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首页> 外文期刊>Marine biotechnology >Nitroreductase-mediated Gonadal Dysgenesis for Infertility Control of Genetically Modified Zebrafish
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Nitroreductase-mediated Gonadal Dysgenesis for Infertility Control of Genetically Modified Zebrafish

机译:硝基还原酶介导的性腺发育不全用于转基因斑马鱼的不育控制

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摘要

Genetically modified (GM) fish with desirable features such as rapid growth, disease resistance, and cold tolerance, among other traits, have been established in aquaculture. However, commercially available GM fish are restricted because of global concerns over the incomplete assessments of food safety and ecological impact. The ecological impact concerns include gene flow and escape of the GM fish, which may cause extinction of wild natural fish stocks. Infertility control is a core technology for overcoming this obstacle. Although polyploidy technology, GnRH-specific antisense RNA, and RNAi against GnRH gene expression have been used to cause infertility in fish, these approaches are not 100% reliable and are not heritable. In the present study, zebrafish was used as a model to establish an inducible platform of infertility control in GM fish. Nitroreductase, which converts metronidazole substrate into cytotoxin, was fused with EGFP and expressed specifically by oocytes in the Tg(ZP:NTR-EGFP) by a zona pellucida promoter. Through consecutive immersion of metronidazole from 28 to 42 days posthatching, oocyte-specific EGFP expression was eliminated, and atrophy of the gonads was detected by anatomical analysis. These findings reveal that oocyte-specific nitroreductase-mediated catalysis of metronidazole blocks oogenesis and leads to an undeveloped oocyte. Furthermore, oocyte cell death via apoptosis was detected by a TUNEL assay. We found that the gonadal dysgenesis induced by metronidazole resulted in activation of the ovarian killer gene bok, which is a proapoptotic gene member of the Bcl-2 family and led to infertility. These results show that oocyte-specific nitroreductase-mediated catalysis of metronidazole can cause reliable infertility in zebrafish and could potentially be used as a model for other aquaculture fish species.
机译:在水产养殖中已经建立了具有理想特性(例如快速生长,抗病性和耐寒性)的转基因(GM)鱼。然而,由于全球对食品安全和生态影响的评估不完整,商业上可买到的转基因鱼受到限制。对生态影响的关注包括基因流和转基因鱼的逃逸,这可能导致野生天然鱼种群的灭绝。不育控制是克服这一障碍的一项核心技术。尽管已使用多倍体技术,GnRH特异性反义RNA和针对GnRH基因表达的RNAi引起鱼类不育,但这些方法并非100%可靠且不具有遗传性。在本研究中,斑马鱼被用作建立转基因鱼不育控制的诱导平台的模型。硝基还原酶将甲硝唑底物转化为细胞毒素,与EGFP融合,并通过透明带启动子在Tg(ZP:NTR-EGFP)中的卵母细胞中特异性表达。通过在孵化后28到42天连续浸泡甲硝唑,消除了卵母细胞特异性EGFP表达,并通过解剖学分析检测到性腺萎缩。这些发现表明,卵母细胞特异性硝基还原酶介导的甲硝唑催化作用会阻止卵母细胞发生并导致卵母细胞未发育。此外,通过TUNEL测定法检测了通过凋亡引起的卵母细胞死亡。我们发现甲硝唑诱导的性腺发育不全导致卵巢杀手基因bok的激活,该基因是Bcl-2家族的促凋亡基因成员,并导致不育。这些结果表明,卵母细胞特异性硝基还原酶介导的甲硝唑催化可在斑马鱼中引起可靠的不育,并可潜在地用作其他水产养殖鱼类的模型。

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