Re-engineering the adenine deaminase TadA-8e for efficient and specific CRISPR-based cytosine base editing

Liang Chen; Biyun Zhu; Gaomeng Ru; Haowei Meng; Yongchang Yan; Mengjia Hong; Dan Zhang; Changming Luan; Shun Zhang; Hao Wu; Hongyi Gao; Sijia Bai; Changqing Li; Ruoyi Ding; Niannian Xue; Zhixin Lei; Yuting Chen; Yuting Guan; Stefan Siwko; Yiyun Cheng; Gaojie Song; Liren Wang; Chengqi Yi; Mingyao Liu; Dali Li

doi:10.1038/s41587-022-01532-7

Re-engineering the adenine deaminase TadA-8e for efficient and specific CRISPR-based cytosine base editing

Liang Chen, Biyun Zhu, Gaomeng Ru, Haowei Meng, Yongchang Yan, Mengjia Hong, Dan Zhang, Changming Luan, Shun Zhang, Hao Wu, Hongyi Gao, Sijia Bai, Changqing Li, Ruoyi Ding, Niannian Xue, Zhixin Lei, Yuting Chen, Yuting Guan, Stefan Siwko, Yiyun ChengGaojie Song, Liren Wang, Chengqi Yi^*, Mingyao Liu^*, Dali Li^*

^*Corresponding author for this work

School of Life Sciences

Research output: Contribution to journal › Article › peer-review

121 Scopus citations

Abstract

Cytosine base editors (CBEs) efficiently generate precise C·G-to-T·A base conversions, but the activation-induced cytidine deaminase/apolipoprotein B mRNA-editing enzyme catalytic polypeptide-like (AID/APOBEC) protein family deaminase component induces considerable off-target effects and indels. To explore unnatural cytosine deaminases, we repurpose the adenine deaminase TadA-8e for cytosine conversion. The introduction of an N46L variant in TadA-8e eliminates its adenine deaminase activity and results in a TadA-8e-derived C-to-G base editor (Td-CGBE) capable of highly efficient and precise C·G-to-G·C editing. Through fusion with uracil glycosylase inhibitors and further introduction of additional variants, a series of Td-CBEs was obtained either with a high activity similar to that of BE4max or with higher precision compared to other reported accurate CBEs. Td-CGBE/Td-CBEs show very low indel effects and a background level of Cas9-dependent or Cas9-independent DNA/RNA off-target editing. Moreover, Td-CGBE/Td-CBEs are more efficient in generating accurate edits in homopolymeric cytosine sites in cells or mouse embryos, suggesting their accuracy and safety for gene therapy and other applications.

Original language	English
Pages (from-to)	663-672
Number of pages	10
Journal	Nature Biotechnology
Volume	41
Issue number	5
DOIs	https://doi.org/10.1038/s41587-022-01532-7
State	Published - May 2023

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Chen, L., Zhu, B., Ru, G., Meng, H., Yan, Y., Hong, M., Zhang, D., Luan, C., Zhang, S., Wu, H., Gao, H., Bai, S., Li, C., Ding, R., Xue, N., Lei, Z., Chen, Y., Guan, Y., Siwko, S., ... Li, D. (2023). Re-engineering the adenine deaminase TadA-8e for efficient and specific CRISPR-based cytosine base editing. Nature Biotechnology, 41(5), 663-672. https://doi.org/10.1038/s41587-022-01532-7

@article{2e333f8963324ffab313601b918122a0,

title = "Re-engineering the adenine deaminase TadA-8e for efficient and specific CRISPR-based cytosine base editing",

abstract = "Cytosine base editors (CBEs) efficiently generate precise C·G-to-T·A base conversions, but the activation-induced cytidine deaminase/apolipoprotein B mRNA-editing enzyme catalytic polypeptide-like (AID/APOBEC) protein family deaminase component induces considerable off-target effects and indels. To explore unnatural cytosine deaminases, we repurpose the adenine deaminase TadA-8e for cytosine conversion. The introduction of an N46L variant in TadA-8e eliminates its adenine deaminase activity and results in a TadA-8e-derived C-to-G base editor (Td-CGBE) capable of highly efficient and precise C·G-to-G·C editing. Through fusion with uracil glycosylase inhibitors and further introduction of additional variants, a series of Td-CBEs was obtained either with a high activity similar to that of BE4max or with higher precision compared to other reported accurate CBEs. Td-CGBE/Td-CBEs show very low indel effects and a background level of Cas9-dependent or Cas9-independent DNA/RNA off-target editing. Moreover, Td-CGBE/Td-CBEs are more efficient in generating accurate edits in homopolymeric cytosine sites in cells or mouse embryos, suggesting their accuracy and safety for gene therapy and other applications.",

author = "Liang Chen and Biyun Zhu and Gaomeng Ru and Haowei Meng and Yongchang Yan and Mengjia Hong and Dan Zhang and Changming Luan and Shun Zhang and Hao Wu and Hongyi Gao and Sijia Bai and Changqing Li and Ruoyi Ding and Niannian Xue and Zhixin Lei and Yuting Chen and Yuting Guan and Stefan Siwko and Yiyun Cheng and Gaojie Song and Liren Wang and Chengqi Yi and Mingyao Liu and Dali Li",

