4.7 Article

Linear DNA for Rapid Prototyping of Synthetic Biological Circuits in an Escherichia coli Based TX-TL Cell-Free System

期刊

ACS SYNTHETIC BIOLOGY
卷 3, 期 6, 页码 387-397

出版社

AMER CHEMICAL SOC
DOI: 10.1021/sb400131a

关键词

rapid prototyping; TX-TL; cell-free expression; synthetic biology; biomolecular breadImarit synthetic gene circuits; Golden Gate assembly; rapid linear DNA assembly

资金

  1. Defense Advanced Research Projects Agency (DARPA/MTO) Living Foundries program [HR0011-12-C-0065]
  2. UCLA/Caltech Medical Scientist Training Program fellowship
  3. National Defense Science and Engineering Graduate fellowships
  4. Direct For Computer & Info Scie & Enginr
  5. Division of Computing and Communication Foundations [1317694] Funding Source: National Science Foundation
  6. Division of Computing and Communication Foundations
  7. Direct For Computer & Info Scie & Enginr [0832824] Funding Source: National Science Foundation

向作者/读者索取更多资源

Accelerating the pace of synthetic biology experiments requires new approaches for rapid prototyping of circuits from individual DNA regulatory elements. However, current testing standards require days to weeks due to cloning and in vivo transformation. In this work, we first characterized methods to protect linear DNA strands from exonuclease degradation in an Escherichia coli based transcription-translation cell-free system (TX-TL), as well as mechanisms of degradation. This enabled the use of linear DNA PCR products in TX-TL. We then compared expression levels and binding dynamics of different promoters on linear DNA and plasmid DNA. We also demonstrated assembly technology to rapidly build circuits entirely in vitro from separate parts. Using this strategy, we prototyped a four component genetic switch in under 8 h entirely in vitro. Rapid in vitro assembly has future applications for pro totyping multiple component circuits if combined with predictive computational models.

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