Standardization of inducer-activated broad host range expression modules: debugging and refactoring an alkane-responsive AlkS/PalkB device

IF 3.2 4区 生物学 Q1 Agricultural and Biological Sciences Synthetic Biology Pub Date : 2020-12-26 DOI:10.1093/synbio/ysab030
Alejandro Arce-Rodríguez, Ilaria Benedetti, Rafael Silva-Rocha, V. de Lorenzo
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引用次数: 2

Abstract

Although inducible heterologous expression systems have been available since the birth of recombinant DNA technology, the diversity of devices and genetic architectures of the corresponding vectors have often resulted in a lack of reproducibility and interoperability. In an effort to increase predictability of expression of genes of interest in a variety of possible bacterial hosts we propose a composition standard for debugging and reassembling all regulatory parts that participate in the performance of such devices. As a case study we address the n-octane and dicyclopropyl ketone (DCPK)-inducible PalkB promoter of the alkane biodegradation pOCT plasmid of Pseudomonas putida. The standardized expression module consisted of an edited alkS regulatory gene that is divergently expressed and separated of PalkB by a synthetic DNA buffer sequence. The native DNA sequence of the structural alkS gene was modified to alleviate the catabolite repression exerted by some carbon and nitrogen sources through the Crc/Hfq complex of some hosts. The PalkB promoter along with the alkS variants were then formatted as SEVA (Standard European Vector Architecture) cargoes and their activity parameters in P. putida determined with GFP and luminiscent reporters. The thereby refactored system showed improvements in various features desirable in conditional expression modules: inducibility, capacity, noise reduction and on/off ratio. When applied to other promoter/regulator pairs, the compositional standard thereby implemented in the AlkS/PalkB module will enable more complex genetic programming in non-model bacteria.
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诱导剂激活的宽宿主范围表达模块的标准化:烷烃响应AlkS/PalkB设备的调试和重构
虽然自重组DNA技术诞生以来,已经有了可诱导的异种表达系统,但相应载体的设备和遗传结构的多样性往往导致缺乏可重复性和互操作性。为了提高在各种可能的细菌宿主中感兴趣的基因表达的可预测性,我们提出了一种组合标准,用于调试和重组参与此类设备性能的所有调节部分。作为一个案例研究,我们研究了恶臭假单胞菌烷烃生物降解pOCT质粒的正辛烷和双环丙基酮(DCPK)诱导的PalkB启动子。标准化表达模块由编辑的alkS调控基因组成,该基因通过合成的DNA缓冲序列发散表达并与PalkB分离。结构alkS基因的天然DNA序列被修饰,以减轻一些碳和氮源通过一些宿主的Crc/Hfq复合物对分解代谢的抑制。然后将PalkB启动子和alkS变体格式化为SEVA(欧洲标准载体结构)载体,并使用GFP和发光报告器测定其在恶臭假单胞菌中的活性参数。由此重构的系统在条件表达式模块中表现出各种特性的改进:诱导性、容量、降噪和开/关比。当应用于其他启动子/调控子对时,在AlkS/PalkB模块中实现的组成标准将在非模式细菌中实现更复杂的遗传编程。
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来源期刊
Synthetic Biology
Synthetic Biology Agricultural and Biological Sciences-Agricultural and Biological Sciences (miscellaneous)
CiteScore
4.50
自引率
3.10%
发文量
28
审稿时长
25 weeks
期刊最新文献
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