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利用无细胞蛋白合成技术进行柠檬烯生物合成的体外原型设计。

In vitro prototyping of limonene biosynthesis using cell-free protein synthesis.

机构信息

Department of Chemical and Biological Engineering and Center for Synthetic Biology, Northwestern University, Evanston, IL, 60208, USA.

Department of Chemical and Biological Engineering and Center for Synthetic Biology, Northwestern University, Evanston, IL, 60208, USA.

出版信息

Metab Eng. 2020 Sep;61:251-260. doi: 10.1016/j.ymben.2020.05.006. Epub 2020 May 25.

DOI:10.1016/j.ymben.2020.05.006
PMID:32464283
Abstract

Metabolic engineering of microorganisms to produce sustainable chemicals has emerged as an important part of the global bioeconomy. Unfortunately, efforts to design and engineer microbial cell factories are challenging because design-build-test cycles, iterations of re-engineering organisms to test and optimize new sets of enzymes, are slow. To alleviate this challenge, we demonstrate a cell-free approach termed in vitro Prototyping and Rapid Optimization of Biosynthetic Enzymes (or iPROBE). In iPROBE, a large number of pathway combinations can be rapidly built and optimized. The key idea is to use cell-free protein synthesis (CFPS) to manufacture pathway enzymes in separate reactions that are then mixed to modularly assemble multiple, distinct biosynthetic pathways. As a model, we apply our approach to the 9-step heterologous enzyme pathway to limonene in extracts from Escherichia coli. In iterative cycles of design, we studied the impact of 54 enzyme homologs, multiple enzyme levels, and cofactor concentrations on pathway performance. In total, we screened over 150 unique sets of enzymes in 580 unique pathway conditions to increase limonene production in 24 h from 0.2 to 4.5 mM (23-610 mg/L). Finally, to demonstrate the modularity of this pathway, we also synthesized the biofuel precursors pinene and bisabolene. We anticipate that iPROBE will accelerate design-build-test cycles for metabolic engineering, enabling data-driven multiplexed cell-free methods for testing large combinations of biosynthetic enzymes to inform cellular design.

摘要

微生物代谢工程已成为全球生物经济的重要组成部分,用于生产可持续化学品。然而,设计和工程微生物细胞工厂的努力具有挑战性,因为设计-构建-测试周期(即重新设计生物体以测试和优化新酶组的迭代)缓慢。为了缓解这一挑战,我们展示了一种称为体外原型设计和快速优化生物合成酶(iPROBE)的无细胞方法。在 iPROBE 中,可以快速构建和优化大量的途径组合。其关键思想是使用无细胞蛋白合成(CFPS)在单独的反应中制造途径酶,然后将这些反应混合以模块化地组装多个不同的生物合成途径。作为一个模型,我们将我们的方法应用于来自大肠杆菌的提取物中的 9 步异源酶途径来生产柠檬烯。在设计的迭代循环中,我们研究了 54 种酶同源物、多种酶水平和辅因子浓度对途径性能的影响。总的来说,我们在 580 种独特的途径条件下筛选了超过 150 种独特的酶组合,将柠檬烯的产量从 24 小时的 0.2 毫摩尔增加到 4.5 毫摩尔(23-610 毫克/升)。最后,为了展示该途径的模块化,我们还合成了生物燃料前体蒎烯和双醇烯。我们预计 iPROBE 将加速代谢工程的设计-构建-测试循环,实现基于数据的多路复用无细胞方法来测试大量生物合成酶,从而为细胞设计提供信息。

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