AI Article Synopsis

  • A novel ethanol fermentation regulatory gene from a fast-growing yeast strain (MC15) was replaced in a high-yield strain (MF01) to boost ethanol production from sugarcane molasses.
  • The transfer of this gene resulted in the modified strain (MF01-PHO4) achieving a 5.30% increase in ethanol yield and a 12.5% reduction in fermentation time compared to the original strain MF01.
  • This research highlights the potential for targeted genetic modifications in yeast to enhance ethanol production efficiency in industrial applications.

Article Abstract

Replacement of a novel candidate ethanol fermentation-associated regulatory gene, , from a fast-growing strain MC15, as determined through comparative genomics analysis among three yeast strains with significant differences in ethanol yield, is hypothesised to shorten the fermentation time and enhance ethanol production from sugarcane molasses. This study sought to test this hypothesis through a novel strategy involving the transfer of the gene from a low ethanol-producing, yet fast-growing strain MC15 to a high ethanol-producing industrial strain MF01 through homologous recombination. The results indicated that in the industrially engineered strain MF01-PHO4 displayed genomic stability with a mean maximum ethanol yield that rose to 114.71 g L, accounting for a 5.30% increase in ethanol yield and 12.5% decrease in fermentation time in comparison with that in the original strain MF01, which was the current highest ethanol-producing strain in SCM fermentation in the reported literature. These results serve to advance our current understanding of the association between improving ethanol yield and replacement of , while providing a feasible strategy for industrially engineered yeast strains to improve ethanol production efficiently.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC9048610PMC
http://dx.doi.org/10.1039/c9ra08673kDOI Listing

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