4.8 Article

In vitro DNA SCRaMbLE

期刊

NATURE COMMUNICATIONS
卷 9, 期 -, 页码 -

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NATURE PORTFOLIO
DOI: 10.1038/s41467-018-03743-6

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资金

  1. National Natural Science Foundation of China [21750001, 21621004, 21676192]
  2. Ministry of Science and Technology of China (973 Program) [2014CB745100]
  3. International S&T Cooperation Program of China [2015DFA00960]
  4. NSF [MCB-1026068, MCB-1158201]
  5. Div Of Molecular and Cellular Bioscience
  6. Direct For Biological Sciences [1616111] Funding Source: National Science Foundation

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The power of synthetic biology has enabled the expression of heterologous pathways in cells, as well as genome-scale synthesis projects. The complexity of biological networks makes rational de novo design a grand challenge. Introducing features that confer genetic flexibility is a powerful strategy for downstream engineering. Here we develop an in vitro method of DNA library construction based on structural variation to accomplish this goal. The in vitro SCRaMbLE system uses Cre recombinase mixed in a test tube with purified DNA encoding multiple loxPsym sites. Using a beta-carotene pathway designed for expression in yeast as an example, we demonstrate top-down and bottom-up in vitro SCRaMbLE, enabling optimization of biosynthetic pathway flux via the rearrangement of relevant transcription units. We show that our system provides a straightforward way to correlate phenotype and genotype and is potentially amenable to biochemical optimization in ways that the in vivo system cannot achieve.

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