4.7 Article

Optimization and compartmentalization of a cell-free mixture of DNA amplification and protein translation

Journal

APPLIED MICROBIOLOGY AND BIOTECHNOLOGY
Volume 106, Issue 24, Pages 8139-8149

Publisher

SPRINGER
DOI: 10.1007/s00253-022-12278-2

Keywords

Cell-free system; Replication-cycle reaction; Protein translation; Compartmentalization; Droplets

Funding

  1. National Key R&D Program of China, Synthetic Biology Research [2019YFA0904500]
  2. China Postdoctoral Science Foundation [2021M691034]

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Recent studies have shown the importance of the reconstituted cell-free DNA replisome and in vitro transcription and translation systems from Escherichia coli in applied and synthetic biology. This study combines these two systems and evaluates their compatibility and performance, showing that optimized reaction buffers can improve their performance and provide new avenues for rewiring the central dogma of molecular biology in synthetic cell models.
Recent studies have shown that the reconstituted cell-free DNA replisome and in vitro transcription and translation systems from Escherichia coli are highly important in applied and synthetic biology. To date, no attempt has been made to combine those two systems. Here, we study the performance of the mixed two separately exploited systems commercially available as RCR and PURE systems. Regarding the genetic information flow from DNA to proteins, mixtures with various ratios of RCR/PURE gave low protein expression, possibly due to the well-known conflict between replication and transcription or inappropriate buffer conditions. To further increase the compatibility of the two systems, rationally designed reaction buffers with a lower concentration of nucleoside triphosphates in 50 mM HEPES (pH7.6) were evaluated, showing increased performance from RCR/PURE (85%/15%) in a time-dependent manner. The compatibility was also validated in compartmentalized cell-sized droplets encapsulating the same RCR/PURE soup. Our findings can help to better fine-tune the reaction conditions of RCR-PURE systems and provide new avenues for rewiring the central dogma of molecular biology as self-sustaining systems in synthetic cell models.

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