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Stable Nuclear Transformation of the Closterium peracerosum–strigosum–littorale Complex

机译:Peracerosum –strigosum –littorale复合物的稳定核转化

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Although charophycean algae form a relevant monophyly with embryophytes and hence occupy a fundamental place in the development of Streptophyta, no tools for genetic transformation in these organisms have been developed. Here we present the first stable nuclear transformation system for the unicellular Zygnematales, the Closterium peracerosum–strigosum–littorale complex (C. psl complex), which is one of the most useful organisms for experimental research on charophycean algae. When a vector, pSA106, containing the dominant selectable marker ble (phleomycin-resistant) gene and a reporter cgfp (Chlamydomonas-adapted green fluorescent protein) gene was introduced into cells via particle bombardment, a total of 19 phleomycin-resistant cells were obtained in the presence of a low concentration of phleomycin. Six isogenic strains isolated using conditioned medium showed consecutive cgfp expression and long-term stability for phleomycin resistance. DNA analyses verified single or tandem/redundant integration of ∼10 copies of pSA106 into the C. psl complex genome. We also constructed an overexpression vector, pSA1102, and then integrated a CpPI gene encoding minus-specific sex pheromone into pSA1102. Ectopic overexpression of CpPI and the pheromonal function were confirmed when the vector pSA1102_CpPI was introduced into mt+ cells. The present efficient transformation system for the C. psl complex should provide not only a basis for molecular investigation of Closterium but also an insight into important processes in early development and evolution of Streptophyta.
机译:尽管硫藻藻类藻类与胚藻形成了一个相关的单亲生物,因此在链霉菌的发育中占据了根本的地位,但是尚未开发出在这些生物中进行遗传转化的工具。在这里,我们介绍了第一个稳定的单细胞梭菌变态稳定的核转化系统,即梭菌-strigosum-littorale复合物(C. psl复合物),这是对藻类藻类进行实验研究的最有用的生物之一。当通过粒子轰击将包含显性选择标记ble(抗霉素)基因和报告基因cgfp(衣藻的绿色荧光蛋白)基因的载体pSA106导入细胞时,共获得19个抗phleomycin的细胞。低浓度的霉素的存在。使用条件培养基分离的六个同基因菌株显示了连续的cgfp表达和对毛霉素抗性的长期稳定性。 DNA分析证实了约10个拷贝的pSA106单或串联/冗余整合到C. psl复合基因组中。我们还构建了一个过表达载体pSA1102,然后将编码负特异性性信息素的CpPI基因整合到pSA1102中。将载体pSA1102_CpPI导入mt + 细胞后,证实了CpPI的异位表达和信息素功能。目前有效的C. psl复合体转化系统不仅应为梭菌的分子研究提供基础,而且应为链霉菌的早期发育和进化中的重要过程提供见识。

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