Programmable Synthetic Upstream Activating Sequence Library for Fine-Tuning Gene Expression Levels in Saccharomyces cerevisiae

发起人 上游激活序列 基因 抄写(语言学) 突变体 生物 突变 计算生物学 酿酒酵母 调节顺序 上游(联网) 合成生物学 遗传学 CAAT箱 基因组文库 转录因子 基因表达 计算机科学 肽序列 语言学 哲学 计算机网络
作者
Shiyun Li,Lizhou Ma,Wenxuan Fu,Ruifang Su,Yunying Zhao,Yu Deng
出处
期刊:ACS Synthetic Biology [American Chemical Society]
卷期号:11 (3): 1228-1239 被引量:12
标识
DOI:10.1021/acssynbio.1c00511
摘要

A wide dynamic range of promoters is necessary for fine-tuning transcription levels. However, weak intensity and narrow dynamic range limit transcriptional regulation via constitutive promoters. The upstream activation sequence (UAS) located upstream of the core promoter is a crucial region that could obviously enhance promoter strength. Herein, we created a random mutagenesis library consisting of 330 different variants based on the UAS of the TDH3 promoter with an ∼37-fold dynamic range by error-prone polymerase chain reaction (PCR) and obtained strong intensity mutant UAS, which was ∼12-fold greater than the wild-type UASTDH3. Analysis of the mutant library revealed 15 strength-enhancing sites and their corresponding bases of the UASTDH3 regions, which provided the impetus for a synthetic library. The resulting 32 768 mutant UAS library was constructed by permutation and combination of the bases of the 15 enhancing sites. To characterize the library, a strength prediction model was built by correlating DNA structural features and UAS strength, which provided a model between UAS sequence and intensity. Following characterization, the UAS library was applied to precisely regulate gene expression in the production of β-carotene, proving that the UAS library would be a useful tool for gene tuning in metabolic engineering. In summary, we designed, constructed, and characterized a UAS library that facilitated precise tuning of transcription levels of target proteins.
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