Study of the CRISPR/Cas3 System for Xenotransplantation

•bpNLS-Cascade, BPNLS-hCas3, and pBS-U6icrRNA were prepared.•The effect of the CRISPR/Cas3 system on pig cell was confimed.•CRISPR/Cas3 system provided the target genome with relative large deletion. The CRISPR/Cas3 system, classified in class I system, was recently focused as a new technology. For...

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Bibliographic Details
Published in:Transplantation proceedings 2022-03, Vol.54 (2), p.522-524
Main Authors: Miyagawa, Shuji, Watanabe, Masahito, Nagashima, Hiroshi, Sato, Kazuki, Kogata, Shuhei, Toyama, Chiyoshi, Masahata, Kazunori, Kamiyama, Masafumi, Yamamoto, Riho, Eguchi, Hiroshi, Maeda, Akira, Yoshimi, Kazuto, Mashimo, Tomoji, Okuyama, Hiroomi
Format: Article
Language:English
Subjects:
Animals
CRISPR-Cas Systems
Escherichia coli
Humans
Swine
Transfection
Transplantation, Heterologous
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Summary:•bpNLS-Cascade, BPNLS-hCas3, and pBS-U6icrRNA were prepared.•The effect of the CRISPR/Cas3 system on pig cell was confimed.•CRISPR/Cas3 system provided the target genome with relative large deletion. The CRISPR/Cas3 system, classified in class I system, was recently focused as a new technology. For application of this system to porcine cells, the plasmids of bpNLS-Cascade, BPNLS-hCas3, and pBS-U6icrRNA were prepared. Initially, 2 crRNAs were established in the exon 9 of pig Gal-T (GGTA1) as #45 and #86. Next, hCas3 + #45 + #86 (group 1, control), Cascade + hCas3 + #45 (group 2), Cascade + hCas3 + #86 (group 3), and Cascade + hCas3 + #45 + #86 (group 4) were set and transfected into pig fibroblasts. Transfected cells were analyzed for bulk expression of α1,3Gal epitope by fluorescence-activated cell sorting (FACS), using a GSI-B4 lectin 2 days after the transfection. As the results, changes of expression are observed in order of G4>G2>G3, indicating the effect of the Cas3 system. Therefore, the nested polymerase chain reaction (PCR) for target region of GGTA1 was performed. Next, the PCR products from each group were checked in blotting, and the products were placed into the cloning sit of TOPO vector and transformed into Escherichia coli. Sixteen colonies of each group were checked by PCR, and clones containing PCR product with slightly varying length were evaluated. The direct sequence of these PCR changes were demonstrated as 294 to 754 bp deletions. In conclusion, we confirmed the effect of the CRISPR/Cas3 system on pig cell, especially in xenotransplantation.
ISSN:0041-1345
1873-2623
DOI:10.1016/j.transproceed.2021.09.070