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CRISPR-Cas9靶向诱变导致多倍体油菜中不同同源基因拷贝的同时修饰()。

CRISPR-Cas9 Targeted Mutagenesis Leads to Simultaneous Modification of Different Homoeologous Gene Copies in Polyploid Oilseed Rape ().

作者信息

Braatz Janina, Harloff Hans-Joachim, Mascher Martin, Stein Nils, Himmelbach Axel, Jung Christian

机构信息

Plant Breeding Institute, Christian-Albrechts-University of Kiel, 24098 Kiel, Germany (J.B., H.-J.H., C.J.).

Leibniz Institute of Plant Genetics and Crop Plant Research Gatersleben, 06466 Stadt Seeland, Germany (M.M., N.S., A.H.); and.

出版信息

Plant Physiol. 2017 Jun;174(2):935-942. doi: 10.1104/pp.17.00426. Epub 2017 Apr 18.

Abstract

In polyploid species, altering a trait by random mutagenesis is highly inefficient due to gene redundancy. We have stably transformed tetraploid oilseed rape () with a CRISPR-Cas9 construct targeting two () homoeologs. is involved in valve margin development and, thus, contributes to seed shattering from mature fruits. Knocking out would increase shatter resistance to avoid seed loss during mechanical harvest. We obtained a transgenic T1 plant with four mutant alleles by the use of a single target sequence. All mutations were stably inherited to the T2 progeny. The T2 generation was devoid of any wild-type alleles, proving that the underlying T1 was a nonchimeric double heterozygote. T-DNA and loci were not linked, as indicated by random segregation in the T2 generation. Hence, we could select double mutants lacking the T-DNA already in the first offspring generation. However, whole-genome sequencing data revealed at least five independent insertions of vector backbone sequences. We did not detect any off-target effects in two genome regions homologous to the target sequence. The simultaneous alteration of multiple homoeologs by CRISPR-Cas9 mutagenesis without any background mutations will offer new opportunities for using mutant genotypes in rapeseed breeding.

摘要

在多倍体物种中,由于基因冗余,通过随机诱变改变性状的效率非常低。我们用靶向两个 () 同源基因的CRISPR-Cas9构建体稳定转化了四倍体油菜()。 参与瓣膜边缘发育,因此,导致成熟果实中的种子散落。敲除 将增加抗散落性,以避免机械收获期间的种子损失。通过使用单个靶序列,我们获得了具有四个 突变等位基因的转基因T1植株。所有突变都稳定遗传到T2后代。T2代没有任何野生型等位基因,证明潜在的T1是一个非嵌合双杂合子。如T2代中的随机分离所示,T-DNA和 位点没有连锁。因此,我们可以在第一代后代中选择已经缺失T-DNA的双突变体。然而,全基因组测序数据显示载体骨架序列至少有五个独立插入。我们在与靶序列同源的两个基因组区域中未检测到任何脱靶效应。通过CRISPR-Cas9诱变同时改变多个同源基因而没有任何背景突变,将为在油菜育种中使用突变基因型提供新的机会。

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