Synthetic nucleases for genome engineering in plants: prospects for a bright future

被引:160
作者
Puchta, Holger [1 ]
Fauser, Friedrich [1 ]
机构
[1] Karlsruhe Inst Technol, Bot Inst 2, D-76049 Karlsruhe, Germany
基金
欧洲研究理事会;
关键词
gene technology; double-strand break repair; synthetic nucleases; targeted mutagenesis; gene targeting; DOUBLE-STRAND BREAKS; SITE-DIRECTED MUTAGENESIS; DNA-BINDING SPECIFICITY; ZINC-FINGER NUCLEASES; HOMOLOGOUS RECOMBINATION; TARGETED MUTAGENESIS; DIFFERENT PATHWAYS; RESTRICTION ENZYMES; T-DNA; GENE;
D O I
10.1111/tpj.12338
中图分类号
Q94 [植物学];
学科分类号
071001 ;
摘要
By inducing double-strand breaks (DSB), it is possible to initiate DNA recombination. For a long time, it was not possible to use DSB induction for efficient genome engineering due to the lack of a means to target DSBs to specific sites. This limitation was overcome by development of modified meganucleases and synthetic DNA-binding domains. Domains derived from zinc-finger transcription factors or transcription activator-like effectors may be designed to recognize almost any DNA sequence. By fusing these domains to the endonuclease domains of a classII restriction enzyme, an active endonuclease dimer may be formed that introduces a site-specific DSB. Recent studies demonstrate that gene knockouts via non-homologous end joining or gene modification via homologous recombination are becoming routine in many plant species. By creating a single genomic DSB, complete knockout of a gene, sequence-specific integration of foreign DNA or subtle modification of individual amino acids in a specific protein domain may be achieved. The induction of two or more DSBs allows complex genomic rearrangements such as deletions, inversions or the exchange of chromosome arms. The potential for controlled genome engineering in plants is tremendous. The recently discovered RNA-based CRISPR/Cas system, a new tool to induce multiple DSBs, and sophisticated technical applications, such as the in planta gene targeting system, are further steps in this development. At present, the focus remains on engineering of single genes; in the future, engineering of whole genomes will become an option.
引用
收藏
页码:727 / 741
页数:15
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