AI Article Synopsis

  • Eukaryotic microorganisms, like Aspergillus niger, convert l-arabinose to l-arabitol using a specific enzyme called l-arabinose reductase (larA), which is different from the enzyme for d-xylose, known as d-xylose reductase (xyrA).
  • The study found that larA is specifically up-regulated when l-arabinose is present, while xyrA is activated by d-xylose, although there is a temporary increase in larA expression when d-xylose is fed to the microorganism.
  • Deleting the larA gene slows growth on l-arabinose but does not affect growth on d-xylose, indicating that lar

Article Abstract

The first enzyme in the pathway for l-arabinose catabolism in eukaryotic microorganisms is a reductase, reducing l-arabinose to l-arabitol. The enzymes catalyzing this reduction are in general nonspecific and would also reduce d-xylose to xylitol, the first step in eukaryotic d-xylose catabolism. It is not clear whether microorganisms use different enzymes depending on the carbon source. Here we show that Aspergillus niger makes use of two different enzymes. We identified, cloned, and characterized an l-arabinose reductase, larA, that is different from the d-xylose reductase, xyrA. The larA is up-regulated on l-arabinose, while the xyrA is up-regulated on d-xylose. There is however an initial up-regulation of larA also on d-xylose but that fades away after about 4 h. The deletion of the larA gene in A. niger results in a slow growth phenotype on l-arabinose, whereas the growth on d-xylose is unaffected. The l-arabinose reductase can convert l-arabinose and d-xylose to their corresponding sugar alcohols but has a higher affinity for l-arabinose. The K(m) for l-arabinose is 54 + or - 6 mm and for d-xylose 155 + or - 15 mm.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC2911281PMC
http://dx.doi.org/10.1074/jbc.M110.113399DOI Listing

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