设计、构建和表征放线菌中精细基因表达的合成启动子文库。

Design, construction and characterisation of a synthetic promoter library for fine-tuned gene expression in actinomycetes.

机构信息

Albert-Ludwigs-University of Freiburg, Pharmaceutical Biology and Biotechnology, Stefan-Meier-st. 19, Freiburg 79104, Germany.

出版信息

Metab Eng. 2013 Sep;19:98-106. doi: 10.1016/j.ymben.2013.07.006. Epub 2013 Jul 20.

DOI:10.1016/j.ymben.2013.07.006

PMID:23876413

Abstract

We developed a synthetic promoter library for actinomycetes based on the -10 and -35 consensus sequences of the constitutive and widely used ermEp1 promoter. The sequences located upstream, in between and downstream of these consensus sequences were randomised using degenerate primers and cloned into an integrative plasmid upstream of the gusA reporter gene. Using this system, we created promoters with strengths ranging from 2% to 319% compared with ermEp1. The strongest synthetic promoter was used in a proof-of-principle approach to achieve the overexpression of a natural type III polyketide synthase. We observed high correlation between the number of gusA reporter gene RNA-Seq reads and the GusA reporter protein activity, indicating that GusA is indeed a transcription-level reporter system.

摘要

我们基于组成型且广泛使用的 ermEp1 启动子的-10 和-35 共识序列，为放线菌开发了一个合成启动子文库。这些共识序列上游、之间和下游的序列使用简并引物随机化，并克隆到 gusA 报告基因的整合质粒上游。使用该系统，我们创建了与 ermEp1 相比强度从 2%到 319%的启动子。最强的合成启动子用于原理验证方法，以实现天然 III 型聚酮合酶的过表达。我们观察到 GusA 报告基因 RNA-Seq 读数的数量与 GusA 报告蛋白活性之间高度相关，表明 GusA 确实是一个转录水平的报告系统。

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设计、构建和表征放线菌中精细基因表达的合成启动子文库。

Design, construction and characterisation of a synthetic promoter library for fine-tuned gene expression in actinomycetes.

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