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Polyethylene glycol-mediated transformation of fused egfp-hph gene under the control of gpd promoter in Pleurotus eryngii

机译:杏鲍菇gpd启动子控制下的聚乙二醇介导的egfp-hph融合基因转化

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摘要

Pleurotus eryngii was transformed using a polyethylene glycol-mediated method. A plasmid, pEPUGH, containing a reporter gene (enhanced green fluorescent protein gene, egfp) and a positive selectable marker gene (hygromycin phosphotransferase gene, hph) was constructed. The fused egfp-hph gene was placed under the control of the strong and constitutive native gpd promoter from P. eryngii. The recombinant plasmid was used to transform of P. eryngii protoplasts. Successful transformation was demonstrated by molecular analyses. Moreover, the mycelia of the transformants showed green epipolic dispersion on fluorescence microscopy. About 90-210 transformants were produced per mug plasmid DNA per 10~7 viable protoplasts.
机译:用聚乙二醇介导的方法转化杏鲍菇。构建了含有报告基因(增强的绿色荧光蛋白基因,egfp)和阳性选择标记基因(潮霉素磷酸转移酶基因,hph)的质粒pEPUGH。融合的egfp-hph基因被置于来自假单胞菌的强而组成性的天然gpd启动子的控制之下。重组质粒用于转化杏单胞菌的原生质体。分子分析证明成功的转化。此外,转化体的菌丝体在荧光显微镜下显示出绿色的主峰分散。每10-7个活原生质体的每个杯状质粒DNA产生约90-210个转化体。

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