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解析用于体外激活转录遗传回路的无细胞提取物制备方法

Deconstructing Cell-Free Extract Preparation for in Vitro Activation of Transcriptional Genetic Circuitry.

作者信息

Silverman Adam D, Kelley-Loughnane Nancy, Lucks Julius B, Jewett Michael C

机构信息

711th Human Performance Wing , Air Force Research Laboratory , Wright-Patterson Air Force Base , Ohio 45433 , United States.

Interdisciplinary Biological Sciences Program , Northwestern University , Evanston , Illinois 60208 , United States.

出版信息

ACS Synth Biol. 2019 Feb 15;8(2):403-414. doi: 10.1021/acssynbio.8b00430. Epub 2019 Jan 29.

Abstract

Recent advances in cell-free gene expression (CFE) systems have enabled their use for a host of synthetic biology applications, particularly for rapid prototyping of genetic circuits and biosensors. Despite the proliferation of cell-free protein synthesis platforms, the large number of currently existing protocols for making CFE extracts muddles the collective understanding of how the extract preparation method affects its functionality. A key aspect of extract performance relevant to many applications is the activity of the native host transcriptional machinery that can mediate protein synthesis. However, protein yields from genes transcribed in vitro by the native Escherichia coli RNA polymerase are variable for different extract preparation techniques, and specifically low in some conventional crude extracts originally optimized for expression by the bacteriophage transcriptional machinery. Here, we show that cell-free expression of genes under bacterial σ promoters is constrained by the rate of transcription in crude extracts, and that processing the extract with a ribosomal runoff reaction and subsequent dialysis alleviates this constraint. Surprisingly, these processing steps only enhance protein synthesis in genes under native regulation, indicating that the translation rate is unaffected. We further investigate the role of other common extract preparation process variants on extract performance and demonstrate that bacterial transcription is inhibited by including glucose in the growth culture but is unaffected by flash-freezing the cell pellet prior to lysis. Our final streamlined and detailed protocol for preparing extract by sonication generates extract that facilitates expression from a diverse set of sensing modalities including protein and RNA regulators. We anticipate that this work will clarify the methodology for generating CFE extracts that are active for biosensing using native transcriptional machinery and will encourage the further proliferation of cell-free gene expression technology for new applications.

摘要

无细胞基因表达(CFE)系统的最新进展使其能够用于一系列合成生物学应用,特别是用于遗传电路和生物传感器的快速原型制作。尽管无细胞蛋白质合成平台不断涌现,但目前大量用于制备CFE提取物的现有方案却让人们对提取物制备方法如何影响其功能的总体理解变得模糊不清。与许多应用相关的提取物性能的一个关键方面是能够介导蛋白质合成的天然宿主转录机制的活性。然而,对于不同的提取物制备技术,由天然大肠杆菌RNA聚合酶体外转录的基因所产生的蛋白质产量存在差异,并且在一些最初为噬菌体转录机制表达而优化的传统粗提取物中产量特别低。在这里,我们表明细菌σ启动子下基因的无细胞表达受到粗提取物中转录速率的限制,并且通过核糖体延伸反应和随后的透析处理提取物可以缓解这种限制。令人惊讶的是,这些处理步骤仅增强了天然调控下基因的蛋白质合成,这表明翻译速率不受影响。我们进一步研究了其他常见的提取物制备过程变量对提取物性能的作用,并证明在生长培养物中加入葡萄糖会抑制细菌转录,但在裂解前对细胞沉淀进行速冻则不会影响细菌转录。我们最终通过超声处理制备提取物的简化且详细的方案所产生的提取物有助于从包括蛋白质和RNA调节剂在内的多种传感模式进行表达。我们预计这项工作将阐明使用天然转录机制生成对生物传感具有活性的CFE提取物的方法,并将鼓励无细胞基因表达技术在新应用中的进一步推广。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/24a5/6584022/af34f3077631/nihms-1034937-f0002.jpg

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