The oleaginous yeast Yarrowia lipolytica is an emerging host for production of fatty acid-derived chemicals. To enable rapid iterative metabolic engineering of this yeast, there is a need for well-characterized genetic parts and convenient and reliable methods for their incorporation into yeast. Here, the EasyCloneYALI genetic toolbox, which allows streamlined strain construction with high genome editing efficiencies in Y. lipolytica via the CRISPR/Cas9 technology is presented. The toolbox allows marker-free integration of gene expression vectors into characterized genome sites as well as marker-free deletion of genes with the help of CRISPR/Cas9. Genome editing efficiencies above 80% were achieved with transformation protocols using non-replicating DNA repair fragments (such as DNA oligos). Furthermore, the toolbox includes a set of integrative gene expression vectors with prototrophic markers conferring resistance to hygromycin and nourseothricin.
Conferring
methylotrophy on industrial microorganisms would enable
the production of diverse products from one-carbon feedstocks and
contribute to establishing a low-carbon society. Rebuilding methylotrophs,
however, requires a thorough metabolic refactoring and is highly challenging.
Only recently was synthetic methylotrophy achieved in model microorganismsEscherichia coli and baker’s yeast Saccharomyces cerevisiae. Here, we have engineered
industrially important yeast Yarrowia lipolytica to assimilate methanol. Through rationally constructing a chimeric
assimilation pathway, rewiring the native metabolism for improved
precursor supply, and laboratory evolution, we improved the methanol
assimilation from undetectable to a level of 1.1 g/L per 72 h and
enabled methanol-supported cellular maintenance. By transcriptomic
analysis, we further found that fine-tuning of methanol assimilation
and ribulose monophosphate/xylulose monophosphate (RuMP/XuMP) regeneration
and strengthening formate dehydrogenation and the serine pathway were
beneficial for methanol assimilation. This work paves the way for
creating synthetic methylotrophic yeast cell factories for low-carbon
economy.
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