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Efficient CRISPR/Cas9-mediated gene editing in Guangdong small-ear spotted pig cells using an optimized electrotransfection method

机译:高效的CRISPR / CAS9介导的基因在广东小耳斑猪细胞中使用优化的电扫描方法编辑

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摘要

Objectives Guangdong Small-ear Spotted (GDSS) pigs are a pig breed native to China that possesses unfortunate disadvantages, such as slow growth rate, low lean-meat percentage, and reduced feed utilization. In contrast to traditional genetic breeding methods with long cycle time and high cost, CRISPR/Cas9-mediated gene editing for the modification of the pig genome can quickly improve production traits, and therefore this technique exhibits important potential in the genetic improvement and resource development of GDSS pigs. In the present study, we aimed to establish an efficient CRISPR/Cas9-mediated gene-editing system for GDSS pig cells by optimizing the electrotransfection parameters, and to realize efficient CRISPR/Cas9-mediated gene editing of GDSS pig cells. Results After optimization of electrotransfection parameters for the transfection of GDSS pig cells, we demonstrated that a voltage of 150 V and a single pulse with a pulse duration of 20 ms were the optimal electrotransfection parameters for gene editing in these cells. In addition, our study generated GDSS pig single-cell colonies with biallelic mutations in the myostatin (MSTN) gene and insulin-like growth factor 2 (IGF2) intron-3 locus, which play an important role in pig muscle growth and muscle development. The single-cell colonies showed no foreign gene integration or off-target effects, and maintained normal cell morphology and viability. These gene-edited, single-cell colonies can in the future be used as donor cells to generate MSTN- and IGF2-edited GDSS pigs using somatic cell nuclear transfer (SCNT). Conclusions This study establishes the foundation for genetic improvement and resource development of GDSS pigs using CRISPR/Cas9-mediated gene editing combined with SCNT.
机译:目的广东小耳朵斑点(GDSS)猪是中国原产的猪种,具有不幸的缺点,如缓慢的增长率,低瘦肉百分比和减少的饲料利用率。与具有长循环时间和高成本的传统遗传育种方法相比,CRISPR / CAS9介导的基因编辑用于猪基因组的改性可以迅速提高生产性状,因此该技术在遗传改善和资源开发中表现出重要的潜力GDSS猪。在本研究中,我们旨在通过优化电流反应参数来建立用于GDSS猪细胞的有效的CRISPR / CAS9介导的基因编辑系统,并实现GDSS猪细胞的有效CRISPR / CAS9介导的基因编辑。结果在优化电粉猪细胞转染的电流反应参数后,我们证明了150V的电压和脉冲持续时间为20 ms的单个脉冲是用于这些细胞中基因编辑的最佳电流反应参数。此外,我们的研究在肌抑素(MSTN)基因(MSTN)基因和胰岛素样生长因子2(IGF2)内含子 - 3个基因座中生成了具有双胞胎突变的GDS猪单细胞菌落,这在猪肌肉生长和肌肉发育中起重要作用。单细胞菌落显示出外部基因整合或脱靶效果,并保持正常的细胞形态和活力。这些基因编辑的单细胞菌落可以在将来用作供体细胞使用体细胞核转移(SCNT)产生MSTN-和IGF2编辑的GDSS猪。结论本研究建立了使用CRISPR / CAS9介导的基因编辑与SCNT联合使用CRISPR / CAS9介导的GDSS猪的遗传改善和资源开发的基础。

著录项

  • 来源
    《Biotechnology Letters》 |2020年第11期|共19页
  • 作者单位

    Foshan Univ Sch Life Sci &

    Engn Guangdong Prov Key Lab Anim Mol Design &

    Precise Foshan 528225 Peoples R China;

    Foshan Univ Sch Life Sci &

    Engn Guangdong Prov Key Lab Anim Mol Design &

    Precise Foshan 528225 Peoples R China;

    Foshan Univ Guangdong Prov Engn &

    Technol Res Ctr Gene Editin Sch Med Engn Foshan 528225 Peoples R China;

    Foshan Univ Sch Life Sci &

    Engn Guangdong Prov Key Lab Anim Mol Design &

    Precise Foshan 528225 Peoples R China;

    Foshan Univ Guangdong Prov Engn &

    Technol Res Ctr Gene Editin Sch Med Engn Foshan 528225 Peoples R China;

    Foshan Univ Guangdong Prov Engn &

    Technol Res Ctr Gene Editin Sch Med Engn Foshan 528225 Peoples R China;

    Guangdong Acad Agr Sci Inst Anim Sci State Key Lab Livestock &

    Poultry Breeding Guangdong Key Lab Anim Breeding &

    Nutr Guangzhou 510640 Peoples R China;

    Foshan Univ Sch Life Sci &

    Engn Guangdong Prov Key Lab Anim Mol Design &

    Precise Foshan 528225 Peoples R China;

  • 收录信息
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 分子生物学;
  • 关键词

    CRISPR; Cas9-mediated gene editing; Myostatin (MSTN); Insulin-like growth factor 2 (IGF2); Guangdong small-ear spotted (GDSS) pig; Electrotransfection;

    机译:CRISPR;CAS9介导的基因编辑;肌肉素(MSTN);胰岛素样生长因子2(IGF2);广东小耳朵斑点(GDSS)猪;电力反应;

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