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Chloroplast Transformation of Platymonas (Tetraselmis) subcordiformis with the bar Gene as Selectable Marker

机译:bar基因为选择标记的桔梗侧叶绿体的叶绿体转化

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摘要

The objective of this research was to establish a chloroplast transformation technique for Platymonas (Tetraselmis) subcordiformis. Employing the gfp gene as a reporter and the bar gene as a selectable marker, transformation vectors of P. subcordiformis chloroplast were constructed with endogenous fragments rrn16S-trnl (left) and trnA-rrn23S (right) as a recombination site of the chloroplast genome. The plasmids were transferred into P. subcordiformis via particle bombardment. Confocal laser scanning microscopy indicated that the green fluorescence protein was localized in the chloroplast of P. subcordiformis, confirming the activity of the Chlamydomonas reinhardtii promoter. Cells transformed with the bar gene were selected using the herbicide Basta. Resistant colonies were analyzed by PCR and Southern blotting, and the results indicated that the bar gene was successfully integrated into the chloroplast genome via homologous recombination. The technique will improve genetic engineering of this alga.
机译:这项研究的目的是建立叶绿体(Petraselmis)皮下分离的叶绿体转化技术。利用gfp基因作为报告基因,bar基因作为选择标记,构建了带有内源性片段rrn16S-trnl(左)和trnA-rrn23S(右)作为叶绿体基因组重组位点的次球形叶绿体的转化载体。通过粒子轰击将质粒转移到皮下假单胞菌中。共聚焦激光扫描显微镜检查表明绿色荧光蛋白位于皮下假单胞菌的叶绿体中,证实了莱茵衣藻启动子的活性。使用除草剂Basta选择用bar基因转化的细胞。通过PCR和Southern印迹分析抗性菌落,结果表明bar基因通过同源重组成功整合到叶绿体基因组中。该技术将改善这种藻类的基因工程。

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