CRISPR-transient expression in soybean for simplified gRNA screening in planta

被引:0
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作者
Koltun, Alessandra [1 ]
Volpi e Silva, Nathalia [2 ]
Angelotti-Mendonca, Jessika
Marin, Silvana Regina Rockenbach [2 ]
Goncalves, Leandro Simoes Azeredo [2 ]
Nepomuceno, Alexandre Lima [3 ]
Mertz-Henning, Liliane Marcia [2 ]
机构
[1] Univ Estadual Maringa, Ctr Ciencias Agr, Ave Colombo 5-790,Bloco J45, BR-87020900 Maringa, Parana, Brazil
[2] Embrapa Soja, Rodovia Carlos Joao St S-N,Caixa Postal 4006, BR-86085981 Maringa, Parana, Brazil
[3] Univ Estadual Londrina, Rodovia Celso Garcia Cid,PR 445,Km 380, BR-86057970 Londrina, Parana, Brazil
关键词
Index terms; Glycine max; CRISPR vector construction; gRNA validation; mutation detection;
D O I
10.1590/S1678-3921.pab2023.v58.03000
中图分类号
S [农业科学];
学科分类号
09 ;
摘要
The objective of this work was to develop a method to create and validate CRISPR-Cas systems and different gRNAs in soybean (Glycine max) embryos. Two model genes were used for simple mutation with one gRNA or partial gene deletion with two guides. The gRNAs were inserted into the CRISPR transformation vectors by a type IIS restriction enzyme or by subcloning and inserting the promoter + gRNA2 in the final transformation vector using the classic restriction enzyme cloning method. The vectors were successfully constructed for one and two gRNAs. Agrobacterium-mediated transient transformation in soybean was carried out to test the quality of gRNAs and of the system itself (expression cassette). Simple mutation and gene deletion were detected in the embryos transformed after DNA enrichment by enzyme digestion followed by polymerase chain reaction and sequencing, which indicates that the CRISPR-Cas system and guides were working. This protocol can be used to accelerate CRISPR-based genome editing strategies for genetic transformation in soybean.
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页数:10
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