note = "Publisher Copyright: {\textcopyright} 2022, The Author(s), under exclusive licence to Springer Nature America, Inc.",

year = "2023",

month = may,

doi = "10.1038/s41587-022-01532-7",

language = "英语",

volume = "41",

pages = "663--672",

journal = "Nature Biotechnology",

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Chen, L, Zhu, B, Ru, G, Meng, H, Yan, Y, Hong, M, Zhang, D, Luan, C, Zhang, S, Wu, H, Gao, H, Bai, S, Li, C, Ding, R, Xue, N, Lei, Z, Chen, Y, Guan, Y, Siwko, S, Cheng, Y , Song, G , Wang, L, Yi, C, Liu, M & Li, D 2023, 'Re-engineering the adenine deaminase TadA-8e for efficient and specific CRISPR-based cytosine base editing', Nature Biotechnology, vol. 41, no. 5, pp. 663-672. https://doi.org/10.1038/s41587-022-01532-7

TY - JOUR

T1 - Re-engineering the adenine deaminase TadA-8e for efficient and specific CRISPR-based cytosine base editing

AU - Chen, Liang

AU - Zhu, Biyun

AU - Ru, Gaomeng

AU - Meng, Haowei

AU - Yan, Yongchang

AU - Hong, Mengjia

AU - Zhang, Dan

AU - Luan, Changming

AU - Zhang, Shun

AU - Wu, Hao

AU - Gao, Hongyi

AU - Bai, Sijia

AU - Li, Changqing

AU - Ding, Ruoyi

AU - Xue, Niannian

AU - Lei, Zhixin

AU - Chen, Yuting

AU - Guan, Yuting

AU - Siwko, Stefan

AU - Cheng, Yiyun

AU - Song, Gaojie

AU - Wang, Liren

AU - Yi, Chengqi

AU - Liu, Mingyao

AU - Li, Dali

PY - 2023/5

Y1 - 2023/5

N2 - Cytosine base editors (CBEs) efficiently generate precise C·G-to-T·A base conversions, but the activation-induced cytidine deaminase/apolipoprotein B mRNA-editing enzyme catalytic polypeptide-like (AID/APOBEC) protein family deaminase component induces considerable off-target effects and indels. To explore unnatural cytosine deaminases, we repurpose the adenine deaminase TadA-8e for cytosine conversion. The introduction of an N46L variant in TadA-8e eliminates its adenine deaminase activity and results in a TadA-8e-derived C-to-G base editor (Td-CGBE) capable of highly efficient and precise C·G-to-G·C editing. Through fusion with uracil glycosylase inhibitors and further introduction of additional variants, a series of Td-CBEs was obtained either with a high activity similar to that of BE4max or with higher precision compared to other reported accurate CBEs. Td-CGBE/Td-CBEs show very low indel effects and a background level of Cas9-dependent or Cas9-independent DNA/RNA off-target editing. Moreover, Td-CGBE/Td-CBEs are more efficient in generating accurate edits in homopolymeric cytosine sites in cells or mouse embryos, suggesting their accuracy and safety for gene therapy and other applications.

AB - Cytosine base editors (CBEs) efficiently generate precise C·G-to-T·A base conversions, but the activation-induced cytidine deaminase/apolipoprotein B mRNA-editing enzyme catalytic polypeptide-like (AID/APOBEC) protein family deaminase component induces considerable off-target effects and indels. To explore unnatural cytosine deaminases, we repurpose the adenine deaminase TadA-8e for cytosine conversion. The introduction of an N46L variant in TadA-8e eliminates its adenine deaminase activity and results in a TadA-8e-derived C-to-G base editor (Td-CGBE) capable of highly efficient and precise C·G-to-G·C editing. Through fusion with uracil glycosylase inhibitors and further introduction of additional variants, a series of Td-CBEs was obtained either with a high activity similar to that of BE4max or with higher precision compared to other reported accurate CBEs. Td-CGBE/Td-CBEs show very low indel effects and a background level of Cas9-dependent or Cas9-independent DNA/RNA off-target editing. Moreover, Td-CGBE/Td-CBEs are more efficient in generating accurate edits in homopolymeric cytosine sites in cells or mouse embryos, suggesting their accuracy and safety for gene therapy and other applications.

UR - https://www.scopus.com/pages/publications/85141662712

U2 - 10.1038/s41587-022-01532-7

DO - 10.1038/s41587-022-01532-7

M3 - 文章

C2 - 36357717

AN - SCOPUS:85141662712

SN - 1087-0156

VL - 41

SP - 663

EP - 672

JO - Nature Biotechnology

JF - Nature Biotechnology

IS - 5

ER -

Re-engineering the adenine deaminase TadA-8e for efficient and specific CRISPR-based cytosine base editing

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