4.6 Article

Engineering Filamentous Fungi for Conversion of D-Galacturonic Acid to L-Galactonic Acid

期刊

APPLIED AND ENVIRONMENTAL MICROBIOLOGY
卷 78, 期 24, 页码 8676-8683

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AMER SOC MICROBIOLOGY
DOI: 10.1128/AEM.02171-12

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资金

  1. Academy of Finland under the Finish Centre of Excellence in White Biotechnology-Green Chemistry [118573]
  2. Academy of Finland under the research program Cadfiss [122131]
  3. Academy of Finland under the research program Sustainable Energy [131869]
  4. Academy of Finland (AKA) [131869, 131869, 122131, 122131] Funding Source: Academy of Finland (AKA)

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D-Galacturonic acid, the main monomer of pectin, is an attractive substrate for bioconversions, since pectin-rich biomass is abundantly available and pectin is easily hydrolyzed. L-Galactonic acid is an intermediate in the eukaryotic pathway for D-galacturonic acid catabolism, but extracellular accumulation of L-galactonic acid has not been reported. By deleting the gene encoding L-galactonic acid dehydratase (lgd1 or gaaB) in two filamentous fungi, strains were obtained that converted D-galacturonic acid to L-galactonic acid. Both Trichoderma reesei Delta lgd1 and Aspergillus niger Delta gaaB strains produced L-galactonate at yields of 0.6 to 0.9 g per g of substrate consumed. Although T. reesei Delta lgd1 could produce L-galactonate at pH 5.5, a lower pH was necessary for A. niger Delta gaaB. Provision of a cosubstrate improved the production rate and titer in both strains. Intracellular accumulation of L-galactonate (40 to 70 mg g biomass(-1)) suggested that export may be limiting. Deletion of the L-galactonate dehydratase from A. niger was found to delay induction of D-galacturonate reductase and overexpression of the reductase improved initial production rates. Deletion of the L-galactonate dehydratase from A. niger also delayed or prevented induction of the putative D-galacturonate transporter An14g04280. In addition, A. niger Delta gaaB produced L-galactonate from polygalacturonate as efficiently as from the monomer.

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