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Introducing a class of standardized and interchangeable parts utilizing programmed ribosomal frameshifts for synthetic biology applications

机译:引入一类利用程序化核糖体移码进行标准化和可互换的零件用于合成生物学应用

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摘要

Synthetic biology and the rational design of biological devices depend on the availability of standardized and interchangeable biological parts with diverse range of functions. Reliable access to different reading frames during translation has largely been overlooked as functionality for bioengineering applications. Here we report the construction and initial characterization of the first member of such a class of biological parts that conforms to the BioBrick Standard (RFC25), allowing its interchangeable use in biological devices. Using our standardized frameshifting signal consisting of a UUUAAAG slippery sequence, a 6 nt spacer and an engineered pseudoknot based on the infectious bronchitis virus pseudoknot PK401 embedded in a dual reporter construct, we confirm that the frameshifting activity is comparable to the previously published frequency despite the introduced sequence changes. The frameshifting activity is demonstrated using SDS-PAGE and fluorescence spectroscopy. Standardized programmable ribosomal frameshift parts with specific frameshifting frequencies will be of utility for applications such as double coding DNA sequences by expanding the codable space into the -1 frame. Programmed shifting into the -1 frame to bypass a stop codon allows labeling of a protein pool with a fixed stoichiometry of fusion protein, as well as the construction of multi-enzyme expression constructs with specific expression ratios. A detailed understanding of the structural basis of programmed frameshifting will provide the opportunities to rationally design frameshifting elements with a wide range of applications in synthetic biology, including signals that are regulated by small ligands.
机译:合成生物学和生物装置的合理设计取决于具有各种功能的标准化和可互换的生物部件的可用性。作为生物工程应用程序的功能,在翻译过程中可靠地访问不同的阅读框已被广泛忽略。在这里,我们报告了符合BioBrick标准(RFC25)的此类生物零件的第一成员的构造和初始表征,可在生物设备中互换使用。使用我们的标准移码信号,该信号由UUUAAAG滑序列,6 nt间隔基和基于嵌入双重报告基因构建体中的传染性支气管炎病毒伪结PK401的工程化假结组成,我们确认移码活性与之前公布的频率相当引入了序列更改。使用SDS-PAGE和荧光光谱法证明了移码活性。具有特定移码频率的标准化可编程核糖体移码部件将通过将可编码空间扩展到-1帧,用于诸如双编码DNA序列的应用。通过程序转换到-1框架以绕过终止密码子,可以用固定的化学计量的融合蛋白标记蛋白质库,并可以构建具有特定表达比例的多酶表达构建体。对程序化移码的结构基础的详细了解将为合理设计移码元素提供机会,在合成生物学中具有广泛的应用,包括受小配体调节的信号。

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