cells or T cells), this CRISPR-Cas9 reporter gene system could be broadly applied to a number of in vivo cell tracking studies.
Databáze: MEDLINE