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Novel S. cerevisiae Hybrid Synthetic Promoters Based on Foreign Core Promoter Sequences

机译:基于外核促进剂序列的新型S.酿酒酵母杂化综合启动子

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摘要

Promoters are fundamental components of synthetic gene circuits. They are DNA segments where transcription initiation takes place. New constitutive and regulated promoters are constantly engineered in order to meet the requirements for protein and RNA expression into different genetic networks. In this work, we constructed and optimized new synthetic constitutive promoters for the yeast Saccharomyces cerevisiae. We started from foreign (e.g., viral) core promoters as templates. They are, usually, unfunctional in yeast but can be activated by extending them with a short sequence, from the CYC1 promoter, containing various transcription start sites (TSSs). Transcription was modulated by mutating the TATA box composition and varying its distance from the TSS. We found that gene expression is maximized when the TATA box has the form TATAAAA or TATATAA and lies between 30 and 70 nucleotides upstream of the TSS. Core promoters were turned into stronger promoters via the addition of a short UAS. In particular, the 40 nt bipartite UAS from the GPD promoter can enhance protein synthesis considerably when placed 150 nt upstream of the TATA box. Overall, we extended the pool of S. cerevisiae promoters with 59 new samples, the strongest overcoming the native TEF2 promoter.
机译:促进剂是合成基因电路的基本组分。它们是转录启动发生的DNA段。新的组成型和监管启动子被持续设计,以满足蛋白质和RNA表达到不同遗传网络的要求。在这项工作中,我们为酵母酿酒酵母构建和优化了新的合成组成型启动子。我们从外国(例如病毒)核心启动子开始作为模板。通常,通常,酵母中的未官能化,但可以通过从CYC1启动子延伸它们的短序列来激活,含有各种转录起始位点(TSSS)。通过突变塔塔盒组合物并改变其距TSS的距离来调节转录。我们发现当塔塔盒具有TataAAA或TatataA的形成时,基因表达最大化,并且位于TSS上游的30至70个核苷酸之间。通过添加短UAS将核心启动子变成更强的启动子。特别地,来自GPD启动子的40nt二分uA可以在放置在塔塔箱的上游150nt时显着增强蛋白质合成。总的来说,我们用59种新样品延伸了S.酿酒酵母促进剂的池,最强大的克服天然TEF2启动子。

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