Precise single base substitution in the shibire gene by CRISPR/Cas9-mediated homology directed repair in Bactrocera tryoni.

IF 2.9 Q2 Biochemistry, Genetics and Molecular Biology BMC Genetics Pub Date : 2020-12-18 DOI:10.1186/s12863-020-00934-3
Amanda Choo, Elisabeth Fung, Isabel Y Chen, Robert Saint, Peter Crisp, Simon W Baxter
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引用次数: 6

Abstract

Background: Pest eradication using the Sterile Insect Technique (SIT) involves high-density releases of sterilized males that mate with wild females and ultimately suppress the population. Sterilized females are not required for SIT and their removal or separation from males prior to release remains challenging. In order to develop genetic sexing strains (GSS), conditional traits such as temperature sensitive lethality are required.

Results: Here we introduce a known Drosophila melanogaster temperature sensitive embryonic lethal mutation into Bactrocera tryoni, a serious horticultural pest in Australia. A non-synonymous point mutation in the D. melanogaster gene shibire causes embryonic lethality at 29 °C and we successfully used CRISPR/Cas9 technology to recreate the orthologous shibire temperature sensitive-1 (shits1) mutation in B. tryoni. Genotypic analyses over three generations revealed that a high fitness cost was associated with the shits1 mutant allele and shits1 homozygotes were not viable at 21 °C, which is a more severe phenotype than that documented in D. melanogaster.

Conclusions: We have demonstrated the first successful use of CRISPR/Cas9 to introduce precise single base substitutions in an endogenous gene via homology-directed repair in an agricultural pest insect and this technology can be used to trial other conditional mutations for the ultimate aim of generating genetic sexing strains for SIT.

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利用CRISPR/ cas9介导的同源性定向修复技术精确替换特氏小实蝇shibire基因的单碱基。
背景:利用昆虫不育技术(Sterile Insect Technique, SIT)消灭害虫需要高密度释放绝育雄虫与野生雌虫交配,最终抑制种群数量。绝育的雌性不需要进行SIT,在释放之前将它们从雄性中移除或分离仍然具有挑战性。为了培育遗传性别株系(GSS),需要具备温度敏感致死性等条件性状。结果:我们将一种已知的黑腹果蝇温敏胚胎致死性突变引入澳大利亚严重园艺害虫特氏小实蝇(Bactrocera tryoni)。研究人员利用CRISPR/Cas9技术成功地在特氏杆菌中重建了shibire温度敏感-1 (shits1)同源突变。三代基因型分析显示,shits1突变等位基因具有较高的适应度成本,shits1纯合子在21°C下不能存活,这是一种比D. melanogaster更严重的表型。结论:我们首次成功利用CRISPR/Cas9在农业害虫体内通过同源定向修复引入内源基因的精确单碱基替换,该技术可用于试验其他条件突变,最终目的是产生SIT的遗传性别菌株。
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来源期刊
BMC Genetics
BMC Genetics 生物-遗传学
CiteScore
4.30
自引率
0.00%
发文量
77
审稿时长
4-8 weeks
期刊介绍: BMC Genetics is an open access, peer-reviewed journal that considers articles on all aspects of inheritance and variation in individuals and among populations.
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