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首页> 外文期刊>Molecules >Application of the Cre/loxP Site-Specific Recombination System for Gene Transformation in Aurantiochytrium limacinum
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Application of the Cre/loxP Site-Specific Recombination System for Gene Transformation in Aurantiochytrium limacinum

机译:Cre / loxP位点特异性重组系统在淡金金鱼中进行基因转化的应用

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摘要

The Cre/loxP site-specific recombination system was applied to Aurantiochytrium limacinum to obtain a transformant without the antibiotic resistance marker gene. First, the enhanced green fluorescent protein gene (egfp) and chloramphenicol resistance gene (Cm-r), along with the two loxP loci, were integrated into the genome of A. limacinum OUC88 using 18S rDNA sequences as the homologous recombination sites. Then plasmid pSH65, containing a zeocin resistance gene (Ble(r)) was transferred into A. limacinum OUC_CG. After induction with galactose, repeated passage in culture and PCR-based assessment, the pSH65 plasmid was lost and A. limacinum OUC_EG host was shown to no longer have resistance to 100 mg chloramphenicol/L or 5 mg zeocin/L. Through southern blotting and fluorescence detection, egfp was found to be integrated into the genome of A. limacinum OUC_EG, and EGFP was successfully expressed in the cells. The successful application of the Cre/loxP system demonstrates an experimental basis for genetic modification of A. limacinum so as to obtain transformed strains with no antibiotic resistance marker genes.
机译:将Cre / loxP位点特异性重组系统应用于淡红金鱼(Aurantiochytrium limacinum),以获得不含抗生素抗性标记基因的转化体。首先,使用18S rDNA序列作为同源重组位点,将增强的绿色荧光蛋白基因(egfp)和氯霉素抗性基因(Cm-r)以及两个loxP基因座整合到A. limacinum OUC88的基因组中。然后将含有博来霉素抗性基因(Ble(r))的质粒pSH65转移到青曲霉OUC_CG中。用半乳糖诱导后,在培养中反复传代并进行基于PCR的评估,pSH65质粒丢失,并且显示青果曲霉OUC_EG宿主不再对100 mg氯霉素/ L或5 mg zeocin / L具有抗性。通过Southern印迹和荧光检测,发现egfp已整合到青曲霉OUC_EG的基因组中,并在细胞中成功表达了EGFP。 Cre / loxP系统的成功应用证明了对金黄色葡萄球菌进行基因修饰以获得无抗生素抗性标记基因的转化菌株的实验基础。

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