4.5 Article

SpRY greatly expands the genome editing scope in rice with highly flexible PAM recognition

Journal

GENOME BIOLOGY
Volume 22, Issue 1, Pages -

Publisher

BMC
DOI: 10.1186/s13059-020-02231-9

Keywords

CRISPR; SpG; SpRY; Genome editing; Base editing; Self-targeting; Oryza sativa L

Funding

  1. National Natural Science Foundation of China [31871948, 31930089]
  2. Fundamental Research Funds
  3. Agricultural Science and Technology Innovation Program of the Chinese Academy of Agricultural Sciences [Y2020PT26]
  4. National Transgenic Science and Technology Program of China [2019ZX08010-003]

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This study thoroughly investigated the nuclease activity and PAM preference of two structurally engineered SpCas9 variants, SpG and SpRY, in transgenic rice, with SpRY showing broad PAM compatibility and expanding the targeting scope of CRISPR-based tools in plant genome engineering.
BackgroundPlant genome engineering mediated by various CRISPR-based tools requires specific protospacer adjacent motifs (PAMs), such as the well-performed NGG, NG, and NNG, to initiate target recognition, which notably restricts the editable range of the plant genome.ResultsIn this study, we thoroughly investigate the nuclease activity and the PAM preference of two structurally engineered SpCas9 variants, SpG and SpRY, in transgenic rice. Our study shows that SpG nuclease favors NGD PAMs, albeit less efficiently than the previously described SpCas9-NG, and that SpRY nuclease achieves efficient editing across a wide range of genomic loci, exhibiting a preference of NGD as well as NAN PAMs. Furthermore, SpRY-fused cytidine deaminase hAID*Delta and adenosine deaminase TadA8e are generated, respectively. These constructs efficiently induce C-to-T and A-to-G conversions in the target genes toward various non-canonical PAMs, including non-G PAMs. Remarkably, high-frequency self-editing events (indels and DNA fragments deletion) in the integrated T-DNA fragments as a result of the nuclease activity of SpRY are observed, whereas the self-editing of SpRY nickase-mediated base editor is quite low in transgenic rice lines.ConclusionsThe broad PAM compatibility of SpRY greatly expands the targeting scope of CRISPR-based tools in plant genome engineering.

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