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Harnessing DSB repair to promote efficient homology-dependent and -independent prime editing

Author

Listed:
  • Martin Peterka

    (BioPharmaceuticals R&D Unit, AstraZeneca)

  • Nina Akrap

    (BioPharmaceuticals R&D Unit, AstraZeneca)

  • Songyuan Li

    (BioPharmaceuticals R&D Unit, AstraZeneca)

  • Sandra Wimberger

    (BioPharmaceuticals R&D Unit, AstraZeneca
    University of Gothenburg)

  • Pei-Pei Hsieh

    (BioPharmaceuticals R&D Unit, AstraZeneca)

  • Dmitrii Degtev

    (BioPharmaceuticals R&D Unit, AstraZeneca)

  • Burcu Bestas

    (BioPharmaceuticals R&D Unit, AstraZeneca)

  • Jack Barr

    (BioPharmaceuticals R&D Unit, AstraZeneca)

  • Stijn Plassche

    (BioPharmaceuticals R&D Unit, AstraZeneca)

  • Patricia Mendoza-Garcia

    (BioPharmaceuticals R&D Unit, AstraZeneca)

  • Saša Šviković

    (BioPharmaceuticals R&D Unit, AstraZeneca)

  • Grzegorz Sienski

    (BioPharmaceuticals R&D Unit, AstraZeneca)

  • Mike Firth

    (Discovery Sciences, AstraZeneca)

  • Marcello Maresca

    (BioPharmaceuticals R&D Unit, AstraZeneca)

Abstract

Prime editing recently emerged as a next-generation approach for precise genome editing. Here we exploit DNA double-strand break (DSB) repair to develop two strategies that install precise genomic insertions using an SpCas9 nuclease-based prime editor (PEn). We first demonstrate that PEn coupled to a regular prime editing guide RNA (pegRNA) efficiently promotes short genomic insertions through a homology-dependent DSB repair mechanism. While PEn editing leads to increased levels of by-products, it can rescue pegRNAs that perform poorly with a nickase-based prime editor. We also present a small molecule approach that yields increased product purity of PEn editing. Next, we develop a homology-independent PEn editing strategy, which installs genomic insertions at DSBs through the non-homologous end joining pathway (NHEJ). Lastly, we show that PEn-mediated insertions at DSBs prevent Cas9-induced large chromosomal deletions and provide evidence that continuous Cas9-mediated cutting is one of the mechanisms by which Cas9-induced large deletions arise. Altogether, this work expands the current prime editing toolbox by leveraging distinct DNA repair mechanisms including NHEJ, which represents the primary pathway of DSB repair in mammalian cells.

Suggested Citation

  • Martin Peterka & Nina Akrap & Songyuan Li & Sandra Wimberger & Pei-Pei Hsieh & Dmitrii Degtev & Burcu Bestas & Jack Barr & Stijn Plassche & Patricia Mendoza-Garcia & Saša Šviković & Grzegorz Sienski &, 2022. "Harnessing DSB repair to promote efficient homology-dependent and -independent prime editing," Nature Communications, Nature, vol. 13(1), pages 1-9, December.
    • Handle: RePEc:nat:natcom:v:13:y:2022:i:1:d:10.1038_s41467-022-28771-1
    DOI: 10.1038/s41467-022-28771-1
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    References listed on IDEAS

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    Cited by:

    1. Jianli Tao & Daniel E. Bauer & Roberto Chiarle, 2023. "Assessing and advancing the safety of CRISPR-Cas tools: from DNA to RNA editing," Nature Communications, Nature, vol. 14(1), pages 1-16, December.
    2. Sébastien Levesque & Diana Mayorga & Jean-Philippe Fiset & Claudia Goupil & Alexis Duringer & Andréanne Loiselle & Eva Bouchard & Daniel Agudelo & Yannick Doyon, 2022. "Marker-free co-selection for successive rounds of prime editing in human cells," Nature Communications, Nature, vol. 13(1), pages 1-14, December.
    3. Xiangyang Li & Guiquan Zhang & Shisheng Huang & Yao Liu & Jin Tang & Mingtian Zhong & Xin Wang & Wenjun Sun & Yuan Yao & Quanjiang Ji & Xiaolong Wang & Jianghuai Liu & Shiqiang Zhu & Xingxu Huang, 2023. "Development of a versatile nuclease prime editor with upgraded precision," Nature Communications, Nature, vol. 14(1), pages 1-13, December.

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