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Expression of heterologous sigma factors enables functional screening of metagenomic and heterologous genomic libraries

机译:异源sigma因子的表达可对宏基因组和异源基因组文库进行功能筛选

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摘要

A key limitation in using heterologous genomic or metagenomic libraries in functional genomics and genome engineering is the low expression of heterologous genes in screening hosts, such as Escherichia coli. To overcome this limitation, here we generate E. coli strains capable of recognizing heterologous promoters by expressing heterologous sigma factors. Among seven sigma factors tested, RpoD from Lactobacillus plantarum (Lpl) appears to be able of initiating transcription from all sources of DNA. Using the promoter GFP-trap concept, we successfully screen several heterologous and metagenomic DNA libraries, thus enlarging the genomic space that can be functionally sampled in E. coli. For an application, we show that screening fosmid-based Lpl genomic libraries in an E. coli strain with a chromosomally integrated Lpl rpoD enables the identification of Lpl genetic determinants imparting strong ethanol tolerance in E. coli. Transcriptome analysis confirms increased expression of heterologous genes in the engineered strain.
机译:在功能基因组学和基因组工程中使用异源基因组或宏基因组库的关键限制是异源基因在筛选宿主(如大肠杆菌)中的低表达。为了克服这个限制,在这里我们产生了能够通过表达异源σ因子识别异源启动子的大肠杆菌菌株。在测试的七个sigma因子中,植物乳杆菌(Lpl)的RpoD似乎能够启动所有DNA来源的转录。使用启动子GFP捕集器概念,我们成功地筛选了几个异源和宏基因组DNA库,从而扩大了可在大肠杆菌中进行功能采样的基因组空间。对于一个应用程序,我们表明在具有染色体整合的Lpl rpoD的大肠杆菌菌株中筛选基于化石的Lpl基因组文库可以鉴定在大肠杆菌中具有强大乙醇耐受性的Lpl基因决定簇。转录组分析证实了工程菌株中异源基因的表达增加。

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