Generating Cyclin M2(CNNM2) knockout zebrafish using CRISPR/Cas9 system
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College of Fisheries and Life Science,Shanghai Ocean University,College of Fisheries and Life Science,Shanghai Ocean University,College of Fisheries and Life Science,Shanghai Ocean University,College of Fisheries and Life Science,Shanghai Ocean University

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    Abstract:

    Cyclin M2(CNNM2) is one of the regulatory transport genes involved in zebrafish Mg2+ homeostasis. We generated CNNM2 gene knockout zebrafish by CRISPR/Cas9 system which has been developed into a novel gene targeting system in recent years.First, we constructed the sgRNA expression vector targeting zebrafish CNNM2 gene. Then, after in vitro transcription of sgRNA and Cas9 vectors, we co-injected them into one-cell fertilized eggs of zebrafish to generate zebrafish with targeted mutation. After 24-48 h, injected embryos were collected and used to conduct mutation analysis with restriction endonuclease and sequencing. To further verify the stability of genetic mutations, we selected mutated founder to outcross with wild type zebrafish. A knockout and wild-type outcross F0 efficiency were obtained, and then F1 were analyzed by PCR and sequencing of the caudal fin. The results showed F0 and F1 were introduced insertion, deletion and frameshift mutations to some extent, and F0 mutation efficiency was 88%. The CNNM2 gene knockout zebrafish generated in this study can be transmitted by germline and provide a basis for further study of CNNM2 and Mg2+ homeostasis.

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黄振玉,竹个个,邹华锋,吕为群.利用CRISPR/Cas9敲除斑马鱼细胞周期蛋白M2(CNNM2)基因[J].上海海洋大学学报,2015,24(6):810-816.
HUANG Zhenyu, ZHU Gege, ZOU Huafeng, L&#; Weiqun. Generating Cyclin M2(CNNM2) knockout zebrafish using CRISPR/Cas9 system[J]. Journal of Shanghai Ocean University,2015,24(6):810-816.

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History
  • Received:March 13,2015
  • Revised:June 26,2015
  • Adopted:September 09,2015
  • Online: December 01,2015
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