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Highly efficient CRISPR-mediated large DNA docking and multiplexed prime editing using a single baculovirus

Nucleic Acids Res. 2022-07; 
Francesco Aulicino, Martin Pelosse, Christine Toelzer, Julien Capin, Erwin Ilegems, Parisa Meysami, Ruth Rollarson, Per-Olof Berggren, Mark Simon Dillingham, Christiane Schaffitzel, Moin A Saleem, Gavin I Welsh, Imre Berger
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Synthetic sgRNA and crRNA Service … were PCR amplified from synthetic vectors from GenScript. SpCas9 was PCR amplified from … 10 ul of purified bacmid were resuspended in 130 ul Sf-900 II media with 10 ul X-treme XP … Get A Quote

摘要

CRISPR-based precise gene-editing requires simultaneous delivery of multiple components into living cells, rapidly exceeding the cargo capacity of traditional viral vector systems. This challenge represents a major roadblock to genome engineering applications. Here we exploit the unmatched heterologous DNA cargo capacity of baculovirus to resolve this bottleneck in human cells. By encoding Cas9, sgRNA and Donor DNAs on a single, rapidly assembled baculoviral vector, we achieve with up to 30% efficacy whole-exon replacement in the intronic β-actin (ACTB) locus, including site-specific docking of very large DNA payloads. We use our approach to rescue wild-type podocin expression in steroid-resistant nephrotic sy... More

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