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通过调节核小体结构设计合成酵母启动子。

Design of synthetic yeast promoters via tuning of nucleosome architecture.

作者信息

Curran Kathleen A, Crook Nathan C, Karim Ashty S, Gupta Akash, Wagman Allison M, Alper Hal S

机构信息

Department of Chemical Engineering, The University of Texas at Austin, 200 E Dean Keeton St. Stop C0400, Austin, TX 78712.

Institute for Cellular and Molecular Biology, The University of Texas at Austin, 2500 Speedway Avenue, Austin, TX 78712.

出版信息

Nat Commun. 2014 May 27;5:4002. doi: 10.1038/ncomms5002.

Abstract

Model-based design of biological parts is a critical goal of synthetic biology, especially for eukaryotes. Here we demonstrate that nucleosome architecture can have a role in defining yeast promoter activity and utilize a computationally-guided approach that can enable both the redesign of endogenous promoter sequences and the de novo design of synthetic promoters. Initially, we use our approach to reprogram native promoters for increased expression and evaluate their performance in various genetic contexts. Increases in expression ranging from 1.5- to nearly 6-fold in a plasmid-based system and up to 16-fold in a genomic context were obtained. Next, we demonstrate that, in a single design cycle, it is possible to create functional, purely synthetic yeast promoters that achieve substantial expression levels (within the top sixth percentile among native yeast promoters). In doing so, this work establishes a unique DNA-level specification of promoter activity and demonstrates predictive design of synthetic parts.

摘要

基于模型的生物部件设计是合成生物学的一个关键目标,对真核生物而言尤其如此。在此,我们证明核小体结构在定义酵母启动子活性方面可发挥作用,并采用一种计算引导方法,该方法既能对内源启动子序列进行重新设计,也能对合成启动子进行从头设计。最初,我们使用我们的方法对天然启动子进行重新编程以提高表达,并在各种遗传背景下评估它们的性能。在基于质粒的系统中,表达增加了1.5至近6倍,在基因组背景下则高达16倍。接下来,我们证明,在单个设计周期内,有可能创建出功能正常、纯合成的酵母启动子,这些启动子能实现相当高的表达水平(在天然酵母启动子的前六分之一百分位之内)。通过这样做,这项工作建立了启动子活性独特的DNA水平规范,并展示了合成部件的预测性设计。

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