4.8 Article

biGBac enables rapid gene assembly for the expression of large multisubunit protein complexes

Publisher

NATL ACAD SCIENCES
DOI: 10.1073/pnas.1604935113

Keywords

protein complexes; baculovirus-insect cell expression; Gibson assembly

Funding

  1. Boehringer Ingelheim
  2. Austrian Research Promotion Agency (FFG Laura Bassi Centre for Optimized Structural Studies)
  3. European Union [227764]
  4. Austrian Science Fund (SFB-F34)
  5. Deutsche Forschungsgemeinschaft [Sonderforschungsbereich 860]
  6. Jane Coffin Childs Foundation
  7. Leukemia AMP
  8. Lymphoma Society
  9. American Lebanese Syrian Associated Charities
  10. NIH [R37GM065930, P30CA021765]
  11. Howard Hughes Medical Institute
  12. Austrian Science Fund (Wittgenstein award)

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Analyses of protein complexes are facilitated by methods that enable the generation of recombinant complexes via coexpression of their subunits from multigene DNA constructs. However, low experimental throughput limits the generation of such constructs in parallel. Here we describe a method that allows up to 25 cDNAs to be assembled into a single baculoviral expression vector in only two steps. This method, called biGBac, uses computationally optimized DNA linker sequences that enable the efficient assembly of linear DNA fragments, using reactions developed by Gibson for the generation of synthetic genomes. The biGBac method uses a flexible and modular mix and match approach and enables the generation of baculoviruses from DNA constructs at any assembly stage. Importantly, it is simple, efficient, and fast enough to allow the manual generation of many multigene expression constructs in parallel. We have used this method to generate and characterize recombinant forms of the anaphase-promoting complex/cyclosome, cohesin, and kinetochore complexes.

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