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Adenine base editor engineering reduces editing of bystander cytosines

Authors
Jeong, You KyeongLee, SeokHoonHwang, Gue-HoHong, Sung-AhPark, Se-eunKim, Jin-SooWoo, Jae-SungBae, Sangsu
Issue Date
11월-2021
Publisher
NATURE PORTFOLIO
Citation
NATURE BIOTECHNOLOGY, v.39, no.11, pp.1426 - +
Indexed
SCIE
SCOPUS
Journal Title
NATURE BIOTECHNOLOGY
Volume
39
Number
11
Start Page
1426
End Page
+
URI
https://scholar.korea.ac.kr/handle/2021.sw.korea/135830
DOI
10.1038/s41587-021-00943-2
ISSN
1087-0156
Abstract
Adenine base editors (ABEs) catalyze specific A-to-G conversions at genomic sites of interest. However, ABEs also induce cytosine deamination at the target site. To reduce the cytosine editing activity, we engineered a commonly used adenosine deaminase, TadA7.10, and found that ABE7.10 with a D108Q mutation in TadA7.10 exhibited tenfold reduced cytosine deamination activity. The D108Q mutation also reduces cytosine deamination activity in two recently developed high-activity versions of ABE, ABE8e and ABE8s, and is compatible with V106W, a mutation that reduces off-target RNA editing. ABE7.10 containing a P48R mutation displayed increased cytosine deamination activity and a substantially reduced adenine editing rate, yielding a TC-specific base editing tool for TC-to-TT or TC-to-TG conversions that broadens the utility of base editors. Engineered variants of adenine base editors have reduced cytosine base editing or a specific C-to-G base editing activity.
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