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Fine-Tuning of Photoautotrophic Protein Production by Combining Promoters and Neutral Sites in the Cyanobacterium Synechocystis sp. Strain PCC 6803

机译:通过结合启动子和蓝藻中性位点的微调光合自养蛋白生产。应变PCC 6803

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摘要

Cyanobacteria are photosynthetic cell factories that use solar energy to convert CO2 into useful products. Despite this attractive feature, the development of tools for engineering cyanobacterial chassis has lagged behind that for heterotrophs such as Escherichia coli or Saccharomyces cerevisiae. Heterologous genes in cyanobacteria are often integrated at presumptively “neutral” chromosomal sites, with unknown effects. We used transcriptome sequencing (RNA-seq) data for the model cyanobacterium Synechocystis sp. strain PCC 6803 to identify neutral sites from which no transcripts are expressed. We characterized the two largest such sites on the chromosome, a site on an endogenous plasmid, and a shuttle vector by integrating an enhanced yellow fluorescent protein (EYFP) expression cassette expressed from either the Pcpc560 or the Ptrc1O promoter into each locus. Expression from the endogenous plasmid was as much as 14-fold higher than that from the chromosome, with intermediate expression from the shuttle vector. The expression characteristics of each locus correlated predictably with the promoters used. These findings provide novel, characterized tools for synthetic biology and metabolic engineering in cyanobacteria.
机译:蓝细菌是光合作用的细胞工厂,利用太阳能将二氧化碳转化为有用的产品。尽管具有这一吸引人的功能,但用于工程化蓝细菌底盘的工具的开发却落后于诸如大肠杆菌或酿酒酵母等异养生物的工具。蓝细菌中的异源基因通常整合在推测为“中性”的染色体位点,其作用未知。我们使用了转录组测序(RNA-seq)数据,用于模型蓝藻集胞藻属sp。株PCC 6803,以鉴定没有转录本的中性位点。我们通过整合从Pcpc560或Ptrc10O启动子表达的增强型黄色荧光蛋白(EYFP)表达盒,将染色体上两个最大的此类位点,内源质粒上的位点和穿梭载体进行了表征。来自内源质粒的表达比来自染色体的表达高14倍,而来自穿梭载体的表达则中等。每个基因座的表达特征与使用的启动子可预测地相关。这些发现为蓝细菌的合成生物学和代谢工程提供了新颖,特征化的工具。

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