Efficient selection of a biallelic and nonchimeric gene-edited tree using Oxford Nanopore Technologies sequencing

索引 放大器 生物 仆从 遗传学 纳米孔测序 清脆的 INDEL突变 计算生物学 DNA测序 突变 突变体 冷PCR 基因 Cas9 聚合酶链反应 点突变 基因型 单核苷酸多态性
作者
Ryôsuke Satô,Yoshihiko Nanasato,Naoki Takata,Soichiro Nagano,Eitaro Fukatsu,Takeshi Fujino,Katushi Yamaguchi,Yoshinari Moriguchi,Shuji Shigenobu,Yutaka Suzuki,Masahiro Kasahara,S. Ueno
出处
期刊:Tree Physiology [Oxford University Press]
标识
DOI:10.1093/treephys/tpad158
摘要

Abstract The clustered regularly interspaced short palindromic repeats (CRISPR)/CRISPR-associated protein 9 nuclease (Cas9) system is a versatile and essential biotechnological tool in the life sciences that allows efficient genome editing. When generating gene-edited trees, T0-generation plants are often used for subsequent analysis because of the time that is required to obtain the desired mutants via crossing. However, T0-generation plants exhibit various unexpected mutations, which emphasizes the need to identify mutants with expected mutation patterns. The two critical checkpoints in this process are to confirm the expected mutation patterns in both alleles and to exclude somatic chimeric plants. In this study, we generated gene-edited Cryptomeria japonica plants and established a method to determine chimerism and mutation patterns using fragment analysis and Oxford Nanopore Technologies (ONT)-based amplicon sequencing. In the first screening, fragment analysis, i.e., indel detection via amplicon analysis (IDAA), was used to predict indel mutation patterns in both alleles and to discriminate somatic chimeric plants in 188 candidate mutants. In the second screening, we precisely determined the mutation patterns and chimerism in the mutants using ONT-based amplicon sequencing, where confirmation of both alleles can be achieved using allele-specific markers flanking the single guide RNA (sgRNA) target site. In the present study, a bioinformatic analysis procedure was developed and provided for the rapid and accurate determination of DNA mutation patterns using ONT-based amplicon sequencing. As ONT amplicon sequencing has a low running cost compared with other long-read analysis methods, such as PacBio, it is a powerful tool in plant genetics and biotechnology to select gene-edited plants with expected indel patterns in the T0-generation.
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