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. 2025 Sep;43(9):1548-1561.
doi: 10.1038/s41587-024-02430-w. Epub 2024 Oct 9.

A circularly permuted CasRx platform for efficient, site-specific RNA editing

Yuanming Wang #  1   2 Kaiwen Ivy Liu #  1   2 Mengying Mandy Liu #  1   2 Kean Hean Ooi #  1   2 Tram Anh Nguyen  1 Jiunn En Chee  1   2   3 Shun Xiang Danny Teo  1   2   4 Shan He  2   3 Jie Wen Douglas Tay  1   3 Seok Yee Teo  1   3 Kai Shin Liew  1 Xiao Yu Ge  1 Zhi Jian Ng  1 Hasmik Avagyan  1 Hao Liu  1 Zirong Yi  1 Keziah Chang  2 Eng Piew Louis Kok  2 Runjia Chen  2   5 Chun En Yau  2   6 Jun Wei Koh  2   6 Yue Wan  2   3   7 Meng How Tan  8   9   10
Affiliations

A circularly permuted CasRx platform for efficient, site-specific RNA editing

Yuanming Wang et al. Nat Biotechnol. 2025 Sep.

Abstract

Inactive Cas13 orthologs have been fused to a mutant human ADAR2 deaminase domain at the C terminus to enable programmable adenosine-to-inosine (A-to-I) RNA editing in selected transcripts. Although promising, existing RNA-editing tools generally suffer from a trade-off between efficacy and specificity, and off-target editing remains an unsolved problem. Here we describe the development of an optimized RNA-editing platform by rational protein engineering, CasRx-based Programmable Editing of RNA Technology (xPERT). We demonstrate that the topological rearrangement of a CasRx K940L mutant by circular permutation results in a robust scaffold for the tethering of a deaminase domain. We benchmark our tool against the REPAIR system and show that xPERT exhibits strong on-target activity like REPAIRv1 but low off-target editing like REPAIRv2. Our xPERT platform can be used to alter RNA sequence information without risking genome damage, effect temporary cellular changes and customize protein function.

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Conflict of interest statement

Competing interests: M.H.T., Y. Wang, K.I.L. and K.H.O. are co-inventors on a patent that has been filed for xPERT (application under the Patent Cooperation Treaty: PCT/SG2020/050599). The other authors declare no competing interests.

References

    1. Cox, D. B., Platt, R. J. & Zhang, F. Therapeutic genome editing: prospects and challenges. Nat. Med. 21, 121–131 (2015). - PubMed - PMC - DOI
    1. Ihry, R. J. et al. p53 inhibits CRISPR–Cas9 engineering in human pluripotent stem cells. Nat. Med. 24, 939–946 (2018). - PubMed - DOI
    1. Haapaniemi, E., Botla, S., Persson, J., Schmierer, B. & Taipale, J. CRISPR–Cas9 genome editing induces a p53-mediated DNA damage response. Nat. Med. 24, 927–930 (2018). - PubMed - DOI
    1. Nishikura, K. A-to-I editing of coding and non-coding RNAs by ADARs. Nat. Rev. Mol. Cell Biol. 17, 83–96 (2016). - PubMed - DOI
    1. Merkle, T. et al. Precise RNA editing by recruiting endogenous ADARs with antisense oligonucleotides. Nat. Biotechnol. 37, 133–138 (2019). - PubMed - DOI

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