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Engineering glucose metabolism for enhanced muconic acid production in Pseudomonas putida KT2440.

Author information

Affiliations

  • 1. National Bioenergy Center, National Renewable Energy Laboratory, Golden, CO, 80401, USA.
      Authors
    • Bentley GJ 1
    • Salvachúa D 1
    • Black BA 1
    • Ramirez K 1
    • De Capite A 1
    • Michener WE 1
    • Werner AZ 1
    • Nelson R 1
    • Foust L 1
    • Johnson CW 1
    • Beckham GT 1
    (11 authors)
  • 2. Bioscience Division, MS M888, Los Alamos National Laboratory, Los Alamos, NM, 87545, USA.
      Authors
    • Narayanan N 2
    • Jha RK 2
    • Dale T 2
    (3 authors)
  • 3. Biosciences Division, Oak Ridge National Laboratory, Oak Ridge, TN, 37831, USA; Current Address: Biosciences Division, Pacific Northwest National Laboratory, Richland, WA, 99354, USA.
      Authors
    • Elmore JR 3
    (1 author)
  • 4. Biosciences Division, Oak Ridge National Laboratory, Oak Ridge, TN, 37831, USA.
      Authors
    • Peabody GL 4
    • Klingeman DM 4
    • Schindel HS 4
    • Guss AM 4
    (4 authors)

ORCIDs linked to this article

Metabolic Engineering, 10 Jan 2020, 59:64-75
https://doi.org/10.1016/j.ymben.2020.01.001 PMID: 31931111 

This article has been corrected. See Metab Eng. 2022 Jul;72:66-67.

Abstract 

Pseudomonas putida KT2440 has received increasing attention as an important biocatalyst for the conversion of diverse carbon sources to multiple products, including the olefinic diacid, cis,cis-muconic acid (muconate). P. putida has been previously engineered to produce muconate from glucose; however, periplasmic oxidation of glucose causes substantial 2-ketogluconate accumulation, reducing product yield and selectivity. Deletion of the glucose dehydrogenase gene (gcd) prevents 2-ketogluconate accumulation, but dramatically slows growth and muconate production. In this work, we employed adaptive laboratory evolution to improve muconate production in strains incapable of producing 2-ketogluconate. Growth-based selection improved growth, but reduced muconate titer. A new muconate-responsive biosensor was therefore developed to enable muconate-based screening using fluorescence activated cell sorting. Sorted clones demonstrated both improved growth and muconate production. Mutations identified by whole genome resequencing of these isolates indicated that glucose metabolism may be dysregulated in strains lacking gcd. Using this information, we used targeted engineering to recapitulate improvements achieved by evolution. Deletion of the transcriptional repressor gene hexR improved strain growth and increased the muconate production rate, and the impact of this deletion was investigated using transcriptomics. The genes gntZ and gacS were also disrupted in several evolved clones, and deletion of these genes further improved strain growth and muconate production. Together, these targets provide a suite of modifications that improve glucose conversion to muconate by P. putida in the context of gcd deletion. Prior to this work, our engineered strain lacking gcd generated 7.0 g/L muconate at a productivity of 0.07 g/L/h and a 38% yield (mol/mol) in a fed-batch bioreactor. Here, the resulting strain with the deletion of hexR, gntZ, and gacS achieved 22.0 g/L at 0.21 g/L/h and a 35.6% yield (mol/mol) from glucose in similar conditions. These strategies enabled enhanced muconic acid production and may also improve production of other target molecules from glucose in P. putida.

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Read article at publisher's site: https://doi.org/10.1016/j.ymben.2020.01.001

Read article for free, from open access legal sources, via Unpaywall: http://manuscript.elsevier.com/S1096717619303994/pdf/S1096717619303994.pdfUnpaywall

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Bioenergy Technologies Office